Your search keyword '"Camillo Almici"' showing total 80 results

1. Allogeneic Solid Platelet-Rich Plasma for Persistent Epithelial Neurotrophic Defects: A Protocol and Pilot Study

Author

Vito Romano, Stefano Bignotti, Eliana Forbice, Andrea Bianchetti, Camillo Almici, and Francesco Semeraro

Subjects

fibrin glue, persistent epithelial defect, Ophthalmology, contact lens, fibrin glue, persistent epithelial defect, platelet-rich plasma, neurotrophic keratopathy, contact lens, neurotrophic keratopathy, platelet-rich plasma

Published

2022

2. Supplementary Figures from Collapse of the Plasmacytoid Dendritic Cell Compartment in Advanced Cutaneous Melanomas by Components of the Tumor Cell Secretome

Author

William Vermi, Fabio Facchetti, Ausilia Manganoni, Paolo Bergese, Aldo Scarpa, Rosanna Verardi, Camillo Almici, Michele Simbolo, Camillo Farisoglio, Ester Fonsatti, Michele Maio, Mattia Bugatti, Giulio Rossi, Mariella Chiudinelli, Stefano Calza, Laura Melocchi, Luisa Benerini, Francesca Consoli, Lucia Paolini, Daniele Moratto, Matilde Monti, and Raffaella Vescovi

Abstract

Supplementary Figures

Published

2023

3. Data from Collapse of the Plasmacytoid Dendritic Cell Compartment in Advanced Cutaneous Melanomas by Components of the Tumor Cell Secretome

Author

William Vermi, Fabio Facchetti, Ausilia Manganoni, Paolo Bergese, Aldo Scarpa, Rosanna Verardi, Camillo Almici, Michele Simbolo, Camillo Farisoglio, Ester Fonsatti, Michele Maio, Mattia Bugatti, Giulio Rossi, Mariella Chiudinelli, Stefano Calza, Laura Melocchi, Luisa Benerini, Francesca Consoli, Lucia Paolini, Daniele Moratto, Matilde Monti, and Raffaella Vescovi

Abstract

Melanoma is an immunogenic neoplasm infiltrated by T cells, although these adaptive T cells usually fail to eradicate the tumor. Plasmacytoid dendritic cells (PDCs) are potent regulators of the adaptive immune response and can eliminate melanoma cells via TLR-mediated effector functions. The PDC compartment is maintained by progressively restricted bone marrow progenitors. Terminally differentiated PDCs exit the bone marrow into the circulation, then home to lymph nodes and inflamed peripheral tissues. Infiltration by PDCs is documented in various cancers. However, their role within the melanoma immune contexture is not completely known. We found that in locoregional primary cutaneous melanoma (PCM), PDC infiltration was heterogeneous, occurred early, and was recurrently localized at the invasive margin, the site where PDCs interact with CD8+ T cells. A reduced PDC density was coupled with an increased Breslow thickness and somatic mutations at the NRAS p.Q61 codon. Compared with what was seen in PCM, high numbers of PDCs were found in regional lymph nodes, as also identified by in silico analysis. In contrast, in metastatic melanoma patients, PDCs were mostly absent in the tumor tissues and were significantly reduced in the circulation, particularly in the advanced M1c group. Exposure of circulating PDCs to melanoma cell supernatant (SN-mel) depleted of extracellular vesicles resulted in significant PDC death. SN-mel exposure also resulted in a defect of PDC differentiation from CD34+ progenitors. These findings indicate that soluble components released by melanoma cells support the collapse of the PDC compartment, with clinical implications for refining TLR agonist–based trials.

Published

2023

4. Supplementary Tables from Collapse of the Plasmacytoid Dendritic Cell Compartment in Advanced Cutaneous Melanomas by Components of the Tumor Cell Secretome

Author

William Vermi, Fabio Facchetti, Ausilia Manganoni, Paolo Bergese, Aldo Scarpa, Rosanna Verardi, Camillo Almici, Michele Simbolo, Camillo Farisoglio, Ester Fonsatti, Michele Maio, Mattia Bugatti, Giulio Rossi, Mariella Chiudinelli, Stefano Calza, Laura Melocchi, Luisa Benerini, Francesca Consoli, Lucia Paolini, Daniele Moratto, Matilde Monti, and Raffaella Vescovi

Abstract

Supplementary tables

Published

2023

5. The role of clonal hematopoiesis as driver of therapy-related myeloid neoplasms after autologous stem cell transplantation

Author

Doriana Gramegna, Diego Bertoli, Chiara Cattaneo, Camillo Almici, Alessandro Re, Angelo Belotti, Erika Borlenghi, Gaetana Lanzi, Silvana Archetti, Rosanna Verardi, Duilio Brugnoni, Margherita Sciumè, Rosa Daffini, Aldo M. Roccaro, Alessandra Tucci, and Giuseppe Rossi

Subjects

Myeloproliferative Disorders, Core Binding Factor Alpha 2 Subunit, Mutation, Hematopoietic Stem Cell Transplantation, Humans, Neoplasms, Second Primary, Hematology, General Medicine, Clonal Hematopoiesis, Transplantation, Autologous, Hematopoiesis

Abstract

Therapy-related myeloid neoplasm (t-MN) is a threatening complication of autologous stem cell transplantation (ASCT). Detecting clonal hematopoiesis (CH) mutations in cryopreserved cells before ASCT has been associated with a higher risk of t-MN, but the evolution of molecular abnormalities from pre-ASCT to t-MN, within the same patient, remains to be elucidated. We evaluated the mutational profile of 19 lymphoma/myeloma patients, at both pre-ASCT and t-MN diagnosis, using a targeted NGS approach; 26 non-developing t-MN control patients were also studied pre-ASCT. At ASCT, we found a higher frequency of CH in patients developing t-MN (58%) than in those who did not (23%) (P = 0.029); mutations in epigenetic (DNMT3A, TET2, and ASXL1) and DNA repair genes (PPM1D, RAD21, TP53, and STAG2) were the most represented. At t-MN, CH increased to 82% of patients. Cumulative mutational burden and variant allele frequency (VAF) also increased at t-MN. CH clones detected at ASCT were found at t-MN in eight out of 16 patients, mainly with stable VAF. Among the new driver mutations appeared at t-MN, TP53 increased from one to 13 mutations, in nine patients; being associated with complex karyotype. Mutations in transcription factor (RUNX1, CEBPA) and intracellular signaling genes (FLT3, RAS genes) also increased from three to 17 mutations in eight patients, presenting with a normal karyotype. Overall, we found that preexisting CH at ASCT rarely causes t-MN directly, but may rather facilitate the appearance of new mutations, especially those involving TP53, RUNX1, and RAS, that can drive the evolution to t-MN of at least two distinct types.

Published

2022

6. Targeting the immune microenvironment in Waldenström Macroglobulinemia via halting the CD40/CD40-ligand axis

Author

Antonio Sacco, Vanessa Desantis, Jon Celay, Viviana Giustini, Fabio Rigali, Francesco D Savino, Michele Cea, Debora Soncini, Antonia Cagnetta, Antonio Giovanni Solimando, Deborah D'Aliberti, Silvia Spinelli, Daniele Ramazzotti, Camillo Almici, Katia Todoerti, Antonino Neri, Antonella Anastasia, Alessandra Tucci, Marina Motta, Marco Chiarini, Yawara Kawano, Jose-Al Martinez-Climent, Rocco Piazza, Aldo M Roccaro, Sacco, A, Desantis, V, Celay, J, Giustini, V, Rigali, F, Savino, F, Cea, M, Soncini, D, Cagnetta, A, Solimando, A, D'Aliberti, D, Spinelli, S, Ramazzotti, D, Almici, C, Todoerti, K, Neri, A, Anastasia, A, Tucci, A, Motta, M, Chiarini, M, Kawano, Y, Martinez-Climent, J, Piazza, R, and Roccaro, A

Subjects

Immunology, Cell Biology, Hematology, Waldenström Macroglobulinemia, Biochemistry

Abstract

Recent investigations have improved our understanding of the molecular aberrations supporting Waldenström macroglobulinemia (WM) biology; however, whether the immune microenvironment contributes to WM pathogenesis remains unanswered. First, we showed how a transgenic murine model of human-like lymphoplasmacytic lymphoma/WM exhibits an increased number of regulatory T cells (Tregs) relative to control mice. These findings were translated into the WM clinical setting, in which the transcriptomic profiling of Tregs derived from patients with WM unveiled a peculiar WM-devoted messenger RNA signature, with significant enrichment for genes related to nuclear factor κB–mediated tumor necrosis factor α signaling, MAPK, and PI3K/AKT, which was paralleled by a different Treg functional phenotype. We demonstrated significantly higher Treg induction, expansion, and proliferation triggered by WM cells, compared with their normal cellular counterpart; with a more profound effect within the context of CXCR4C1013G-mutated WM cells. By investigating the B-cell–to–T-cell cross talk at single-cell level, we identified the CD40/CD40-ligand as a potentially relevant axis that supports WM cell–Tregs interaction. Our findings demonstrate the existence of a Treg-mediated immunosuppressive phenotype in WM, which can be therapeutically reversed by blocking the CD40L/CD40 axis to inhibit WM cell growth.

Published

2023

7. High risk-myelodysplastic syndrome following CAR T-cell therapy in a patient with relapsed diffuse large B cell lymphoma: A case report and literature review

Author

Eugenia Accorsi Buttini, Mirko Farina, Luisa Lorenzi, Nicola Polverelli, Vera Radici, Enrico Morello, Federica Colnaghi, Camillo Almici, Emilio Ferrari, Andrea Bianchetti, Alessandro Leoni, Federica Re, Katia Bosio, Simona Bernardi, Michele Malagola, Alessandro Re, and Domenico Russo

Subjects

next generation sequencing, Cancer Research, Oncology, CAR T-cell therapy, clonal hematopoiesis, diffuse large B cell lymphoma, myelodysplastic syndrome

Abstract

BackgroundChimeric antigen receptor (CAR) T-cell therapy represents the most advanced immunotherapy against relapsed/refractory B cell malignancies. While cytokine release syndrome and immune effector cell-associated neurotoxicity syndrome are distinctive, known CAR T-cell acute adverse events, hematological toxicity has been increasingly reported. Cytopenia following CAR T-cell treatment is attributed in most cases to lymphodepletion regimens, bridging chemotherapy, or radiotherapy. However, when cytopenia becomes prolonged, the development of myelodysplastic syndrome (MDS) should be considered.Case presentationWe report a case of high risk (HR)-MDS following CAR T-cell therapy in a patient with relapsed diffuse large B cell lymphoma. Eight months after CAR T-cell infusion, the blood count showed progressive, worsening cytopenia and the bone marrow biopsy revealed multilineage dysplasia without excess of blasts associated with chromosome 7 deletion and RUNX1 mutation. Next generation sequencing analysis, retrospectively performed on stored samples, showed a germ line CSF3R mutation, CEBPA clonal hematopoiesis, but no RUNX1 lesion.ConclusionWe describe a case of HR-MDS, with deletion of chromosome 7 and acquisition of RUNX1 mutation, developing after CAR T-cell therapy in a patient with clonal hematopoiesis (CH). Previous chemotherapy favored MDS onset; however, we could not exclude the fact that the impairment of immunosurveillance related to either lymphodepletion or CAR T-cell infusion may play a role in MDS development. Thus, we designed a multicenter prospective study (ClonHema-CAR-T-Study) to investigate if cytopenia after CAR T-cell treatment may be due to underling CH as well as the presence of secondary myeloid malignancies.

Published

2023

8. Timely Leukapheresis May Interfere with the 'Fitness' of Lymphocytes Collected for CAR-T Treatment in High Risk DLBCL Patients

Author

Mirko Farina, Marco Chiarini, Camillo Almici, Eugenia Accorsi Buttini, Francesco Zuccalà, Simone Piva, Irene Volonghi, Loris Poli, Simona Bernardi, Federica Colnaghi, Federica Re, Alessandro Leoni, Nicola Polverelli, Alessandro Turra, Enrico Morello, Anna Galvagni, Daniele Moratto, Duilio Brugnoni, Chiara Cattaneo, Emilio Ferrari, Andrea Bianchetti, Michele Malagola, Alessandro Re, and Domenico Russo

Subjects

Cancer Research, Oncology, pre-emptive lymphocytoapheresis, CAR-T, Lymphocytes fitness, T-cells repertoire

Abstract

The development of chimeric antigen receptor (CAR)-T cell therapy has revolutionized the treatment of hematological diseases. However, approximately 60% of patients relapse after CAR-T cell therapy, and no clear cause for this failure has been identified. The objective of the Bio-CAR-T BS study (ClinicalTrials.gov: NCT05366569) is to improve our understanding of the lymphocyte harvest to maximize the quality of the CAR-T cell product. Of the 14 patients enrolled, 11 were diagnosed with DLBCL, 2 with PMBCL, and 1 with ALL. Five of 11 DLBCL patients met the criteria for “pre-emptive” Lymphocytes-apheresis (being at high risk of second relapse), and 6 were included in the standard-of-care Lymphocytes-apheresis group. Previous autologous stem cell transplantation (ASCT) and age were significantly different between the two groups. At the time of Lymphocyte-apheresis, patients in the “pre-emptive” group had more “fit” lymphocytes (higher CD4+/CD8+ ratio; higher naïve T cells levels) compared with standard group, probably due to the impact of ASCT. At the same time, also being older than 60 years results in a more “exhausted” lymphocyte profile. Overall, “pre-emptive” Ly-apheresis in DLBCL patients at high risk of relapse appears to be feasible and may allow the timely collection of “fit” lymphocytes for CAR-T cell manufacturing.

Published

2022

9. HLA class I and HPA9b related fetal-neonatal alloimmune thrombocytopenia

Author

Sara Barbieri, Alessandro Copeta, Nicoletta Revelli, Alberto Malagoli, Alessia Montani, Enrico Sartori, Camillo Almici, Federico Prefumo, and Susanna Bresciani

Subjects

Thrombocytopenia, Neonatal Alloimmune, Fetus, Histocompatibility Antigens Class I, Infant, Newborn, Humans, Antigens, Human Platelet, Hematology

Published

2021

10. Comparative Mutational Profiling of Hematopoietic Progenitor Cells and Circulating Endothelial Cells (CECs) in Patients with Primary Myelofibrosis

Author

Mariella D'Adda, Andrew Dunbar, Michele Malagola, Federica Re, Katia Bosio, Simona Bernardi, Ross L. Levine, Domenico Russo, Camillo Almici, Mirko Farina, and Nicola Polverelli

Subjects

Male, circulating endothelial cells, Somatic cell, QH301-705.5, CD34, Antigens, CD34, myelofibrosis, medicine.disease_cause, vascular biology-endothelial cells, Article, hematopoiesis-stem and primitive progenitor cells, molecular genetics, Precursor cell, medicine, Humans, Progenitor cell, Biology (General), Myelofibrosis, Aged, Laser capture microdissection, Mutation, business.industry, Endothelial Cells, High-Throughput Nucleotide Sequencing, General Medicine, Hematopoietic Stem Cells, medicine.disease, Haematopoiesis, Primary Myelofibrosis, Case-Control Studies, Cancer research, cardiovascular system, Female, business

Abstract

A role of endothelial cells (ECs) in Primary Myelofibrosis (PMF) was supposed since JAK2 mutation was found in endothelial precursor cells (EPCs) and in ECs captured by laser microdissection. By Cell Search method, the circulating endothelial cells (CECs) from 14 PMF patients and 5 healthy controls have been isolated and compared by NGS with CD34+Hematopoietic stem and progenitors cells (HSPCs) for panel of 54 myeloid-associated mutations. PMF patients had higher levels of CECs. No mutation was found in HSPCs and CECs from controls, while CECs from PMF patients presented several somatic mutations. 72% of evaluable patients shared at least one mutation between HSPCs and CECs. 2 patients shared the JAK2 mutation, together with ABL1, IDH1, TET2 and ASXL1, KMT2A, respectively. 6 out of 8 shared only NON MPN-driver mutations: TET2 and NOTCH1 in one case, individual paired mutations in TP53, KIT, SRSF2, NOTCH1 and WT1, in the other cases. In conclusion, 70% of PMF patients shared at least one mutation between HSPCs and CECs. These latter harbored several myeloid-associated mutations, besides JAK2V617F mutation. Our results support a primary involvement of EC in PMF and provide a new methodological approach for further studies exploring the role of the “neoplastic” vascular niche.

Published

2021

11. Chitosan‐based scaffold counteracts hypertrophic and fibrotic markers in chondrogenic differentiated mesenchymal stromal cells

Author

Cristina Manferdini, Kamol Dey, Gina Lisignoli, Silvia Agnelli, Erminia Mariani, Andrea Bianchetti, Nicoletta Zini, Federica Re, Domenico Russo, Camillo Almici, Luciana Sartore, Elena Gabusi, Manferdini C., Gabusi E., Sartore L., Dey K., Agnelli S., Almici C., Bianchetti A., Zini N., Russo D., Re F., Mariani E., and Lisignoli G.

Subjects

Scaffold, Swine, Medicine (miscellaneous), 02 engineering and technology, Chitosan, chemistry.chemical_compound, chondrogenic differentiation, fibrotic marker, 0303 health sciences, Tissue Scaffolds, Hydrolysis, stress relaxation, fibrotic markers, Cell Differentiation, Hydrogels, Cell biology, medicine.anatomical_structure, mesenchymal stromal cell, mesenchymal stromal cells, Chondrogenesis, chitosan scaffold, human platelet lysate, hypertrophic markers, Animals, Biomarkers, Bone Marrow Cells, Cell Proliferation, Chondrocytes, Collagen Type II, Fibrosis, Hypertrophy, Mesenchymal Stem Cells, Stress, Mechanical, 0206 medical engineering, Biomedical Engineering, SOX9, Stress, Biomaterials, 03 medical and health sciences, medicine, Aggrecan, 030304 developmental biology, hypertrophic marker, Cartilage, Mesenchymal stem cell, Mechanical, 020601 biomedical engineering, In vitro, chemistry

Abstract

Cartilage tissue engineering remains problematic because no systems are able to induce signals that contribute to native cartilage structure formation. Therefore, we tested the potentiality of gelatin-polyethylene glycol scaffolds containing three different concentrations of chitosan (CH; 0%, 8%, and 16%) on chondrogenic differentiation of human platelet lysate-expanded human bone marrow mesenchymal stromal cells (hBM-MSCs). Typical chondrogenic (SOX9, collagen type 2, and aggrecan), hypertrophic (collagen type 10), and fibrotic (collagen type 1) markers were evaluated at gene and protein level at Days 1, 28, and 48. We demonstrated that 16% CH scaffold had the highest percentage of relaxation with the fastest relaxation rate. In particular, 16% CH scaffold, combined with chondrogenic factor TGFβ3, was more efficient in inducing hBM-MSCs chondrogenic differentiation compared with 0% or 8% scaffolds. Collagen type 2, SOX9, and aggrecan showed the same expression in all scaffolds, whereas collagen types 10 and 1 markers were efficiently down-modulated only in 16% CH. We demonstrated that using human platelet lysate chronically during hBM-MSCs chondrogenic differentiation, the chondrogenic, hypertrophic, and fibrotic markers were significantly decreased. Our data demonstrate that only a high concentration of CH, combined with TGFβ3, creates an environment capable of guiding in vitro hBM-MSCs towards a phenotypically stable chondrogenesis.

Published

2019

12. Collapse of the Plasmacytoid Dendritic Cell Compartment in Advanced Cutaneous Melanomas by Components of the Tumor Cell Secretome

Author

Mattia Bugatti, Ausilia Maria Manganoni, Matilde Monti, Camillo Almici, Aldo Scarpa, Ester Fonsatti, Francesca Consoli, Michele Maio, Luisa Benerini, Giulio Rossi, Daniele Moratto, Fabio Facchetti, Paolo Bergese, Rosanna Verardi, Raffaella Vescovi, Stefano Calza, William Vermi, Camillo Farisoglio, Michele Simbolo, Mariella Chiudinelli, Lucia Paolini, and Laura Melocchi

Subjects

Adult, Male, Proto-Oncogene Proteins B-raf, EXPRESSION, RECRUITMENT, 0301 basic medicine, Cancer Research, Skin Neoplasms, Immunology, CD34, MICROENVIRONMENT, Plasmacytoid dendritic cell, Biology, EARLY MARKER, Proto-Oncogene Proteins p21(ras), Young Adult, 03 medical and health sciences, 0302 clinical medicine, Immune system, medicine, Humans, Melanoma, Aged, LACTATE-DEHYDROGENASE, Aged, 80 and over, LACTIC-ACID, CUTTING EDGE, LYMPH-NODES, hemic and immune systems, Dendritic Cells, Middle Aged, Acquired immune system, medicine.disease, PD-1 BLOCKADE, 030104 developmental biology, medicine.anatomical_structure, 030220 oncology & carcinogenesis, Cutaneous melanoma, Disease Progression, Cancer research, Female, Bone marrow, Chemokines, Sentinel Lymph Node, RESPONSES, CD8

Abstract

Melanoma is an immunogenic neoplasm infiltrated by T cells, although these adaptive T cells usually fail to eradicate the tumor. Plasmacytoid dendritic cells (PDCs) are potent regulators of the adaptive immune response and can eliminate melanoma cells via TLR-mediated effector functions. The PDC compartment is maintained by progressively restricted bone marrow progenitors. Terminally differentiated PDCs exit the bone marrow into the circulation, then home to lymph nodes and inflamed peripheral tissues. Infiltration by PDCs is documented in various cancers. However, their role within the melanoma immune contexture is not completely known. We found that in locoregional primary cutaneous melanoma (PCM), PDC infiltration was heterogeneous, occurred early, and was recurrently localized at the invasive margin, the site where PDCs interact with CD8+ T cells. A reduced PDC density was coupled with an increased Breslow thickness and somatic mutations at the NRAS p.Q61 codon. Compared with what was seen in PCM, high numbers of PDCs were found in regional lymph nodes, as also identified by in silico analysis. In contrast, in metastatic melanoma patients, PDCs were mostly absent in the tumor tissues and were significantly reduced in the circulation, particularly in the advanced M1c group. Exposure of circulating PDCs to melanoma cell supernatant (SN-mel) depleted of extracellular vesicles resulted in significant PDC death. SN-mel exposure also resulted in a defect of PDC differentiation from CD34+ progenitors. These findings indicate that soluble components released by melanoma cells support the collapse of the PDC compartment, with clinical implications for refining TLR agonist–based trials.

Published

2019

13. A Blood Bank Standardized Production of Human Platelet Lysate for Mesenchymal Stromal Cell Expansion: Proteomic Characterization and Biological Effects

Author

Michele Guindani, Camillo Almici, Rosanna Verardi, Andrea Bianchetti, Simona Braga, Giovanna Piovani, Fulvio Magni, Gina Lisignoli, Arabella Neva, Clizia Chinello, Domenico Russo, Lisa Pagani, Bianchetti, A, Chinello, C, Guindani, M, Braga, S, Neva, A, Verardi, R, Piovani, G, Pagani, L, Lisignoli, G, Magni, F, Russo, D, and Almici, C

Subjects

0301 basic medicine, Chemokine, Stromal cell, QH301-705.5, human platelet lysate, blood banks standards, 030204 cardiovascular system & hematology, growth factors, mass spectrometry, mesenchymal stromal cells, Cell therapy, Andrology, Cell and Developmental Biology, 03 medical and health sciences, 0302 clinical medicine, Methods, Doubling time, Platelet, Biology (General), Whole blood, biology, Chemistry, Mesenchymal stem cell, growth factor, Cell Biology, 030104 developmental biology, mesenchymal stromal cell, blood banks standard, biology.protein, Fetal bovine serum, Developmental Biology

Abstract

Human platelet lysate (hPL) is considered a valid substitute to fetal bovine serum (FBS) in the expansion of mesenchymal stromal cells (MSC), and it is commonly produced starting from intermediate side products of whole blood donations. Through freeze–thaw cycles, hPL is highly enriched in chemokines, growth factors, and adhesion and immunologic molecules. Cell therapy protocols, using hPL instead of FBS for the expansion of cells, are approved by regulatory authorities without concerns, and its administration in patients is considered safe. However, published data are fairly difficult to compare, since the production of hPL is highly variable. This study proposes to optimize and standardize the hPL productive process by using instruments, technologies, and quality/safety standards required for blood bank activities and products. The quality and improved selection of the starting material (i.e., the whole blood), together with the improvement of the production process, guarantee a product characterized by higher content and quality of growth factors as well as a reduction in batch-to-batch variability. By increasing the number of freeze/thaw cycles from one (hPL1c) to four (hPL4c), we obtained a favorable effect on the release of growth factors from platelet α granules. Those changes have directly translated into biological effects leading to a decreasing doubling time (DT) of MSC expansion at 7 days (49.41 ± 2.62 vs. 40.61 ± 1.11 h, p < 0.001). Furthermore, mass spectrometry (MS)-based evaluation has shown that the proliferative effects of hPL4c are also combined with a lower batch-to-batch variability (10–15 vs. 21–31%) at the proteomic level. In conclusion, we have considered lot-to-lot hPL variability, and by the strict application of blood bank standards, we have obtained a standardized, reproducible, safe, cheap, and ready-to-use product.

Published

2021

14. Mineralization of 3D Osteogenic Model Based on Gelatin-Dextran Hybrid Hydrogel Scaffold Bioengineered with Mesenchymal Stromal Cells: A Multiparametric Evaluation

Author

Fulvio Magni, Camillo Almici, Pierangelo Guizzi, Kamol Dey, Elisa Borsani, Luciana Sartore, Andrew Smith, Simona Bernardi, Federica Re, Allia Mahajneh, Camilla Baratto, Matteo Ferroni, Domenico Russo, and Guido Faglia

Subjects

Technology, Scaffold, food.ingredient, human platelet lysate, 02 engineering and technology, macromolecular substances, Gelatin, Article, MALDI-MS, Extracellular matrix, 03 medical and health sciences, chemistry.chemical_compound, food, medicine, General Materials Science, bone regeneration hydrogel scaffold, mesenchymal stromal cells, Raman spectroscopy, 030304 developmental biology, Microscopy, QC120-168.85, 0303 health sciences, Chemistry, QH201-278.5, Mesenchymal stem cell, technology, industry, and agriculture, Mineralization (soil science), Engineering (General). Civil engineering (General), 021001 nanoscience & nanotechnology, TK1-9971, Dextran, medicine.anatomical_structure, Descriptive and experimental mechanics, Biophysics, Electrical engineering. Electronics. Nuclear engineering, Bone marrow, TA1-2040, 0210 nano-technology, Fetal bovine serum

Abstract

Gelatin–dextran hydrogel scaffolds (G-PEG-Dx) were evaluated for their ability to activate the bone marrow human mesenchymal stromal cells (BM-hMSCs) towards mineralization. G-PEG-Dx1 and G-PEG-Dx2, with identical composition but different architecture, were seeded with BM-hMSCs in presence of fetal bovine serum or human platelet lysate (hPL) with or without osteogenic medium. G-PEG-Dx1, characterized by a lower degree of crosslinking and larger pores, was able to induce a better cell colonization than G-PEG-Dx2. At day 28, G-PEG-Dx2, with hPL and osteogenic factors, was more efficient than G-PEG-Dx1 in inducing mineralization. Scanning electron microscopy (SEM) and Raman spectroscopy showed that extracellular matrix produced by BM-hMSCs and calcium-positive mineralization were present along the backbone of the G-PEG-Dx2, even though it was colonized to a lesser degree by hMSCs than G-PEG-Dx1. These findings were confirmed by matrix-assisted laser desorption/ionization mass spectrometry imaging (MALDI-MSI), detecting distinct lipidomic signatures that were associated with the different degree of scaffold mineralization. Our data show that the architecture and morphology of G-PEG-Dx2 is determinant and better than that of G-PEG-Dx1 in promoting a faster mineralization, suggesting a more favorable and active role for improving bone repair.

Published

2021

15. Chitosan-Hydrogel Polymeric Scaffold Acts as an Independent Primary Inducer of Osteogenic Differentiation in Human Mesenchymal Stromal Cells

Author

Simona Bernardi, Domenico Russo, Katia Bosio, Michele Malagola, Kamol Dey, Pierangelo Guizzi, Camillo Almici, Luciana Sartore, and Federica Re

Subjects

endocrine system, osteopontin, scaffold, hydrogel, chitosan, regenerative medicine, osteogenic differentiation, digital PCR, Adipose tissue, 02 engineering and technology, lcsh:Technology, Regenerative medicine, Article, 03 medical and health sciences, medicine, General Materials Science, Inducer, Osteopontin, lcsh:Microscopy, lcsh:QC120-168.85, 030304 developmental biology, 0303 health sciences, lcsh:QH201-278.5, biology, lcsh:T, Chemistry, Mesenchymal stem cell, 021001 nanoscience & nanotechnology, Regenerative process, equipment and supplies, Cell biology, medicine.anatomical_structure, lcsh:TA1-2040, biology.protein, lcsh:Descriptive and experimental mechanics, lcsh:Electrical engineering. Electronics. Nuclear engineering, Bone marrow, lcsh:Engineering (General). Civil engineering (General), 0210 nano-technology, lcsh:TK1-9971, Fetal bovine serum

Abstract

Regenerative medicine aims to restore damaged tissues and mainly takes advantage of human mesenchymal stromal cells (hMSCs), either alone or combined with three-dimensional scaffolds. The scaffold is generally considered a support, and its contribution to hMSC proliferation and differentiation is unknown or poorly investigated. The aim of this study was to evaluate the capability of an innovative three-dimensional gelatin&ndash, chitosan hybrid hydrogel scaffold (HC) to activate the osteogenic differentiation process in hMSCs. We seeded hMSCs from adipose tissue (AT-hMSCs) and bone marrow (BM-hMSCs) in highly performing HC of varying chitosan content in the presence of growing medium (GM) or osteogenic medium (OM) combined with Fetal Bovine Serum (FBS) or human platelet lysate (hPL). We primarily evaluated the viability and the proliferation of AT-hMSCs and BM-hMSCs under different conditions. Then, in order to analyse the activation of osteogenic differentiation, the osteopontin (OPN) transcript was absolutely quantified at day 21 by digital PCR. OPN was expressed under all conditions, in both BM-hMSCs and AT-hMSCs. Cells seeded in HC cultured with OM+hPL presented the highest OPN transcript levels, as expected. Interestingly, both BM-hMSCs and AT-hMSCs cultured with GM+FBS expressed OPN. In particular, BM-hMSCs cultured with GM+FBS expressed more OPN than those cultured with GM+hPL and OM+FBS, AT-hMSCs cultured with GM+FBS presented a lower expression of OPN when compared with those cultured with GM+hPL, but no significant difference was detected when compared with AT-hMSCs cultured with OM+FBS. No OPN expression was detected in negative controls. These results show the capability of HC to primarily and independently activate osteogenic differentiation pathways in hMCSs. Therefore, these scaffolds may be considered no more as a simple support, rather than active players in the differentiative and regenerative process.

Published

2020

16. Polysaccharides on gelatin-based hydrogels differently affect chondrogenic differentiation of human mesenchymal stromal cells

Author

Domenico Russo, Cristina Manferdini, Gina Lisignoli, Luciana Sartore, Kamol Dey, Erminia Mariani, Elena Gabusi, Federica Re, Giorgio Ramorino, Nicoletta Zini, Camillo Almici, and Yasmin Saleh

Subjects

food.ingredient, Materials science, Bioengineering, macromolecular substances, 02 engineering and technology, 010402 general chemistry, 01 natural sciences, Gelatin, Biomaterials, Chitosan, chemistry.chemical_compound, food, Tissue engineering, Stress relaxing hydrogel, medicine, Humans, Cartilage, Mesenchymal stem cell, technology, industry, and agriculture, Cell Differentiation, Hydrogels, Mesenchymal Stem Cells, 021001 nanoscience & nanotechnology, Chondrogenesis, 0104 chemical sciences, medicine.anatomical_structure, chemistry, Cartilage regeneration, Chitosan/dextran-based scaffold, Human mesenchymal stromal cells, Mechanics of Materials, Self-healing hydrogels, Biophysics, 0210 nano-technology, Ethylene glycol

Abstract

Selection of feasible hybrid-hydrogels for best chondrogenic differentiation of human mesenchymal stromal cells (hMSCs) represents an important challenge in cartilage regeneration. In this study, three-dimensional hybrid hydrogels obtained by chemical crosslinking of poly (ethylene glycol) diglycidyl ether (PEGDGE), gelatin (G) without or with chitosan (Ch) or dextran (Dx) polysaccharides were developed. The hydrogels, namely G-PEG, G-PEG-Ch and G-PEG-Dx, were prepared with an innovative, versatile and cell-friendly technique that involves two preparation steps specifically chosen to increase the degree of crosslinking and the physical-mechanical stability of the product: a first homogeneous phase reaction followed by directional freezing, freeze-drying and post-curing. Chondrogenic differentiation of human bone marrow mesenchymal stromal cells (hBM-MSC) was tested on these hydrogels to ascertain whether the presence of different polysaccharides could favor the formation of the native cartilage structure. We demonstrated that the hydrogels exhibited an open pore porous morphology with high interconnectivity and the incorporation of Ch and Dx into the G-PEG common backbone determined a slightly reduced stiffness compared to that of G-PEG hydrogels. We demonstrated that G-PEG-Dx showed a significant increase of its anisotropic characteristic and G-PEG-Ch exhibited higher and faster stress relaxation behavior than the other hydrogels. These characteristics were associated to absence of chondrogenic differentiation on G-PEG-Dx scaffold and good chondrogenic differentiation on G-PEG and G-PEG-Ch. Furthermore, G-PEG-Ch induced the minor collagen proteins and the formation of collagen fibrils with a diameter like native cartilage. This study demonstrated that both anisotropic and stress relaxation characteristics of the hybrid hydrogels were important features directly influencing the chondrogenic differentiation potentiality of hBM-MSC.

Published

2021

17. 3D gelatin-chitosan hybrid hydrogels combined with human platelet lysate highly support human mesenchymal stem cell proliferation and osteogenic differentiation

Author

Domenico Russo, Luigi Fabrizio Rodella, Fabio Savoldi, Cristina Manferdini, Gina Lisignoli, Kamol Dey, Luciana Sartore, Manuel Salmerón-Sánchez, Silvia Agnelli, Simona Bernardi, Vladimira Moulisova, Corrado Paganelli, Andrea Bianchetti, Fulvio Magni, Nicola Lopomo, Emilio Sardini, Federica Re, Camillo Almici, Marco Cantini, Elisa Borsani, Clizia Chinello, Pierangelo Guizzi, Re, F, Sartore, L, Moulisova, V, Cantini, M, Almici, C, Bianchetti, A, Chinello, C, Dey, K, Agnelli, S, Manferdini, C, Bernardi, S, Lopomo, N, Sardini, E, Borsani, E, Rodella, L, Savoldi, F, Paganelli, C, Guizzi, P, Lisignoli, G, Magni, F, Salmeron-Sanchez, M, and Russo, D

Subjects

food.ingredient, human platelet lysate, Biomedical Engineering, Medicine (miscellaneous), Adipose tissue, macromolecular substances, 02 engineering and technology, Gelatin, lcsh:Biochemistry, Biomaterials, human mesenchymal stem cells, 03 medical and health sciences, food, bone regeneration, Tissue engineering, human mesenchymal stem cell, medicine, lcsh:QD415-436, Mesenchymal stem cell proliferation, Bone regeneration, 030304 developmental biology, 0303 health sciences, Hybrid chitosan-gelatin hydrogel, tissue engineering, Chemistry, Mesenchymal stem cell, technology, industry, and agriculture, 021001 nanoscience & nanotechnology, 3. Good health, Cell biology, carbohydrates (lipids), medicine.anatomical_structure, Self-healing hydrogels, Original Article, Bone marrow, 0210 nano-technology

Abstract

Bone marrow and adipose tissue human mesenchymal stem cells were seeded in highly performing 3D gelatin–chitosan hybrid hydrogels of varying chitosan content in the presence of human platelet lysate and evaluated for their proliferation and osteogenic differentiation. Both bone marrow and adipose tissue human mesenchymal stem cells in gelatin–chitosan hybrid hydrogel 1 (chitosan content 8.1%) or gelatin–chitosan hybrid hydrogel 2 (chitosan 14.9%) showed high levels of viability (80%–90%), and their proliferation and osteogenic differentiation was significantly higher with human platelet lysate compared to fetal bovine serum, particularly in gelatin–chitosan hybrid hydrogel 1. Mineralization was detected early, after 21 days of culture, when human platelet lysate was used in the presence of osteogenic stimuli. Proteomic characterization of human platelet lysate highlighted 59 proteins mainly involved in functions related to cell adhesion, cellular repairing mechanisms, and regulation of cell differentiation. In conclusion, the combination of our gelatin–chitosan hybrid hydrogels with hPL represents a promising strategy for bone regenerative medicine using human mesenchymal stem cells.

Published

2019

18. The clinical use of circulating tumor cells (CTCs) enumeration for staging of metastatic breast cancer (MBC): International expert consensus paper

Author

Salvatore Grisanti, Tanja Fehm, Daniele Generali, Jean-Yves Pierga, Dimitrios Mavroudis, Mario Giuliano, Leticia De Mattos-Arruda, Steven Van Laere, Lorenzo Gerratana, Francesca Consoli, Wolfgang Janni, Klaus Pantel, Luc Dirix, Stefan Michiels, Carlos Caldas, Annemie Rutten, Jorge S. Reis-Filho, Michail Ignatiadis, Dieter Peeters, Andrew M. Davis, Sarah-Jane Dawson, Jose Vidal-Martinez, Cristina Raimondi, Massimo Cristofanilli, Alfred Rademaker, Maria Teresa Sandri, Justin Stebbing, Rita Zamarchi, Franziska Meier-Stiegen, Elisabetta Munzone, Jonathan Krell, Vicente Carañana, Erich-Franz Solomayer, Laura Zorzino, Franco Nolè, Paola Gazzaniga, Eduardo Díaz-Rubio, Lauren Darrigues, Luc Cabel, Rafael Gisbert-Criado, Eleni Politaki, Sofia Agelaki, José A. García-Sáenz, Angela Fernandez de Lascoiti, Maria Rosa Cappelletti, Camillo Almici, Luis Manso, François-Clément Bidard, James M. Reuben, Cristofanilli, Massimo, Pierga, Jean-Yve, Reuben, Jame, Rademaker, Alfred, Davis, Andrew A., Peeters, Dieter J., Fehm, Tanja, Nolé, Franco, Gisbert-Criado, Rafael, Mavroudis, Dimitrio, Grisanti, Salvatore, Giuliano, Mario, Garcia-Saenz, Jose A., Stebbing, Justin, Caldas, Carlo, Gazzaniga, Paola, Manso, Lui, Zamarchi, Rita, de Lascoiti, Angela Fernandez, De Mattos-Arruda, Leticia, Ignatiadis, Michail, Cabel, Luc, van Laere, Steven J., Meier-Stiegen, Franziska, Sandri, Maria-Teresa, Vidal-Martinez, Jose, Politaki, Eleni, Consoli, Francesca, Generali, Daniele, Cappelletti, Maria Rosa, Diaz-Rubio, Eduardo, Krell, Jonathan, Dawson, Sarah-Jane, Raimondi, Cristina, Rutten, Annemie, Janni, Wolfgang, Munzone, Elisabetta, Carañana, Vicente, Agelaki, Sofia, Almici, Camillo, Dirix, Luc, Solomayer, Erich-Franz, Zorzino, Laura, Darrigues, Lauren, Reis-Filho, Jorge S., Gerratana, Lorenzo, Michiels, Stefan, Bidard, François-Clément, Pantel, Klaus, Cristofanilli, M., Pierga, J. -Y., Reuben, J., Rademaker, A., Davis, A. A., Peeters, D. J., Fehm, T., Nole, F., Gisbert-Criado, R., Mavroudis, D., Grisanti, S., Giuliano, M., Garcia-Saenz, J. A., Stebbing, J., Caldas, C., Gazzaniga, P., Manso, L., Zamarchi, R., de Lascoiti, A. F., De Mattos-Arruda, L., Ignatiadis, M., Cabel, L., van Laere, S. J., Meier-Stiegen, F., Sandri, M. -T., Vidal-Martinez, J., Politaki, E., Consoli, F., Generali, D., Cappelletti, M. R., Diaz-Rubio, E., Krell, J., Dawson, S. -J., Raimondi, C., Rutten, A., Janni, W., Munzone, E., Caranana, V., Agelaki, S., Almici, C., Dirix, L., Solomayer, E. -F., Zorzino, L., Darrigues, L., Reis-Filho, J. S., Gerratana, L., Michiels, S., Bidard, F. -C., and Pantel, K.

Subjects

0301 basic medicine, Oncology, Survival, biomarker, Neoplastic Cells, 0302 clinical medicine, Circulating tumor cell, Biomarker, Circulating tumor cells, CTCs, MBC, Metastatic breast cancer, Biomarkers, Tumor, Breast Neoplasms, Consensus, Expert Testimony, Female, Humans, International Agencies, Neoplasm Staging, Neoplastic Cells, Circulating, Patient Selection, Circulating, Stage (cooking), MB, Triple-negative breast cancer, Tumor, Hematology, International Agencie, 030220 oncology & carcinogenesis, metastatic breast cancer, Breast Neoplasm, Human, medicine.medical_specialty, Consensu, circulating tumor cell, survival, 03 medical and health sciences, Internal medicine, medicine, Survival analysis, Tumor marker, Cancer staging, business.industry, medicine.disease, CTC, Clinical trial, 030104 developmental biology, circulating tumor cells, Human medicine, business, Biomarkers

Abstract

Background: The heterogeneity of metastatic breast cancer (MBC) necessitates novel biomarkers allowing stratification of patients for treatment selection and drug development. We propose to use the prognostic utility of circulating tumor cells (CTCs) for stratification of patients with stage IV disease. Methods: In a retrospective, pooled analysis of individual patient data from 18 cohorts, including 2436 MBC patients, a CTC threshold of 5 cells per 7.5 ml was used for stratification based on molecular subtypes, disease location, and prior treatments. Patients with >= 5 CTCs were classified as Stage IVaggresive, those with < 5 CTCs as Stage IVindolent. Survival was analyzed using Kaplan-Meier curves and the log rank test. Results: For all patients, Stage IVindolent patients had longer median overall survival than those with Stage IVaggresive (36.3 months vs. 16.0 months, P < 0.0001) and similarly for de novo MBC patients (41.4 months Stage IVindolent vs. 18.7 months Stage IVaggresive p < 0.0001). Moreover, patients with Stage IVindolent disease had significantly longer overall survival across all disease subtypes compared to the aggressive cohort: hormone receptor-positive (44 months vs. 17.3 months, P < 0.0001), HER2-positive (36.7 months vs. 20.4 months, P < 0.0001), and triple negative (23.8 months vs. 9.0 months, P < 0.0001). Similar results were obtained regardless of prior treatment or disease location. Conclusions: We confirm the identification of two subgroups of MBC, Stage IVindolent and Stage IVaggresive, independent of clinical and molecular variables. Thus, CTC count should be considered an important tool for staging of advanced disease and for disease stratification in prospective clinical trials.

Published

2019

19. Counting circulating endothelial cells in allo-HSCT: an ad hoc designed polychromatic flowcytometry-based panel versus the CellSearch System

Author

Gianluca Rotta, Kurt Baeten, Andrea Bianchetti, Domenico Russo, Mirella Marini, Simona Braga, Paola Omedè, Benedetto Bruno, Valeria Cancelli, Andrea Di Palma, Arabella Neva, Rosanna Verardi, Giovanna Piovani, Cristina Skert, and Camillo Almici

Subjects

0301 basic medicine, Oncology, medicine.medical_specialty, medicine.medical_treatment, Allo hsct, Graft vs Host Disease, lcsh:Medicine, Hematopoietic stem cell transplantation, Article, 03 medical and health sciences, 0302 clinical medicine, Hematologic disorders, Internal medicine, medicine, Humans, Transplantation, Homologous, Bland–Altman plot, lcsh:Science, Blood Cells, Multidisciplinary, business.industry, lcsh:R, Limits of agreement, Hematopoietic Stem Cell Transplantation, Endothelial Cells, Flow Cytometry, Clinical routine, Transplantation, surgical procedures, operative, 030104 developmental biology, lcsh:Q, business, 030217 neurology & neurosurgery

Abstract

Physio-pathologic interrelationships between endothelial layer and graft-versus-host disease (GVHD) have been described leading to assess the entity “endothelial GVHD” as the early step for clinical manifestations of acute GVHD. The availability of the CellSearch system has allowed us to monitor Circulating Endothelial Cells (CEC) changes in allogeneic hematopoietic stem cell transplantation (allo-HSCT) as useful tool to help clinicians in GVHD diagnostic definition. We have compared CEC counts generated by an ad hoc designed polychromatic-flowcytometry (PFC) Lyotube with those of the CellSearch system. CEC were counted in parallel at 5 timepoints in 50 patients with malignant hematologic disorders undergoing allo-HSCT (ClinicalTrials.gov, NCT02064972). Spearman rank correlation showed significant association between CEC values at all time points (p = 0.0001). The limits of agreement was demonstrated by Bland Altman plot analysis, showing bias not significant at T1, T3, T4, while at T2 and T5 resulted not estimable. Moreover, Passing Bablok regression analysis showed not significant differences between BD Lyotube and CellSearch system. We show that CEC counts, generated with either the CellSearch system or the PFC-based panel, have a superimposable kinetic in allo-HSCT patients and that both counting procedures hold the potential to enter clinical routine as a suitable tool to assist clinicians in GVHD diagnosis.

Published

2019

20. Abstract P2-08-08: Circulating tumor cells count-based nomograms to predict survival of metastatic breast cancer patients: Results from the European pooled analysis

Author

Pierre Squifflet, S Sleijfers, D Peeters, Jorge S. Reis-Filho, A Fernandez de Lascoiti, Camillo Almici, Salvatore Grisanti, Daniele Generali, Nick Beije, Cristina Raimondi, L. De Mattos-Arruda, Carlos Caldas, J-Y Pierga, L.Y. Dirix, D. Mavroudis, Alberto Bottini, Pier Paolo Gazzaniga, Wolfgang Janni, F-C Bidard, Stefan Michiels, Jonathan Krell, Jose Vidal-Martinez, Rita Zamarchi, S-J Dawson, Laura Zorzino, Annemie Rutten, Franco Nolè, Sophia Agelaki, Francesca Consoli, JA Garcia-Saenz, Michail Ignatiadis, S. Van Laere, Elisabetta Munzone, Rafael Gisbert-Criado, E Solomayer, Eleni Politaki, M. T. Sandri, Eduardo Díaz-Rubio, Luis Manso, Justin Stebbing, Klaus Pantel, Tanja Fehm, Vicente Carañana, and Franziska Meier-Stiegen

Subjects

Oncology, Cancer Research, medicine.medical_specialty, business.industry, Cancer, Nomogram, medicine.disease, Metastatic breast cancer, Surgery, Breast cancer, Pooled analysis, Circulating tumor cell, Internal medicine, Cohort, medicine, business, Prognostic models

Abstract

Background: The European Pooled Analysis of CTC (EPAC) in metastatic breast cancer, based on 1,944 individual data from patients with various tumor types and clinical settings (Bidard et al, Lancet Oncol 2014), has established CTC count (CellSearch) at baseline and during therapy as a level of evidence 1 independent prognostic biomarker and demonstrated its superiority over serum blood markers. As part of the study pre-planned objectives, we sought to establish nomograms allowing accurate individual survival predictions. Methods: Using individual data from 17 centers, we built simplified multivariate prognostic models taking into account the independent prognostic clinico-pathological (CP) characteristics including CTC count, dichotomized using the 5CTC/7.5ml threshold, at baseline and at 3-5 weeks after the start of a new treatment regimen, and derived nomograms for progression-free survival (PFS) and overall survival (OS) prediction at baseline and after 3-5 weeks of treatment. We report here the internal validation of these nomograms. Discrimination of the models was assessed using the c-index estimated by a jackknife procedure and the calibration was visually assessed through 10-fold crossvalidated calibration plots at 1,2,3 years for OS and 1,2 years for PFS. Results: Multivariate models at baseline for PFS and OS were fitted on 1501 and 568 individual patient data with CTC count at baseline and CTC count at baseline and after 3-5 weeks, respectively. Models include tumor subtype, the number of previous chemotherapy lines (0/1/≥2), PS, age (50-65/>65 years), metastasis-free intervals (0/>0-3/>3 years), metastatic sites (liver and CNS) and CTC count at baseline and eventually at 3-5 weeks of treatment. The C-index increased from 0.722 to 0.755 (increase in C-index:0.033, 95% CI [0.019;0.045]) when adding baseline CTC to the CP only model for OS (n=1501). For those patients with CTC values at 3-5 weeks (n=568), there was an additional increase in the C-index when adding CTC at 3-5 weeks to a model with already CP and baseline CTC from 0.731 to 0.743 (increase in C-index 0.013, 95% CI [-0.004;0.025]). The model with CP and baseline CTC counts showed a good calibration for OS at 1,2,3 years and the model with CP, baseline CTC and CTC count at 3-5 weeks a moderately good calibration. Similar results were obtained for PFS. Conclusion: From the largest database with individual CTC data, we were able to build PFS and OS survival nomograms, with satisfactory discrimination and calibration. Our planned next step is to validate the nomogram in an additional cohort. Citation Format: Bidard F-C, Peeters D, Fehm T, Nole F, Gisbert-Criado R, Mavroudis D, Grisanti S, Generali D, Garcia-Saenz JA, Stebbing J, Caldas C, Gazzaniga P, Manso L, Zamarchi R, Fernandez de Lascoiti A, de Mattos-Arruda L, Ignatiadis M, van Laere SJ, Meier-Stiegen F, Sandri M-T, Vidal-Martinez J, Politaki E, Consoli F, Bottini A, Diaz-Rubio E, Krell J, Dawson S-J, Raimondi C, Rutten A, Janni W, Munzone E, Carañana V, Agelaki S, Almici C, Dirix L, Solomayer E, Zorzino L, Reis-Filho JS, Squifflet P, Pantel K, Beije N, Sleijfers S, Pierga J-Y, Michiels S. Circulating tumor cells count-based nomograms to predict survival of metastatic breast cancer patients: Results from the European pooled analysis. [abstract]. In: Proceedings of the Thirty-Eighth Annual CTRC-AACR San Antonio Breast Cancer Symposium: 2015 Dec 8-12; San Antonio, TX. Philadelphia (PA): AACR; Cancer Res 2016;76(4 Suppl):Abstract nr P2-08-08.

Published

2016

21. Impedance-Based Monitoring of Mesenchymal Stromal Cell Three-Dimensional Proliferation Using Aerosol Jet Printed Sensors: A Tissue Engineering Application

Author

Luciana Sartore, Federica Re, Kamol Dey, Nicola Lopomo, Mauro Serpelloni, Giovanna Piovani, Emilio Sardini, Michele Guindani, Andrea Bianchetti, Simona Braga, Edoardo Cantu, Camillo Almici, Mirella Marini, Sarah Tonello, and Domenico Russo

Subjects

Scaffold, Stromal cell, Materials science, Bioengineering, 02 engineering and technology, lcsh:Technology, Capacitance, Article, aerosol jet printing, 03 medical and health sciences, Engineering, Tissue engineering, General Materials Science, lcsh:Microscopy, Electrical impedance, lcsh:QC120-168.85, 030304 developmental biology, 0303 health sciences, lcsh:QH201-278.5, lcsh:T, Mesenchymal stem cell, Phase angle, 021001 nanoscience & nanotechnology, 3D monitoring, lcsh:TA1-2040, impedance-based cell spectroscopy, tissue engineering, Aerosol jet printing, Impedance-based cell spectroscopy, Mesenchymal stromal cells, Chemical Sciences, lcsh:Descriptive and experimental mechanics, lcsh:Electrical engineering. Electronics. Nuclear engineering, lcsh:Engineering (General). Civil engineering (General), mesenchymal stromal cells, 0210 nano-technology, lcsh:TK1-9971, Polyimide, Biotechnology, Biomedical engineering

Abstract

One of the main hurdles to improving scaffolds for regenerative medicine is the development of non-invasive methods to monitor cell proliferation within three-dimensional environments. Recently, an electrical impedance-based approach has been identified as promising for three-dimensional proliferation assays. A low-cost impedance-based solution, easily integrable with multi-well plates, is here presented. Sensors were developed using biocompatible carbon-based ink on foldable polyimide substrates by means of a novel aerosol jet printing technique. The setup was tested to monitor the proliferation of human mesenchymal stromal cells into previously validated gelatin-chitosan hybrid hydrogel scaffolds. Reliability of the methodology was assessed comparing variations of the electrical impedance parameters with the outcomes of enzymatic proliferation assay. Results obtained showed a magnitude increase and a phase angle decrease at 4 kHz (maximum of 2.5 kΩ and &minus, 9 degrees) and an exponential increase of the modeled resistance and capacitance components due to the cell proliferation (maximum of 1.5 kΩ and 200 nF). A statistically significant relationship with enzymatic assay outcomes could be detected for both phase angle and electric model parameters. Overall, these findings support the potentiality of this non-invasive approach for continuous monitoring of scaffold-based cultures, being also promising in the perspective of optimizing the scaffold-culture system.

Published

2020

22. A standardized flow cytometry network study for the assessment of circulating endothelial cell physiological ranges

Author

Gianluca Rotta, Paola Lanuti, Elena Di Gennaro, Natalia Malara, Alfredo Budillon, Mirella Marini, Pasquale Mastroroberto, Valentina Trunzo, Francesca Losa, Silvia Pinna, Maria Cristina Tirindelli, Marco Marchisio, Paolo Doretto, Alessandra Falda, Emma Muggianu, Lorenza Scotti, Camillo Almici, Giuseppe Musolino, Annamaria Diodato, Carlo Vitagliano, Laura Pierdomenico, Fulvio Zullo, Rosa Azzaro, Sebastiano Miscia, María Roca, Melania Di Cerbo, Domenico Russo, Chiara Gregorj, Michele Morelli, Vincenzo Mollace, Arabella Neva, Giovanna Piovani, Pasquale Simeone, Giuseppe Avvisati, Eva Ercolino, Alessandra Leone, Roberta Venturella, Maria Luisa Di Martino, Giuseppina Bologna, Lanuti, P, Simeone, P, Rotta, G, Almici, C, Avvisati, G, Azzaro, R, Bologna, G, Budillon, A, Di Cerbo, M, Di Gennaro, E, Di Martino, M, Diodato, A, Doretto, P, Ercolino, E, Falda, A, Gregorj, C, Leone, A, Losa, F, Malara, N, Marini, M, Mastroroberto, P, Mollace, V, Morelli, M, Muggianu, E, Musolino, G, Neva, A, Pierdomenico, L, Pinna, S, Piovani, G, Roca, M, Russo, D, Scotti, L, Tirindelli, M, Trunzo, V, Venturella, R, Vitagliano, C, Zullo, F, Marchisio, M, Miscia, S, Lanuti, Paola, Simeone, Pasquale, Rotta, Gianluca, Almici, Camillo, Avvisati, Giuseppe, Azzaro, Rosa, Bologna, Giuseppina, Budillon, Alfredo, Di Cerbo, Melania, Di Gennaro, Elena, Di Martino, Maria Luisa, Diodato, Annamaria, Doretto, Paolo, Ercolino, Eva, Falda, Alessandra, Gregorj, Chiara, Leone, Alessandra, Losa, Francesca, Malara, Natalia, Marini, Mirella, Mastroroberto, Pasquale, Mollace, Vincenzo, Morelli, Michele, Muggianu, Emma, Musolino, Giuseppe, Neva, Arabella, Pierdomenico, Laura, Pinna, Silvia, Piovani, Giovanna, Roca, Maria Serena, Russo, Domenico, Scotti, Lorenza, Tirindelli, Maria Cristina, Trunzo, Valentina, Venturella, Roberta, Vitagliano, Carlo, Zullo, Fulvio, Marchisio, Marco, and Miscia, Sebastiano

Subjects

Adult, Male, 0301 basic medicine, Median Fluorescence Intensity, Circulating endothelial cell, Science, Large population, Cell Separation, Biology, Sensitivity and Specificity, Article, Flow cytometry, Andrology, Young Adult, 03 medical and health sciences, Reference Values, medicine, Humans, High potential, Multidisciplinary, medicine.diagnostic_test, Healthy population, Endothelial Cells, Hematology, Middle Aged, Flow Cytometry, Healthy Volunteers, Peripheral blood, Blood Cell Count, 030104 developmental biology, Biological Variation, Population, cardiovascular system, Feasibility Studies, Medicine, Female, Endothelium, Vascular, Laboratories, Biological variability

Abstract

Circulating endothelial cells (CEC) represent a restricted peripheral blood (PB) cell subpopulation with high potential diagnostic value in many endothelium-involving diseases. However, whereas the interest in CEC studies has grown, the standardization level of their detection has not. Here, we undertook the task to align CEC phenotypes and counts, by standardizing a novel flow cytometry approach, within a network of six laboratories. CEC were identified as alive/nucleated/CD45negative/CD34bright/CD146positive events and enumerated in 269 healthy PB samples. Standardization was demonstrated by the achievement of low inter-laboratory Coefficients of Variation (CVL), calculated on the basis of Median Fluorescence Intensity values of the most stable antigens that allowed CEC identification and count (CVL of CD34bright on CEC ~ 30%; CVL of CD45 on Lymphocytes ~ 20%). By aggregating data acquired from all sites, CEC numbers in the healthy population were captured (medianfemale = 9.31 CEC/mL; medianmale = 11.55 CEC/mL). CEC count biological variability and method specificity were finally assessed. Results, obtained on a large population of donors, demonstrate that the established procedure might be adopted as standardized method for CEC analysis in clinical and in research settings, providing a CEC physiological baseline range, useful as starting point for their clinical monitoring in endothelial dysfunctions.

Published

2018

23. Endothelial progenitor cells, defined by the simultaneous surface expression of VEGFR2 and CD133, are not detectable in healthy peripheral and cord blood

Author

Sebastiano Miscia, Pasquale Simeone, Giuseppe Avvisati, Valentina Trunzo, Camillo Almici, Vincenzo Mollace, Arabella Neva, Elena Di Gennaro, Marco Marchisio, Natalia Malara, Alfredo Budillon, Mirella Marini, Renato Tozzoli, Alessandra Leone, Chiara Gregorj, Paolo Doretto, Melania Di Cerbo, Gianluca Rotta, Alessandra Falda, and Paola Lanuti

Subjects

0301 basic medicine, Histology, medicine.diagnostic_test, CD34, Hematopoietic stem cell, Cell Biology, Biology, Molecular biology, Pathology and Forensic Medicine, Flow cytometry, 03 medical and health sciences, 030104 developmental biology, medicine.anatomical_structure, Antigen, Cord blood, Immunology, cardiovascular system, medicine, CD146, Bone marrow, Progenitor cell, circulatory and respiratory physiology

Abstract

Circulating endothelial cells (CEC) and their progenitors (EPC) are restricted subpopulations of peripheral blood (PB), cord blood (CB), and bone marrow (BM) cells, involved in the endothelial homeostasis maintenance. Both CEC and EPC are thought to represent potential biomarkers in several clinical conditions involving endothelial turnover/remodeling. Although different flow cytometry methods for CEC and EPC characterization have been published so far, none of them have reached consistent conclusions, therefore consensus guidelines with respect to CEC and EPC identification and quantification need to be established. Here, we have carried out an in depth investigation of CEC and EPC phenotypes in healthy PB, CB and BM samples, by optimizing a reliable polychromatic flow cytometry (PFC) panel. Results showed that the brightness of CD34 expression on healthy PB and CB circulating cells represents a key benchmark for the identification of CEC (CD45neg/CD34bright/CD146pos) respect to the hematopoietic stem cell (HSC) compartment (CD45dim/CD34pos/CD146neg). This approach, combined with a dual-platform counting technique, allowed a sharp CEC enumeration in healthy PB (n = 38), and resulting in consistent CEC counts with previously reported data (median = 11.7 cells/ml). In parallel, by using rigorous PFC conditions, CD34pos/CD45dim/CD133pos/VEGFR2pos EPC were not found in any healthy PB or CB sample, since VEGFR2 expression was never detectable on the surface of CD34pos/CD45dim/CD133pos cells. Notably, the putative EPC phenotype was observed in all analyzed BM samples (n = 12), and the expression of CD146 and VEGFR2, on BM cells, was not restricted to the CD34bright compartment, but also appeared on the HSC surface. Altogether, our findings suggest that the previously reported EPC antigen profile, defined by the simultaneous expression of VEGFR2 and CD133 on the surface of CD45dim/CD34pos cells, should be carefully re-evaluated and further studies should be conducted to redefine EPC features in order to translate CEC and EPC characterization into clinical practice.

Published

2015

24. Early consolidation with high-dose therapy and autologous stem cell transplantation is a feasible and effective treatment option in HIV-associated non-Hodgkin lymphoma at high risk

Author

Mariagrazia Michieli, Paola Tozzi, Cristina Skert, A. Levis, P. F Leali, Michele Spina, Camillo Almici, Maurizio Rupolo, Umberto Tirelli, Caterina Bocci, Alessandro Re, Cristina Cattaneo, Alessandra Bandera, Giorgio Rossi, Luisa Verga, Guido Gini, Salvatore Casari, Anna Marina Liberati, and Bernardino Allione

Subjects

0301 basic medicine, Oncology, Adult, Male, medicine.medical_specialty, autologous stem cell transplantation, Adolescent, hiv, Non Hodgkin's lymphoma, autologous stem cell transplantation, Human immunodeficiency virus (HIV), hiv, HIV Infections, medicine.disease_cause, Transplantation, Autologous, 03 medical and health sciences, Young Adult, 0302 clinical medicine, Autologous stem-cell transplantation, immune system diseases, hemic and lymphatic diseases, Internal medicine, Medicine, Effective treatment, Humans, Transplantation, business.industry, Lymphoma, Non-Hodgkin, Hematology, Middle Aged, medicine.disease, Lymphoma, Non-Hodgkin's lymphoma, Consolidation Chemotherapy, Non Hodgkin's lymphoma, 030104 developmental biology, High dose therapy, 030220 oncology & carcinogenesis, Hodgkin lymphoma, Female, business

Abstract

Early consolidation with high-dose therapy and autologous stem cell transplantation is a feasible and effective treatment option in HIV-associated non-Hodgkin lymphoma at high risk

Published

2017

25. Bacterial Blood Stream Infections Negatively Impact on Outcome of Patients Treated with Allogeneic Stem Cell Transplantation: 6 Years Single-Centre Experience

Author

Michele, Malagola, Bendetta, Rambaldi, Giuseppe, Ravizzola, Chiara, Cattaneo, Erika, Borlenghi, Nicola, Polverelli, Alessandro, Turra, Enrico, Morello, Cristina, Skert, Valeria, Cancelli, Federica, Cattina, Giorgio, Giannetta, Simona, Bernardi, Simone, Perucca, Camillo, Almici, Aldo, Roccaro, Liana, Signorini, Roberto, Stellini, Francesco, Castelli, Arnaldo, Caruso, and Domenico, Russo

Subjects

medicine.medical_specialty, Gram-negative bacteria, Gram-positive bacteria, 030501 epidemiology, 03 medical and health sciences, 0302 clinical medicine, Antibiotic resistance, bone marrow transplantation,bacterial infections, antimicrobical resistance, Internal medicine, Epidemiology, medicine, biology, business.industry, lcsh:RC633-647.5, Incidence (epidemiology), Hematology, lcsh:Diseases of the blood and blood-forming organs, biology.organism_classification, Surgery, Transplantation, Infectious Diseases, 030220 oncology & carcinogenesis, Cohort, Coagulase, 0305 other medical science, business

Abstract

Background : Blood stream infections (BSIs) represent a major complication of allo-SCT and are a major cause of morbidity and mortality during and after bone marrow aplasia. Objectives: The objective of this study was to describe the incidence and outcome of BSIs in a cohort of patients submitted to allo-SCT, in order to track changes of the epidemiology and bacteria resistance. Methods : We retrospectively analyzed the microbiological data of 162 patients allotransplanted in Brescia University Hospital, over a period of 6 years. Results : Eighty patients experienced a BSIs for a total of 119 isolates. In 77 cases (65%) a Gram positive bacteria was isolated, being coagulase negative Staphilococci the most frequent species (77% of the cases). In 42 cases (35%) a Gram negative bacteria was isolated (E. coli 57% and P. aeruginosa 24%). Fluoroquinolones resistance was frequent (90% for S. epidermidis , 92% for E. coli , 90% for P. aeruginosa ). Methycillin resistance of S. epidermidis was 100%, 76% of E. coli were ESBL positive and among P. aeruginosa resistance to carbapenems was 40%. The 2 years overall survival of patients with BSIs vs patients without BSIs was 46% vs 60% (HR1,48, p=0,07). P. areuginosa and E. coli were the species with the highest mortality (50% and 33%, respectively). Conclusions : These data confirms that BSIs, mainly sustained by Gram positive bacteria, are frequent in allotransplanted patients (50% of the cases) and may influence the outcome of allotransplanted patients, being antibiotics resistance highly frequent among these bacteria.

Published

2017

26. PBSC mobilization in lymphoma patients: analysis of risk factors for collection failure and development of a predictive score based on the kinetics of circulating CD34+ cells and WBC after chemotherapy and G-CSF mobilization

Author

Lara Cavalli, Claudia Basilico, Gianluca Gaidano, Gianmatteo Pica, Flavia Salvi, Andrea Castelli, Luca Arcaini, Barbara Botto, Camillo Almici, Giuseppe Rossi, Annamaria Nosari, Domenico Russo, Francesco Ripamonti, Umberto Vitolo, Alessandro Levis, Enrico Morello, Cristina Skert, and Angelo Michele Carella

Subjects

Oncology, Cancer Research, medicine.medical_specialty, Chemotherapy, Mobilization, business.industry, medicine.medical_treatment, Hematology, General Medicine, Filgrastim, medicine.disease, Lymphoma, Surgery, Granulocyte colony-stimulating factor, medicine.anatomical_structure, Autologous stem-cell transplantation, White blood cell, Internal medicine, medicine, business, Hematopoietic Stem Cell Mobilization, medicine.drug

Abstract

Autologous stem cell transplantation (ASCT) is a potentially curative treatment of lymphoma, but peripheral blood stem cell (PBSC) mobilization fails in some patients. PBSC mobilizing agents have recently been proved to improve the PBSC yield after a prior mobilization failure. Predictive parameters of mobilization failure allowing for a preemptive, more cost-effective use of such agents during the first mobilization attempt are still poorly defined, particularly during mobilization with chemotherapy + granulocyte colony-stimulating factor (G-CSF). We performed a retrospective analysis of a series of lymphoma patients who were candidates for ASCT, to identify factors influencing PBSC mobilization outcome. Premobilization parameters-age, histology, disease status, mobilizing protocol, and previous treatments-as well as white blood cell (WBC) and PBSC kinetics, markers potentially able to predict failure during the ongoing mobilization attempt, were analyzed in 415 consecutive mobilization procedures in 388 patients. We used chemotherapy + G-CSF in 411 (99%) of mobilization attempts and PBSC collection failed (

Published

2014

27. Single Cell Analysis of Circulating Endothelial Cells in Allogeneic Hematopoietic Stem Cell Transplant; To Whom Do They Belong: Host or Donor?

Author

Cristina Skert, Rosanna Verardi, Giovanna Piovani, Andrea Bianchetti, Simona Braga, Nicolò Manaresi, Piera Balzarini, Mirella Marini, Francesca Fontana, Camillo Almici, Domenico Russo, Gianluca Rotta, Simona Fisogni, Fabio Facchetti, Benedetto Bruno, Michele Malagola, and Arabella Neva

Subjects

medicine.medical_specialty, medicine.diagnostic_test, Circulating endothelial cell, business.industry, medicine.medical_treatment, Immunology, Context (language use), Cell Biology, Hematology, Hematopoietic stem cell transplantation, medicine.disease, Biochemistry, Organ transplantation, Transplantation, Haematopoiesis, surgical procedures, operative, Graft-versus-host disease, Biopsy, cardiovascular system, medicine, business

Abstract

Background. We recently reported that Circulating Endothelial Cell (CEC) count changes represent a promising marker to monitor endothelial damage in patients undergoing allogeneic hematopoietic stem cell transplant (allo-HSCT), potentially becoming a valuable tool in the diagnostic definition of GVHD. Besides confirming an increase of CEC counts at GVHD onset, we repeatedly documented at time of engraftment statistically significant higher numbers of CEC in patients who will not manifest GVHD in comparison to patients in which GVHD will be diagnosed (Transplantation 2014,98:706-12; Bone Marrow Transplantation 2017,52:1637-42; Scientific Reports 2019,9:1-12). Recent knowledges in organ transplant pointed out that endothelial cells from the grafted organ, besides being a continuous source of alloantigens, can downregulate alloreactivity exerting tolerogenic responses. By inference to the allo-HSCT field, it could be envisaged that presence of donor CEC could induce protective effects on alloreactivity. Methods. We planned a study to test the hypothesis that at time of engraftment, CEC present in peripheral blood (PB), besides coming from cells shedding from patient vasculature, could partly belong to donor, originating from the cellular graft. Therefore, in an exploratory set, we performed FISH analysis on flowcytometry-sorted CEC (CD45neg/CD34bright/CD146pos, Lyotube #623920, BD Biosciences) (n=3) and on whole PB derived culture-expanded CEC (n=3) (EGM-2 BulletKit, Lonza), obtained at engraftment in sex-mismatched allo-HSCT. In the confirmatory set (n=15), single CEC were recovered from PB, at engraftment (T1) and at 90 days (T2) after allo-HSCT, through the DEPArrayTM technology (Menarini Silicon Biosystems), after preliminary bulk separation step carried out with the CellSearch® System. Single recovered CEC was whole genome amplified (Ampli1™ WGA Kit) and short tandem repeat (STR) profile determined (Ampli 1TM STR kit) on each single CEC. To confirm host/donor origin, single CEC STR profile was compared to that determined on patient and donor cells before allo-HSCT. Moreover, donor CEC presence was evaluated by CISH analysis on formaline fixed and paraffin-embedded biopsy sections obtained at least three months after sex mismatched allo-HSCT. Results. By positive findings of the exploratory set, we proved, at the single cell level in the confirmatory set, the presence of donor CEC at engraftment (T1) in 4 out of 15 patients (Table 1). Of them, 2 did not manifested GVHD, despite a GVHD risk score of 2, and the other 2 presented GVHD grade I. On the contrary, among the 10 patients in whom no donor CEC were detected, 6 experienced GVHD grade II-III, while 4 did not manifested GVHD, despite a 1-3 GVHD risk score. Conclusions. Our data represent the proof of principle that donor CEC may flow in host PB early on from hematopoietic recovery and seldom persist thereafter at steady-state conditions, being potentially embedded in host vascular wall. These puzzling findings suggest that neovascularization takes place in parallel with hematopoietic engraftment and could provide further clues on shedding light on tissue tolerance in the context of GVHD, opening up paradoxical scenarios on the protective role potentially played by donor CEC. Disclosures Fontana: Menarini Silicon Biosystem: Employment. Rotta:BD Biosciences Italia: Employment. Manaresi:Menarini SIlicon Biosystem: Employment, Membership on an entity's Board of Directors or advisory committees.

Published

2019

28. P4-07-19: Bone Marrow Involvement Is Associated with High Numbers of Circulating Tumor Cells in Peripheral Blood of Metastatic Breast Cancer Patients

Author

Rebecca Pedersini, Edda Simoncini, M Ungari, Francesca Consoli, R. Verardi, Salvatore Grisanti, Camillo Almici, F Bertagna, Lucia Vassalli, Vito Amoroso, and E Montani

Subjects

Oncology, Cancer Research, medicine.medical_specialty, Pathology, Lung, medicine.diagnostic_test, Bone disease, business.industry, Cancer, medicine.disease, Metastatic breast cancer, medicine.anatomical_structure, Circulating tumor cell, Bone scintigraphy, Internal medicine, Biopsy, medicine, Bone marrow, business

Abstract

Introduction: Circulating Tumor Cells (CTCs) levels are dynamic indicators of prognosis and response to therapy in metastatic breast cancer (MBC) patients (pts). CTCs levels have been reported to be higher in pts with bone than visceral metastases, respectively. However, little is known about CTCs levels in pts with BM involvement. We analysed CTC patterns in patients with either visceral, bone or BM to test the hypothesis that BM involvement would facilitate tumor cells to enter the systemic circulation as CTCs. Patients and methods: Sites and extension of metastatic disease were identified with conventional imaging. Bone metastases were diagnosed with either bone scintigraphy or CT-PET and the BM involvement was documented histologically by BM biopsy and metabolically by CT-PET. A training set of 10 pts was evaluated by both BM biopsy and CT-PET to verify the diagnostic performance of CT-PET in identifying BM metastases (M+). We found a 100% concordance between BM biopsy and CT-PET and we therefore used CT-PET for further analyses. The CellSearch System (Veridex LLC, Raritan, NJ, USA) was used for the isolation and enumeration of CTCs in peripheral blood. The Student's t-test and the two-way ANOVA test were used to compare means of CTCs among patients with different metastatic patterns. Results: The CTCs mean and median scores of 129 MBC pts were analysed. Final analysis focused on 101 pts with bone M+. Thirty-three pts had bone M+ alone and 68 pts had bone and visceral M+ (including lymphnodes, brain, liver and lung/pleura). Number of metastatic sites was 1, 2, 3, 4, 5 in 30%, 37%, 25%, 6% and 2% of pts, respectively. BM involvement was documented in 27 (27%) of pts in the whole series and in 12 (33%) of pts with bone M+ alone. Mean CTCs score in the whole series was 392 (0-9993) and the median number of CTCs was 20. In the whole series, BM involvement was associated with higher mean CTCs scores (1350 vs 42, p .014). In pts with bone M+ alone, mean CTCs score was 696 (0-7000) and pts with BM involvement had higher mean CTCs scores (1846 vs 39, p 0.37). Among the different metastatic patterns, the association of bone with BM involvement and liver M+ was correlated with the highest CTCs numbers. We could not perform comparisons in the 68 pts with both bone and visceral localizations because of the variety of metastatic patterns. However, the two-way ANOVA showed a significant influence of BM involvement on mean CTCs scores in pts with different metastatic patterns (p >.001). Conclusions: This work confirms that pts with bone metastases have higher numbers of CTCs than pts with visceral metastases. Extensive bone disease with BM involvement is characterized by an increase in CTCs numbers compared to bone disease without BM involvement. Bone marrow metastases are metabolically more active by CT-PET and can be accurately detected by metabolic imaging without need of BM biopsy. Further studies are ongoing. Citation Information: Cancer Res 2011;71(24 Suppl):Abstract nr P4-07-19.

Published

2011

29. Association between single nucleotide polymorphisms in the XRCC1 and RAD51 genes and clinical radiosensitivity in head and neck cancer

Author

S. Cassani, Claudio Orlando, Lisa Simi, Salvatore Grisanti, Giampaolo Biti, Nicola Pratesi, Caterina Polli, Camillo Almici, Stefano Maria Magrini, Michela Buglione, Calogero Saieva, Lorenzo Livi, Monica Mangoni, Irene Mancini, Fabiola Paiar, and Mario Pazzagli

Subjects

Male, Pathology, Skin erythema, DNA Repair, Radiation Tolerance, Gastroenterology, XRCC1, Gene Frequency, XRCC3, Risk Factors, Nuclear Medicine and Imaging, Genotype, Head and neck cancer, Radiotherapy Dosage, Single Nucleotide, Hematology, DNA-Binding Proteins, Oncology, Head and Neck Neoplasms, Carcinoma, Squamous Cell, Female, Radiology, Adult, Radiotherapy, Single nucleotide polymorphisms, Toxicities, Alleles, Chi-Square Distribution, Glutathione S-Transferase pi, Humans, Proportional Hazards Models, Rad51 Recombinase, Radiation Injuries, Reactive Oxygen Species, Polymorphism, Single Nucleotide, Radiology, Nuclear Medicine and Imaging, medicine.medical_specialty, Single-nucleotide polymorphism, High Resolution Melt, Internal medicine, medicine, Mucositis, Radiology, Nuclear Medicine and imaging, Polymorphism, Allele frequency, business.industry, Carcinoma, medicine.disease, X-ray Repair Cross Complementing Protein 1, Squamous Cell, business

Abstract

Purpose Individual variability in radiosensitivity is large in cancer patients. Single nucleotide polymorphisms (SNPs) in genes involved in DNA repair and in protection against reactive oxygen species (ROS) could be responsible for such cases of radiosensitivity. We investigated the association between the occurrence of acute reactions in 101 patients with squamous cell carcinoma of the head and neck (SCCHN) after radiotherapy (RT) and five genetic polymorphisms: XRCC1 c.1196A > G, XRCC3 c.722C > T, RAD51 (c.-3429G > C, c.-3392G > T), and GSTP1 c.313A > G. Materials and methods Genetic polymorphisms were detected by high resolution melting analysis (HRMA). The development of acute reactions (oral mucositis, skin erythema and dysphagia) associated with genetic polymorphisms was modeled using Cox proportional hazards, accounting for biologically effective dose (BED). Results Development of grade ⩾2 mucositis was increased in all patients (chemo-radiotherapy and radiotherapy alone) with XRCC1-399Gln allele (HR = 1.72). The likelihood of developing grade ⩾2 dysphagia was higher in carriers of RAD51 c.-3429 CC/GC genotypes (HR = 4.00). The presence of at least one SNP or the co-presence of both SNPs in XRCC1 p.Gln399Arg /RAD51 c.-3429 G > C status were associated to higher likelihood of occurrence of acute toxicities (HR = 2.03). Conclusions Our findings showed an association between genetic polymorphisms, XRCC1 c.1196A > G and RAD51 c.-3429 G > C, and the development of radiation-induced toxicities in SCCHN patients.

Published

2011

30. Circulating Tumor Cells and Cardiac Metastasis from Esophageal Cancer: A Case Report

Author

Camillo Almici, Vittorio Ferrari, Giuseppina Arcangeli, Tania Bordonali, Salvatore Grisanti, Francesca Consoli, and Edda Simoncini

Subjects

Pathology, medicine.medical_specialty, medicine.diagnostic_test, Heart metastasis, business.industry, Circulating tumor cell, Esophageal cancer, Cancer, medicine.disease, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, lcsh:RC254-282, Peripheral blood, Oncology, Cardiac magnetic resonance imaging, Cardiac metastasis, Medicine, Myocardial infarction, Published: May 2011, business

Abstract

We report the case of a 67-year-old man affected by metastatic esophageal cancer. The patient developed a symptomatic heart metastasis presenting as mimicking ST-segment elevation myocardial infarction. Cardiac magnetic resonance imaging (MRI) documented the presence of a mass in the apex and septum of the left ventriculum. The dissemination of cancer was confirmed by the detection of circulating tumor cells (CTCs) in the peripheral blood, measured by the CellSearch System (Veridex, LLC, Raritan, N.J., USA). The blood sample drawn at cardiac disease progression revealed the presence of 2 CTCs per 7.5 ml of blood. This report highlights the potential role of CTCs as markers of metastatic spread.

Published

2011

31. Autologous Stem Cell Transplantation Is Effective in Chemosensitive HIV-Associated Lymphoma Irrespective of Previous Therapy and Histological Subtype

Author

Francesco Castelli, Chiara Pagani, Annalisa Peli, Giuseppe Rossi, Salvatore Casari, Chiara Cattaneo, Pierino ferremi Leali, Alessandro Re, Camillo Almici, Nicola Bianchetti, and Emanuele Focà

Subjects

medicine.medical_specialty, business.industry, Immunology, Follicular lymphoma, Cell Biology, Hematology, Aggressive Non-Hodgkin Lymphoma, medicine.disease, Biochemistry, Gastroenterology, Lymphoma, Transplantation, Autologous stem-cell transplantation, Internal medicine, Medicine, Marginal zone B-cell lymphoma, business, Anaplastic large-cell lymphoma, Diffuse large B-cell lymphoma

Abstract

Introduction: Autologous stem cell transplantation (ASCT) is considered safe and effective in patients with HIV-associated lymphoma (HIV-Ly). The reported studies usually analyze togheter different histological subtypes, including classical Hodgkin lymphoma (HL) and a variety of aggressive non Hodgkin lymphoma (NHL), and different indications for ASCT, and report composite outcomes. Aim: We report our single center experience on a large single institution series of patients (pts) with HIV-Ly undergoing ASCT and analyse efficacy according to histology subtypes, indications for ASCT, previous therapy and lymphoma status at transplant, to understand the settings where this treatment approach is most effective and useful. Methods: Retrospective analysis of clinical characteristics and outcome of all consecutive pts with HIV-Ly transplanted at our Institution from March 2001 to February 2018. Results: 62 pts with HIV-Ly underwent ASCT during the study period. Ninety-four % were male; median age was 46 years (range, 29-62). Lymphoma histology was HL in 11 (18%), diffuse large B-cell lymphoma in 22 (35%), Burkitt or Burkitt-like in 13 (21%) , plasmablastic in 10 (16%), T-cell aggressive NHL (3 anaplastic large cell lymphoma, ALK negative, and 1 extranodal NK/T-cell lymphoma, nasal type) in 4 (6%), and indolent B-cell lymphoma (1 follicular lymphoma, and 1 extranodal marginal zone lymphoma) in 2 (3%) pts, respectively. Median CD4+ cells count at ASCT was 208/mL (range, 55-720); 8 pts (13%) had detectable HIV viral load. Eighteen pts (29%) had concomitant hepatitis C and 2 (3%) hepatitis B infection. Indications for ASCT were primary refractory disease (26%), first or subsequent relapse (37%), and consolidation after first line therapy for partial remission (PR) or high risk complete remission (CR) (37%). At the time of ASCT, 10 pts (16%) were in first CR, 45 (73%) had chemosensitive disease (i.e. first PR, chemosensitive relapse/refractory disease), and 7 (11%) had disease refractory to the last chemotherapy (CT) received. Twenty-three patients (37%) had received only 1 line of CT before ASCT, 29 (47%) 2 lines, and 10 (16%) 3 or more lines. Conditioning regimen was BEAM in 47 patients (76%), FEAM in 13 (21%), and 1 each Mitoxantrone-Melphalan and BiCNU-Thiotepa. All pts were receiving cART throughout ASCT except 3 who suspended cART for at least 1 week, due to toxicity and/or oral mucositis. Neutrophil engraftment (neutrophils > 500/mcl) occurred in all pts at a median of 10 days (range, 8-12), and platelet engraftment (platelet count > 20.000/mcl) occurred in all pts at a median of 13 days (range, 9-46), except in one with refractory disease who died of sepsis early after ASCT (treatment-related mortality 1.6%). Twenty-three pts (70%) experienced grade 3-4 toxicity, including oral mucositis (17 patients), gastrointestinal toxicity (8), hepatic toxicity (1), and seizures (1). Twenty-five pts (41%) had an episode of fever of unknown origin. Before engraftment, 22 documented bacterial infections, 1 fungal infection, 2 herpes zoster infections and 5 CMV reactivations were recorded. After a median follow-up of 59 months (range, 1-177) from ASCT, the 5 years-progression free survival (5y-PFS) and OS (5y-OS) were 66.6% and 69.7% respectively, with no significant differences according to different histologies (figure 1). The outcome was satisfactory regardless of the indication for transplant (primary refractory disease, 5y-PFS 50% and 5y-OS 49% , relapse, 5y-PFS 62.6% and 5y-OS 70.7%, and first line consolidation, 5y-PFS 80.3% and 5y-OS 80.1%, P=NS), and number of CT lines before ASCT (1 line, 5y-PFS 80.3% and 5y-OS 80.1%, 2 lines, 5y-PFS 61.3% and 5y- 63.4%, and 3 or more lines, 5y-PFS 53.3% and 5y-OS 66.7%, P=NS). According to the status of lymphoma at the time of ASCT, pts in first CR had a 5y-PFS of 77.8% and 5y-OS of 77.8% and pts with chemosensitive disease 73.7% and 80.3%, while all chemorefractory pts died within 5 months from ASCT, with median PFS and OS of 2 and 3 months respectively (P< 0.001) (figure 2). Conclusion: This is the largest single institution series of HIV-Ly receiving ASCT. We confirm the feasibility and long-term efficacy of this treatment approach in different histological subtypes. ASCT was beneficial also in primary refractory disease and heavily pre-treated pts, provided that lymphoma proved chemosensitive to the last CT received before ASCT. Disclosures Rossi: ABBVIE: Other: ADVISORY BOARD; PFIZER: Other: ADVISORY BOARD; SANDOZ: Honoraria; GILEAD: Other: ADVISORY BOARD; AMGEN: Other: ADVISORY BOARD; SANOFI: Other: ADVISORY BOARD; JANNSEN: Other; JAZZ: Other: ADVISORY BOARD; TEVA: Other: ADVISORY BOARD; CELGENE: Other: ADVISORY BOARD; ROCHE: Other: Advisory Board; NOVARTIS: Honoraria; MUNDIPHARMA: Honoraria; BMS: Honoraria.

Published

2018

32. Endothelial progenitor cells, defined by the simultaneous surface expression of VEGFR2 and CD133, are not detectable in healthy peripheral and cord blood

Author

Paola, Lanuti, Gianluca, Rotta, Camillo, Almici, Giuseppe, Avvisati, Alfredo, Budillon, Paolo, Doretto, Natalia, Malara, Mirella, Marini, Arabella, Neva, Pasquale, Simeone, Elena, Di Gennaro, Alessandra, Leone, Alessandra, Falda, Renato, Tozzoli, Chiara, Gregorj, Melania, Di Cerbo, Valentina, Trunzo, Vincenzo, Mollace, Marco, Marchisio, and Sebastiano, Miscia

Subjects

Adult, Male, Adolescent, Gene Expression, Antigens, CD34, Cell Count, CD146 Antigen, Middle Aged, Fetal Blood, Flow Cytometry, Hematopoietic Stem Cells, Vascular Endothelial Growth Factor Receptor-2, Healthy Volunteers, Immunophenotyping, Benchmarking, Practice Guidelines as Topic, Humans, Leukocyte Common Antigens, Female, AC133 Antigen, Aged, Endothelial Progenitor Cells, Fluorescent Dyes

Abstract

Circulating endothelial cells (CEC) and their progenitors (EPC) are restricted subpopulations of peripheral blood (PB), cord blood (CB), and bone marrow (BM) cells, involved in the endothelial homeostasis maintenance. Both CEC and EPC are thought to represent potential biomarkers in several clinical conditions involving endothelial turnover/remodeling. Although different flow cytometry methods for CEC and EPC characterization have been published so far, none of them have reached consistent conclusions, therefore consensus guidelines with respect to CEC and EPC identification and quantification need to be established. Here, we have carried out an in depth investigation of CEC and EPC phenotypes in healthy PB, CB and BM samples, by optimizing a reliable polychromatic flow cytometry (PFC) panel. Results showed that the brightness of CD34 expression on healthy PB and CB circulating cells represents a key benchmark for the identification of CEC (CD45neg/CD34bright/CD146pos) respect to the hematopoietic stem cell (HSC) compartment (CD45dim/CD34pos/CD146neg). This approach, combined with a dual-platform counting technique, allowed a sharp CEC enumeration in healthy PB (n = 38), and resulting in consistent CEC counts with previously reported data (median = 11.7 cells/ml). In parallel, by using rigorous PFC conditions, CD34pos/CD45dim/CD133pos/VEGFR2pos EPC were not found in any healthy PB or CB sample, since VEGFR2 expression was never detectable on the surface of CD34pos/CD45dim/CD133pos cells. Notably, the putative EPC phenotype was observed in all analyzed BM samples (n = 12), and the expression of CD146 and VEGFR2, on BM cells, was not restricted to the CD34bright compartment, but also appeared on the HSC surface. Altogether, our findings suggest that the previously reported EPC antigen profile, defined by the simultaneous expression of VEGFR2 and CD133 on the surface of CD45dim/CD34pos cells, should be carefully re-evaluated and further studies should be conducted to redefine EPC features in order to translate CEC and EPC characterization into clinical practice.

Published

2015

33. Proangiogenic properties of human myeloma cells: production of angiopoietin-1 and its potential relationship to myeloma-induced angiogenesis

Author

Mirca Lazzaretti, Roberto Sala, Gian C. Gazzola, Mirija Svaldi, Pier Paolo Fattori, Lina Mangoni, Magda Hojden, Paolo Lunghi, Giovanni Roti, Nicola Giuliani, Camillo Almici, Gabriella Sammarelli, Simona Colla, P. Coser, Sabrina Bonomini, Vittorio Rizzoli, Cristina Mancini, Régis Bataille, Giovenzio Genestreti, and Cecilia Caramatti

Subjects

Vascular Endothelial Growth Factor A, Angiogenesis, Endothelial Growth Factors, Biochemistry, Leukemia, Plasma Cell, Neovascularization, chemistry.chemical_compound, RNA, Neoplasm, Lymphokines, Membrane Glycoproteins, Neovascularization, Pathologic, biology, Vascular Endothelial Growth Factors, Antibodies, Monoclonal, Hematology, Middle Aged, Receptor, TIE-2, Angiopoietin receptor, Neoplasm Proteins, Gene Expression Regulation, Neoplastic, Vascular endothelial growth factor, Vascular endothelial growth factor A, medicine.anatomical_structure, Angiopoietin-1, cardiovascular system, Intercellular Signaling Peptides and Proteins, medicine.symptom, Multiple Myeloma, Adult, medicine.medical_specialty, Immunology, Bone Marrow Cells, Angiopoietin-2, Angiopoietin, Proto-Oncogene Proteins, Internal medicine, medicine, Humans, Endothelium, RNA, Messenger, business.industry, Cell Biology, Coculture Techniques, Endocrinology, chemistry, Culture Media, Conditioned, Cancer research, biology.protein, Angiogenesis Inducing Agents, Bone marrow, business

Abstract

Patients with multiple myeloma (MM) have increased bone marrow (BM) angiogenesis; however, the proangiogenic properties of myeloma cells and the mechanisms of MM-induced angiogenesis are not completely clarified. The angiopoietin system has been identified as critical in the regulation of vessel formation. In this study we have demonstrated that myeloma cells express several proangiogenic factors, and, in particular, we found that angiopoietin-1 (Ang-1), but not its antagonist Ang-2, was expressed by several human myeloma cell lines (HMCLs) at the mRNA and the protein levels. In a transwell coculture system, we observed that myeloma cells up-regulated the Ang-1 receptor Tie2 in human BM endothelial cells. Moreover, in an experimental model of angiogenesis, the conditioned medium of HMCLs significantly stimulated vessel formation compared with control or vascular endothelial growth factor (VEGF) treatment. The presence of anti-Tie2 blocking antibody completely blunted the proangiogenic effect of XG-6. Finally, our in vitro results were supported by the in vivo finding of Ang-1, but not Ang-2, mRNA and protein expression in purified MM cells obtained from approximately 47% of patients and by high BM angiogenesis in patients with MM positive for Ang-1, suggesting that the angiopoietin system could be involved, at least in part, in MM-induced angiogenesis.

Published

2003

34. Mesenchymal stromal cells (MSCs) induce ex vivo proliferation and erythroid commitment of cord blood haematopoietic stem cells (CB-CD34+ cells)

Author

Camilla Zanaglio, Sergio Ferrari, Domenico Russo, Mauro Krampera, Maria Teresa Scupoli, Michele Malagola, Claudia Gemelli, Pier Paolo Piccaluga, Andrea Lojacono, Simona Bernardi, Valeria Cancelli, Andrea Di Palma, Giulio Bassi, Edoardo Giacopuzzi, Elisa Zoratti, Giuseppe Borsani, Federica Cattina, Simone Perucca, Mirella Marini, Enrico Tagliafico, Camillo Almici, Perucca, Simone, Di Palma, Andrea, Piccaluga, Pier Paolo, Gemelli, Claudia, Zoratti, Elisa, Bassi, Giulio, Giacopuzzi, Edoardo, Lojacono, Andrea, Borsani, Giuseppe, Tagliafico, Enrico, Scupoli, Maria Teresa, Bernardi, Simona, Zanaglio, Camilla, Cattina, Federica, Cancelli, Valeria, Malagola, Michele, Krampera, Mauro, Marini, Mirella, Almici, Camillo, Ferrari, Sergio, and Russo, Domenico

Subjects

Male, 0301 basic medicine, Microarrays, Cellular differentiation, lcsh:Medicine, Gene Expression, Antigens, CD34, Cell Separation, Spectrum Analysis Techniques, Animal Cells, Medicine and Health Sciences, Coculture Technique, lcsh:Science, Cells, Cultured, Stem cell transplantation for articular cartilage repair, Adult, Adult Stem Cells, Cell Proliferation, Coculture Techniques, Erythroid Cells, Female, Fetal Blood, Hematopoietic Stem Cells, Humans, Mesenchymal Stromal Cells, Transcriptome, Young Adult, Biochemistry, Genetics and Molecular Biology (all), Agricultural and Biological Sciences (all), Multidisciplinary, Mesenchymal Stromal Cell, Chemistry, Stem Cells, Cell Differentiation, Hematology, Flow Cytometry, mesenchymal stomal cells, CD34+ cells, Cord lining, Cell biology, Haematopoiesis, Bioassays and Physiological Analysis, Spectrophotometry, cord blood, Cytophotometry, Cellular Types, Stem cell, Human, Research Article, Adult stem cell, Stromal cell, Research and Analysis Methods, 03 medical and health sciences, Genetics, mesenchymal stomal cells, cord blood, CD34+ cells, Erythroid Cell, lcsh:R, Mesenchymal stem cell, Biology and Life Sciences, Hematopoietic Stem Cell, Mesenchymal Stem Cells, Cell Biology, Hematopoiesis, 030104 developmental biology, Adult Stem Cell, lcsh:Q, Developmental Biology

Abstract

A human bone marrow-derived mesenchymal stromal cell (MSCs) and cord blood-derived CD34+ stem cell co-culture system was set up in order to evaluate the proliferative and differentiative effects induced by MSCs on CD34+ stem cells, and the reciprocal influences on gene expression profiles. After 10 days of co-culture, non-adherent (SN-fraction) and adherent (AD-fraction) CD34+ stem cells were collected and analysed separately. In the presence of MSCs, a significant increase in CD34+ cell number was observed (fold increase = 14.68), mostly in the SN-fraction (fold increase = 13.20). This was combined with a significant increase in CD34+ cell differentiation towards the BFU-E colonies and with a decrease in the CFU-GM. These observations were confirmed by microarray analysis. Through gene set enrichment analysis (GSEA), we noted a significant enrichment in genes involved in heme metabolism (e.g. LAMP2, CLCN3, BMP2K), mitotic spindle formation and proliferation (e.g. PALLD, SOS1, CCNA1) and TGF-beta signalling (e.g. ID1) and a down-modulation of genes participating in myeloid and lymphoid differentiation (e.g. PCGF2) in the co-cultured CD34+ stem cells. On the other hand, a significant enrichment in genes involved in oxygen-level response (e.g. TNFAIP3, SLC2A3, KLF6) and angiogenesis (e.g. VEGFA, IGF1, ID1) was found in the co-cultured MSCs. Taken together, our results suggest that MSCs can exert a priming effect on CD34+ stem cells, regulating their proliferation and erythroid differentiation. In turn, CD34+ stem cells seem to be able to polarise the BM-niche towards the vascular compartment by modulating molecular pathways related to hypoxia and angiogenesis.

Published

2017

35. Clinical validity of circulating tumour cells in patients with metastatic breast cancer : a pooled analysis of individual patient data

Author

Annemie Rutten, Tanja Fehm, Steven Van Laere, Rita Zamarchi, Laura Zorzino, Erich-Franz Solomayer, Alberto Bottini, Carlos Caldas, Salvatore Grisanti, Francesca Consoli, Angela Fernandez de Lascoiti, Luc Dirix, Sofia Agelaki, Camillo Almici, Franco Nolè, Klaus Pantel, Michail Ignatiadis, Dieter Peeters, Justin Stebbing, Paola Gazzaniga, Leticia De Mattos-Arruda, Ronald Lebofsky, Daniele Generali, Jean-Yves Pierga, Jorge S. Reis-Filho, Helene Johannes, Dimitris Mavroudis, Cristina Raimondi, Maria Teresa Sandri, Franziska Meier-Stiegen, Sarah-Jane Dawson, Elisabetta Munzone, Luis Manso, Eduardo Díaz-Rubio, Jonathan Krell, Wolfgang Janni, Jose Vidal-Martinez, Rafael Gisbert-Criado, Eleni Politaki, Jose Ja Garcia-Saenz, Vicente Carañana, François-Clément Bidard, Stefan Michiels, Bidard, François Clément, Peeters, Dieter J., Fehm, Tanja, Nolé, Franco, Gisbert Criado, Rafael, Mavroudis, Dimitrio, Grisanti, Salvatore, Generali, Daniele, Garcia Saenz, Jose A., Stebbing, Justin, Caldas, Carlo, Manso, Lui, Zamarchi, Rita, de Lascoiti, Angela Fernandez, De Mattos Arruda, Leticia, Ignatiadis, Michail, Lebofsky, Ronald, van Laere, Steven J., Meier Stiegen, Franziska, Sandri, Maria Teresa, Vidal Martinez, Jose, Politaki, Eleni, Consoli, Francesca, Bottini, Alberto, Diaz Rubio, Eduardo, Krell, Jonathan, Dawson, Sarah Jane, Raimondi, Cristina, Rutten, Annemie, Janni, Wolfgang, Munzone, Elisabetta, Carañana, Vicente, Agelaki, Sofia, Almici, Camillo, Dirix, Luc, Solomayer, Erich Franz, Zorzino, Laura, Johannes, Helene, Reis Filho, Jorge S., Pantel, Klau, Pierga, Jean Yve, Michiels, Stefan, and Gazzaniga, PAOLA MARIA

Subjects

Oncology, Time Factors, medicine.medical_treatment, Cell Count, Kaplan-Meier Estimate, 0302 clinical medicine, Carcinoembryonic antigen, Risk Factors, Likelihood Functions, 0303 health sciences, biology, Hazard ratio, Middle Aged, Neoplastic Cells, Circulating, Metastatic breast cancer, 3. Good health, Europe, Treatment Outcome, 030220 oncology & carcinogenesis, Predictive value of tests, Female, medicine.medical_specialty, Breast Neoplasms, Disease-Free Survival, 03 medical and health sciences, Predictive Value of Tests, Internal medicine, Biomarkers, Tumor, medicine, Humans, Aged, Proportional Hazards Models, Retrospective Studies, 030304 developmental biology, Chemotherapy, Chi-Square Distribution, Proportional hazards model, business.industry, Mucin-1, Reproducibility of Results, Retrospective cohort study, medicine.disease, Carcinoembryonic Antigen, Surgery, biology.protein, Human medicine, business, Chi-squared distribution

Abstract

We aimed to assess the clinical validity of circulating tumour cell (CTC) quantification for prognostication of patients with metastatic breast cancer by undertaking a pooled analysis of individual patient data.We contacted 51 European centres and asked them to provide reported and unreported anonymised data for individual patients with metastatic breast cancer who participated in studies between January, 2003, and July, 2012. Eligible studies had participants starting a new line of therapy, data for progression-free survival or overall survival, or both, and CTC quantification by the CellSearch method at baseline (before start of new treatment). We used Cox regression models, stratified by study, to establish the association between CTC count and progression-free survival and overall survival. We used the landmark method to assess the prognostic value of CTC and serum marker changes during treatment. We assessed the added value of CTCs or serum markers to prognostic clinicopathological models in a resampling procedure using likelihood ratio (LR) χ(2) statistics.17 centres provided data for 1944 eligible patients from 20 studies. 911 patients (46·9%) had a CTC count of 5 per 7·5 mL or higher at baseline, which was associated with decreased progression-free survival (hazard ratio [HR] 1·92, 95% CI 1·73-2·14, p0·0001) and overall survival (HR 2·78, 95% CI 2·42-3·19, p0·0001) compared with patients with a CTC count of less than 5 per 7·5 mL at baseline. Increased CTC counts 3-5 weeks after start of treatment, adjusted for CTC count at baseline, were associated with shortened progression-free survival (HR 1·85, 95% CI 1·48-2·32, p0·0001) and overall survival (HR 2·26, 95% CI 1·68-3·03) as were increased CTC counts after 6-8 weeks (progression-free survival HR 2·20, 95% CI 1·66-2·90, p0·0001; overall survival HR 2·91, 95% CI 2·01-4·23, p0·0001). Survival prediction was significantly improved by addition of baseline CTC count to the clinicopathological models (progression-free survival LR 38·4, 95% CI 21·9-60·3, p0·0001; overall survival LR 64·9, 95% CI 41·3-93·4, p0·0001). This model was further improved by addition of CTC change at 3-5 weeks (progression-free survival LR 8·2, 95% CI 0·78-20·4, p=0·004; overall survival LR 11·5, 95% CI 2·6-25·1, p=0·0007) and at 6-8 weeks (progression-free survival LR 15·3, 95% CI 5·2-28·3; overall survival LR 14·6, 95% CI 4·0-30·6; both p0·0001). Carcinoembryonic antigen and cancer antigen 15-3 concentrations at baseline and during therapy did not add significant information to the best baseline model.These data confirm the independent prognostic effect of CTC count on progression-free survival and overall survival. CTC count also improves the prognostication of metastatic breast cancer when added to full clinicopathological predictive models, whereas serum tumour markers do not.Janssen Diagnostics, the Nuovo-Soldati foundation for cancer research.

Published

2014

36. Changes in Circulating Endothelial Cells Count Could Become a Valuable Tool in the Diagnostic Definition of Acute Graft-Versus-Host Disease

Author

Alessandro Turra, Michele Malagola, Simona Braga, Mirella Marini, Andrea Bianchetti, Camillo Almici, Arabella Neva, Domenico Russo, Andrea Di Palma, Cristina Skert, and Rosanna Verardi

Subjects

Adult, Male, Risk, medicine.medical_specialty, Transplantation Conditioning, Adolescent, Acute myeloblastic leukemia, Chronic lymphocytic leukemia, medicine.medical_treatment, Graft vs Host Disease, Cell Count, Cell Separation, Hematopoietic stem cell transplantation, Gastroenterology, immune system diseases, Internal medicine, Humans, Transplantation, Homologous, Medicine, Prospective Studies, Multiple myeloma, Transplantation, business.industry, Hematopoietic Stem Cell Transplantation, Endothelial Cells, Myeloid leukemia, Odds ratio, Middle Aged, medicine.disease, Confidence interval, Lymphoma, surgical procedures, operative, Hematologic Neoplasms, Immunology, Female, Endothelium, Vascular, business

Abstract

BACKGROUND Allogeneic hematopoietic stem cell transplantation (allo-HSCT) is burdened by life-threatening complications, with graft-versus-host disease (GvHD) being the major cause of morbility and mortality. Recently, clinical and physiopathologic evidences showed that vascular endothelium can be a target of GvHD in the early phase and circulating endothelial cells (CECs) represent surrogate markers of endothelial damage. METHODS Using the CellSearch System (Veridex LLC, Raritan, NJ), CECs were counted before (T1), after conditioning regimen (T2), at engraftment (T3), at GvHD onset (T4), and after steroid treatment (T5) in 40 patients (7 Hodgkin's Disease, 13 Acute Myeloblastic Leukemia, 5 Acute Lymphoblastic Leukemia, 8 Multiple Myeloma, 3 Chronic Lymphocytic Leukemia, 1 Non-Hodgkin Lymphoma, 1 Chronic Myeloid Leukemia, 2 Severe Aplastic Anemia) undergoing allo-HSCT. RESULTS The median CEC per milliliter at T1 was 20 (n=33, range 4-718), in comparison to a value of 2 (range, 1-14) in controls (P

Published

2014

37. Clonogenic capacity andex vivo expansion potential of umbilical cord blood progenitor cells are not impaired by cryopreservation

Author

Carmelo Carlo-Stella, D. Garau, A Re, R Giachetti, Vittorio Rizzoli, Lina Mangoni, Camillo Almici, John E. Wagner, and Clara Cesana

Subjects

Cryopreservation, Transplantation, CD34, Antigens, CD34, Hematology, Biology, Fetal Blood, Hematopoietic Stem Cells, Andrology, Immunophenotyping, medicine.anatomical_structure, Immunology, medicine, Humans, Bone marrow, Stem cell, Progenitor cell, Clonogenic assay, Ex vivo

Abstract

Umbilical cord blood (UCB) progenitor cells have been demonstrated to possess significant advantages over bone marrow (BM), in terms of proliferative capacity and immunologic reactivity. Therefore, UCB has been recently considered an attractive potential alternative to BM as a source of hematopoietic progenitor cells for clinical applications. Since several programs throughout the world are currently evaluating the feasibility of large-scale UCB banking for unrelated transplants, it was the aim of this study to evaluate whether cryopreservation procedures might heavily impair the clonogenic capacity, the feasibility of CD34+ selection and the ex vivo expansion potential of UCB progenitor cells. UCB samples were collected and cryopreserved as unseparated (n = 21) or mononuclear (MNC) cells (n = 15) within 12 h from delivery, and evaluated for viability, immunophenotype, cell and progenitor numbers after a minimum stay in liquid nitrogen of 6 months (range 6-14 months). Viability was always > 97% and no statistically significant difference was detected by flow cytometric analysis. Clonogenic recovery from unseparated cells was 80-87% for HPP-CFC, CFU-GEMM, BFU-E and CFU-GM, and from MNC cells ranged from 82 to 91% for LTC-IC, CFU-GEMM, BFU-E and CFU-GM. CD34+ selection (n = 8) was performed on fresh and cryopreserved MNC cells using the MiniMACS immunomagnetic separation device, showing no difference in yield (68 +/- 7% vs 57 +/- 4%, P < or = 0.4) or in purity (89 +/- 2% vs 81 +/- 6%, < or = 0.4), for fresh in comparison to cryopreserved MNC cells. After 14 days of liquid culture in the presence of different combinations of SCF, IL-3, IL-6 and G-CSF no statistically significant difference was detected in CFC fold-expansion for fresh or cryopreserved MNC cells and for CD34+ cells, either selected and cultured from fresh or cryopreserved MNC cells. In conclusion we can state that UCB is a potential source of primitive progenitor cells that can be cryopreserved unmanipulated or after physical separation without major losses in clonogenic capacity and immunophenotypic composition. Moreover, CD34+ selection from cryopreserved MNC cells is feasible and ex vivo expansion is not impaired. These results have important implications in the large scale UCB banking, in view of the potential applications of ex vivo expanded hematopoietic progenitor cells for the engraftment of adult patients.

Published

1997

38. Stem cell mobilization in HIV seropositive patients with lymphoma

Author

Bernardino Allione, Salvatore Casari, Marcus Hentrich, Salvatore Gattillo, Pascual Balsalobre, Alessandro Re, Andrés J.M. Ferreri, Silvia Montoto, Mario Mazzucato, Umberto Tirelli, José Luis Díez-Martín, Cristina Skert, Philipp Schommers, Camillo Almici, Mark Bower, José M. Ribera, Michele Spina, Mariagrazia Michieli, Pierino Ferremi, Giuseppe Rossi, and Chiara Cattaneo

Subjects

Adult, Male, medicine.medical_specialty, Cyclophosphamide, medicine.medical_treatment, Population, CD34, Gastroenterology, Young Adult, Internal medicine, HIV Seropositivity, medicine, Humans, education, Hematopoietic Stem Cell Mobilization, Aged, Retrospective Studies, Chemotherapy, education.field_of_study, Mobilization, business.industry, Lymphoma, Non-Hodgkin, Hematology, Articles, Middle Aged, medicine.disease, Hodgkin Disease, Lymphoma, Immunology, Female, Stem cell, business, medicine.drug

Abstract

High-dose chemotherapy with autologous peripheral blood stem cell rescue has been reported as feasible and effective in HIV-associated lymphoma. Although a sufficient number of stem cells seems achievable in most patients, there are cases of stem cell harvest failure. The aim of this study was to describe the mobilization policies used in HIV-associated lymphoma, evaluate the failure rate and identify factors influencing mobilization results. We analyzed 155 patients who underwent attempted stem cell mobilization at 10 European centers from 2000-2012. One hundred and twenty patients had non-Hodgkin lymphoma and 35 Hodgkin lymphoma; 31% had complete remission, 57% chemosensitive disease, 10% refractory disease, 2% untested relapse. Patients were mobilized with chemotherapy + G-CSF (86%) or G-CSF alone (14%); 73% of patients collected2 and 48%5 × 10(6) CD34(+) cells/kg. Low CD4+ count and refractory disease were associated with mobilization failure. Low CD4(+) count, low platelet count and mobilization with G-CSF correlated with lower probability to achieve5 × 10(6) CD34(+) cells/kg, whereas cyclophosphamide ≥ 3 g/m(2) + G-CSF predicted higher collections. Circulating CD34(+) cells and CD34/WBC ratio were strongly associated with collection result. HIV infection alone should not preclude an attempt to obtain stem cells in candidates for autologous transplant as the results are comparable to the HIV-negative population.

Published

2013

39. Comparative Analysis of Mesenchymal Stromal Cells Biological Properties

Author

Patrizia Dell'Era, Patrizia Benzoni, Er Xia, Arabella Neva, Angela De Luca, Elisabetta Crescini, Camillo Almici, Stefano Calza, and Rosanna Verardi

Subjects

Pathology, medicine.medical_specialty, Stromal cell, Article Subject, Mesenchymal stem cell, Mesenchymal stromal cells, Adipose tissue, Biology, adipose tissue, Cell therapy, Immunophenotyping, medicine.anatomical_structure, Cancer research, medicine, Bone marrow, Progenitor cell, Stem cell transplantation for articular cartilage repair

Abstract

The stromal progenitors of mesodermal cells, mesenchymal stromal cells (MSCs), are a heterogeneous population of plastic adherent fibroblast-like cells with extensive proliferative capacity and differentiation potential. Human MSCs have now been isolated from various tissues including bone marrow, muscle, skin, and adipose tissue, the latter being one of the most suitable cell sources for cell therapy, because of its easy accessibility, minimal morbidity, and abundance of cells. Bone marrow and subcutaneous or visceral adipose tissue samples were collected, digested with collagenase if needed, and seeded in Iscove's medium containing 5% human platelet lysate. Nonadherent cells were removed after 2-3 days and the medium was replaced twice a week. Confluent adherent cells were detached, expanded, and analyzed for several biological properties such as morphology, immunophenotype, growth rate, senescence, clonogenicity, differentiation capacity, immunosuppression, and secretion of angiogenic factors. The results show significant differences between lines derived from subcutaneous fat compared to those derived from visceral fat, such as the higher proliferation rate of the first and the strong induction of angiogenesis of the latter. We are convinced that the identification of the peculiarities of MSCs isolated from different tissues will lead to their more accurate use in cell therapy.

Published

2013

40. Selection of myeloid progenitors lacking BCR/ABL mRNA in chronic myelogenous leukemia patients after in vitro treatment with the tyrosine kinase inhibitor genistein

Author

M. T. Rizzo, Antonio Bonati, E. Regazzi, D. Garau, Camillo Almici, Carmelo Carlo-Stella, Lina Mangoni, Barbara Savoldo, Gianpietro Dotti, Gabriella Sammarelli, and Vittorio Rizzoli

Subjects

ABL, medicine.drug_class, Immunology, breakpoint cluster region, Genistein, Cell Biology, Hematology, Biology, medicine.disease, Biochemistry, Tyrosine-kinase inhibitor, Leukemia, chemistry.chemical_compound, Terminal deoxynucleotidyl transferase, chemistry, hemic and lymphatic diseases, medicine, Cancer research, Tyrosine kinase, Chronic myelogenous leukemia

Abstract

Chronic myelogenous leukemia (CML) is a clonal disorder of the hematopoietic stem cell characterized by a chimeric BCR/ABL gene giving rise to a 210-kD fusion protein with dysregulated tyrosine kinase activity. We investigated the effect of genistein, a protein tyrosine kinase inhibitor, on the in vitro growth of CML and normal marrow-derived multi-potent (colony-forming unit-mix [CFU-Mix]), erythroid (burst-forming unit-erythroid [BFU-E]), and granulocyte-macrophage (colony-forming unit-granulocyte-macrophage [CFU-GM]) hematopoietic progenitors. Continuous exposure of CML and normal marrow to genistein induced a statistically significant and dose-dependent suppression of colony formation. Genistein doses causing 50% inhibition of CML and normal progenitors were not significantly different for CFU-Mix (27 mumol/L v 23 mumol/L), BFU-E (31 mumol/L v 29 mumol/L), and CFU-GM (40 mumol/L v 32 mumol/L v 32 mumol/L). Preincubation of CML and normal marrow with genistein (200 mumol/ L for 1 to 18 hours) induced a time-dependent suppression of progenitor cell growth, while sparing a substantial proportion of long-term culture-initiating cells (LTC-IC) from CML (range, 91% +/- 9% to 32% +/- 3%) and normal marrow (range, 85% +/- 8% to 38% +/- 9%). Analysis of individual CML colonies for the presence of the hybrid BCR/ABL mRNA by reverse transcription-polymerase chain reaction (RT-PCR) showed that genistein treatment significantly reduced the mean +/- SD percentage of marrow BCR/ABL+ progenitors both by continuous exposure (76% +/- 18% v 24% +/- 12%, P ‼ or = .004) or preincubation (75% +/- 16% v 21% +/- 10%, P ‼ or = .002) experiments. Preincubation with genistein reduced the percentage of leukemic LTC-IC from 87% +/- 12% to 37% +/- 12% (P ‼ or = .003). Analysis of individual colonies by cytogenetics and RT-PCR confirmed that genistein-induced increase in the percentage of nonleukemic progenitors was not due to suppression of BCR/ABL transcription. Analysis of nuclear DNA fragmentation by DNA gel electrophoresis and terminal deoxynucleotidyl transferase assay showed that preincubation of CML mononuclear and CD34+ cells with genistein induced significant evidence of apoptosis. These observations show that genistein is capable of (1) exerting a strong antiproliferative effect on CFU-Mix, BFU-E, and CFU-GM while sparing the more primitive LTC-IC and (2) selecting benign hematopoietic progenitors from CML marrow, probably through an apoptotic mechanism.

Published

1996

41. Effect of the protein tyrosine kinase inhibitor genistein on normal and leukaemic haemopoietic progenitor cells

Author

D. Garau, Carmelo Carlo-Stella, Antonio Bonati, E. Regazzi, Gianpietro Dotti, Vittorio Rizzoli, Camillo Almici, Lina Mangoni, and M. T. Rizzo

Subjects

medicine.medical_specialty, medicine.drug_class, Genistein, Biology, Tyrosine-kinase inhibitor, chemistry.chemical_compound, Internal medicine, Tumor Cells, Cultured, medicine, Humans, Enzyme Inhibitors, Progenitor cell, Dose-Response Relationship, Drug, Cell growth, Hematology, Protein-Tyrosine Kinases, Hematopoietic Stem Cells, Isoflavones, Leukemia, Myeloid, Acute, Endocrinology, chemistry, Cell culture, Neoplastic cell, Growth inhibition, Stem cell, Cell Division

Abstract

Receptor and nonreceptor protein tyrosine kinases (PTKs) play a key role in the control of normal and neoplastic cell growth. The availability of PTK inhibitors prompted us to evaluate the effects of genistein, a natural inhibitor of PTKs, on in vitro colony formation by normal multilineage colony-forming units (CFU-Mix), erythroid bursts (BFU-E), granulocyte-macrophage colony-forming units (CFU-GM), long-term culture-initiating cells (LTC-IC) and acute myelogenous leukaemia colony-forming units (CFU-AML). Continuous exposure of normal marrow and blood mononuclear non-adherent cells, blood CD34+CD45RA- cells, and leukaemic blasts to increasing doses of genistein (1-100 microM) resulted in a statistically significant (P < or = 0.05) dose-dependent suppression of CFU-Mix, BFU-E, CFU-GM and CFU-AML growth. Regression analysis showed that growth inhibition was linearly related to genistein concentration. Genistein dose causing 50% inhibition (ID50) of CFU-AML was significantly lower compared to CFU-GM ID50 for marrow (19 v 32 microM, P < or = 0.017), unseparated blood (19 v 44 microM, P < or = 0.028) or CD34+CD45RA- blood (19 v 36, P < or = 0.04). Preincubation of leukaemic blasts with genistein (200 microM) for 1-2h confirmed that CFU-AML were significantly more sensitive than normal marrow and blood CFU-GM to genistein. Preincubation conditions which maximally suppressed leukaemic and normal colony growth spared a substantial percentage of marrow (29 +/- 4%) and blood (40 +/- 3%) LTC-IC. In conclusion, our data demonstrate that: (a) genistein strongly inhibits the growth of normal and leukaemic haemopoietic progenitors; (b) growth inhibition is dose- and time-dependent; (c) leukaemic progenitors are more sensitive than normal progenitors to genistein-induced growth inhibition; (d) genistein exerts a direct toxic effect on haemopoietic cells while sparing a substantial proportion of LTC-IC. The potent CFU-AML growth inhibition associated with the relative resistance of normal LTC-IC strongly supports the use of genistein for marrow purging.

Published

1996

42. Contents, Vol. 95, 1996

Author

H.T. Hassan, Diana Linnekin, Hisamaru Hirai, Tiziano Barbui, Anna Rita Migliaccio, Jonathan R. Keller, Sarah R. Weiler, Akihiro Iwamatsu, Nathalie Beslu, Stefano Pileri, C. Nissen, Olivier Rosnet, Sante Tura, M. Federico, Masayuki Yamamoto, Vincent Geenen, Sandra N. Catlin, Nader G. Abraham, Shigehiko Imagawa, John E. Wagner, Hans G. Drexler, Candy S. DeBerry, M. Baiocchi, Giuseppe Saglio, Emanuela Moroni, Patrice Dubreuil, Sylvie Marchetto, Lorenzo Leoncini, Ko Sasaki, Alessandra Fortuna, F. Nappi, Abdellah Benhida, Eric Vandersmissen, Hans-Jörg Bühring, Vittorio Rizzoli, Janis L. Abkowitz, Filippo Gherlinzoni, Doraid Jarrar, Douglas K. Ferris, Jean-Pierre Kremer, Hideharu Odai, Elisabeth Spitzer, Ursula Steckholzer, Gianantonio Rosti, Alessandro Rambaldi, A. Filipowicz, Françoise Birg, Miriam Fogli, Béatrice Goxe, Francis W. Ruscetti, Stefania Damiani, Antonino Carbone, Camillo Almici, Jennifer K. Morrow, K. Pugliese, Wolfgang Ertel, B. Speck, Henri Martens, Peter Dörmer, Nedda K. Hughes, Sergio Ottolenghi, Alessandro Gozzetti, Giovanni Migliaccio, Peter Guttorp, Gianluca Gaidano, Yves Vanneste, Charles Hannum, Teresa Lerede, Renato Bassan, A. Tichelli, Ornella Leone, Gisella Volpe, H. Baldomero, Vincent S. Gallicchio, James Gajewski, Annunziata Gloghini, A. Gratwohl, A. Zander, Barbara Giglioni, Yoshio Yazaki, Sergio Giralt, Guiseppe Visani, Lucia Catani, Kam-Fai Tse, Roberto M. Lemoli, Eishi Ashihara, Robert Rottapel, Imane Achour, Richard E. Champlin, C. Chelucci, Elena Sabattini, L. John, P. D’Aloja, Yasusada Miura, Claudio Ceccarelli, Monica T. Persik, Robert A.J. Oostendorp, P. Verani, Daniel Birnbaum, Ouafae Kecha, Dan L. Longo, Brunangelo Falini, Donatella Santini, Paolo Ghia, R. Bona, Carmelo Carlo-Stella, Yutaka Hanazono, Chrystel Lavagna, Irene Rappold, Sherry Mou, Cristina Pastore, F. Mavilio, and Odile deLapeyrière

Subjects

Hematology, General Medicine

Published

1996

43. Isolation of small, primitive human hematopoietic stem cells: distribution of cell surface cytokine receptors and growth in SCID-Hu mice

Author

Jane S. Lebkowski, Camillo Almici, Amy E. Berson, Lisa R. Schain, Melinda A. Hall, Daniel P Collins, Karen E. Chen, Shawn Fuller, Thomas B. Okarma, and John E. Wagner

Subjects

education.field_of_study, biology, Immunology, Population, Stem cell factor, Cell Biology, Hematology, CD38, Cell cycle, Biochemistry, Molecular biology, CD19, Haematopoiesis, biology.protein, Progenitor cell, Stem cell, education

Abstract

Human CD34+ cells were subfractionated into three size classes using counterflow centrifugal elutriation followed by immunoadsorption to polystyrene cell separation devices. The three CD34+ cell fractions (Fr), Fr 25/29, Fr 33/37, and Fr RO, had mean sizes of 8.5, 9.3 and 13.5 microns, respectively. The majority of cells in the large Fr RO CD34+ cell population expressed the committed stage antigens CD33, CD19, CD38, or HLA-DR and contained the majority of granulocyte- macrophage colony-forming units (CFU-GM), burst-forming units-erythroid (BFU-E), and CFU-mixed lineage (GEMM). In contrast, the small Fr 25/29 CD34+ cells were devoid of committed cell surface antigens and lacked colony-forming activity. When seeded to allogeneic stroma, Fr RO CD34+ cells produced few CFU-GM at week 5, whereas cells from the Fr 25/29 CD34+ cell population showed a 30- to 55-fold expansion of myeloid progenitors at this same time point. Furthermore, CD34+ cells from each size fraction supported ontogeny of T cells in human thymus/liver grafts in severe combined immunodeficient (SCID) mice. Upon cell cycle analyses, greater than 97% of the Fr 25/29 CD34+ cells were in G0/G1 phase, whereas greater proportions of the two larger CD34+ cell fractions were in active cell cycle. Binding of the cytokines interleukin (IL)-1 alpha, IL-3, IL-6, stem cell factor (SCF), macrophage inhibitory protein (MIP)-1 alpha, granulocyte colony- stimulating factor (G-CSF), and granulocyte-macrophage (GM)-CSF to these CD34+ cell populations was also analyzed by flow cytometry. As compared with the larger CD34+ cell fractions, cells in the small Fr 25/29 CD34+ cell population possessed the highest numbers of receptors for SCF, MIP1 alpha, and IL-1 alpha. Collectively, these results indicate that the Fr 25/29 CD34+ cell is a very primitive, quiescent progenitor cell population possessing a high number of receptors for SCF and MIP1 alpha and capable of yielding both myeloid and lymphoid lineages when placed in appropriate in vitro or in vivo culture conditions.

Published

1995

44. Density separation of umbilical cord blood and recovery of hemopoietic progenitor cells: Implications for cord blood banking

Author

John E. Wagner, Vittorio Rizzoli, D. Garau, Alessandro Ventura, Mirella Armanetti, Lina Mangoni, Carmelo Carlo-Stella, Luca Cottafavi, and Camillo Almici

Subjects

Time Factors, Sialic Acid Binding Ig-like Lectin 3, CD34, Antigens, Differentiation, Myelomonocytic, Antigens, CD34, Cell Separation, Hematocrit, Biology, Colony-Forming Units Assay, Andrology, Antigens, CD, Pregnancy, Culture Techniques, Centrifugation, Density Gradient, medicine, Humans, Progenitor cell, Cells, Cultured, Blood Specimen Collection, medicine.diagnostic_test, Hematopoietic Stem Cell Transplantation, Infant, Newborn, Povidone, Cell Biology, Fetal Blood, Hematopoietic Stem Cells, Silicon Dioxide, Transplantation, Haematopoiesis, Cord blood, Immunology, Blood Banks, Molecular Medicine, Female, Stem cell, Cell Adhesion Molecules, Percoll, Developmental Biology

Abstract

Umbilical cord blood (CB) has been evaluated as a potential source of hematopoietic stem cells suitable for clinical use in the transplantation setting. Previous reports have documented a significant loss of progenitor cells by any manipulation other than cryopreservation. We have evaluated the feasibility of fractionating and cryopreserving CB samples with minimal loss of progenitor cells. We have compared various separation procedures based on different density gradients in the attempt to obtain the highest depletion of red blood cells (RBC) while maintaining the highest recovery of progenitor cells. We compared three different densities of Percoll (1.069 g/ml, 1.077 g/ml, 1.084 g/ml), sedimentation over poligeline (Emagel ) and sedimentation over poligeline followed by separation over Ficoll/Hypaque (F/H). Separated samples (n = 25) were analyzed for recovery of CD34+ cells and progenitor cells (CFU-GEMM, BFU-E, CFU-GM). Separation by sedimentation over poligeline followed by F/H allowed the highest depletion of RBC (hematocrit of the final cellular suspension 0.4 +/- 0.1%) while maintaining high recovery of CD34+ cells (85.3 +/- 5.6%) and total recovery for CFU-GEMM, BFU-E and CFU-GM. After cryopreservation, recovery of clonogenic progenitors was 82% for CFU-GEMM, 94% for BFU-E, 82% for CFU-GM and 90% for colony-forming units (CFUs) after five weeks of long-term culture (LTC). We further evaluated the effect of stem cell factor (SCF) on the in vitro growth of hemopoietic progenitors and on replating efficiency.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1995

45. Circulating tumour cells in locally advanced head and neck cancer: preliminary report about their possible role in predicting response to non-surgical treatment and survival

Author

Andrea Bolzoni, Rosanna Verardi, Nadia Pasinetti, Caterina Polli, Michela Buglione, Edda Simoncini, Salvatore Grisanti, Fabiola Paiar, Monica Mangoni, Stefano Maria Magrini, Camillo Almici, Mirella Marini, Francesca Consoli, Gianpaolo Biti, Piero Nicolai, and L. Costa

Subjects

Oncology, Male, Cancer Research, Pathology, Time Factors, medicine.medical_treatment, Cetuximab, Neoplastic Cells, Circulating Tumour Cells, Prostate cancer, Risk Factors, Monoclonal, Antineoplastic Combined Chemotherapy Protocols, Circulating, Prospective Studies, Head and neck cancer, Humanized, Chemotherapy, Radiotherapy, Antibodies, Monoclonal, Antibodies, Monoclonal, Humanized, Antineoplastic Agents, Chi-Square Distribution, Disease Progression, Female, Head and Neck Neoplasms, Humans, Italy, Neoplasm Grading, Neoplasm Staging, Neoplastic Cells, Circulating, Predictive Value of Tests, Risk Assessment, Survival Analysis, Treatment Outcome, Chemoradiotherapy, Hypopharyngeal cancer, medicine.drug, medicine.medical_specialty, Antibodies, Sinonasal undifferentiated carcinoma, Internal medicine, medicine, business.industry, Cancer, medicine.disease, Radiation therapy, business

Abstract

The mechanism of dissemination of locally advanced head and neck cancer (LAHNC) is far to be resolved. Circulating tumour cells (CTC) have been identified as a prognostic factor in metastatic breast and prostate cancer. This prospective multi-centric analysis studied the possible role of CTC identification in LAHNC.CTC were searched in 73 patients with LAHNC (oropharynx, n=39; nasopharynx, n=10; larynx, n=10; paranasal sinuses, n=6, of whom 3 with sinonasal undifferentiated carcinoma, SNUC; hypopharynx, n=5; oral cavity, n=3). All of them (apart from SNUC) had squamous cell cancers. The relationship between CTC positivity and other clinical prognostic factors has been investigated. Response to treatment and survival has been related with changes in CTC number during the treatment.CTC were frequently identified in oro- and hypopharyngeal cancer and in SNUC. They were more frequent in stage IV than in stages I-III disease (18% versus 6%, p=NS (not significant)). Partial or complete response (CR) was related with the absence or disappearance of CTC during treatment (p=0.017). A decrease in the CTC number or their absence throughout the treatment seems also related with non-progressive disease, after both complete or incomplete remission and with the proportion of patients alive and NED (no evidence of disease) (p=0.009).These preliminary data suggest a possible role of CTC determination in head and neck cancer. Additional and longer follow up data need to be collected to confirm these findings.

Published

2012

46. Circulating tumor cells as predictors of prognosis in metastatic breast cancer: clinical application outside a clinical trial

Author

Francesca Consoli, Salvatore Grisanti, Vito Amoroso, Camillo Almici, Rosanna Verardi, Mirella Marini, and Edda Simoncini

Subjects

Adult, Cancer Research, Breast Neoplasms, Hospitals, Community, Kaplan-Meier Estimate, Hospitals, General, Disease-Free Survival, 030218 nuclear medicine & medical imaging, 03 medical and health sciences, 0302 clinical medicine, Predictive Value of Tests, Biomarkers, Tumor, Odds Ratio, Humans, Prospective Studies, Aged, Neoplasm Staging, Proportional Hazards Models, Analysis of Variance, General Medicine, Middle Aged, Neoplastic Cells, Circulating, Prognosis, Treatment Outcome, Oncology, Italy, 030220 oncology & carcinogenesis, Disease Progression, Female

Abstract

Aims and Background Circulating tumor cells have a prognostic role in metastatic breast cancer. The aim of the study was to confirm the ability of circulating tumor cells, detected by the US Food and Drug Administration approved Cell Search assay, to predict the outcome of patients treated in a community general hospital. Patients and Methods. A prospective mono-institutional study was conducted at the Department of Medical Oncology at Spedali Civili, Brescia, Italy, from January 2009 to September 2010. A total of 93 consecutive patients with metastatic breast cancer were enrolled. Patients underwent a blood sample collection to detect circulating tumor cells at baseline and, subsequently, at the first follow-up examination (after 3-4 weeks from the beginning of a systemic therapy). A third sample was drawn at disease progression (at the beginning of a subsequent new course of therapy). The prognostic cutoff value of circulating tumor cells was fixed at 5 cells/7.5 ml of blood. Results At baseline, median overall survival and progression-free survival in the subgroup ≥5 circulating tumor cells/7.5 ml of blood were significantly shorter (5 months and 3 months, respectively) than in the subgroup with Conclusions Our study confirms the role of circulating tumor cells as predictors of prognosis in metastatic breast cancer patients treated in general clinical practice.

Published

2012

47. Biological and chemical selection of ph&hyphen;negative clones

Author

Carmelo Carlo-Stella, Camillo Almici, D. Garau, Lina Mangoni, Giovanna Piovani, and Vittorio Rizzoli

Subjects

Stromal cell, Hematopoietic stem cell, Karyotype, Cell Biology, Biology, medicine.disease, Molecular biology, chemistry.chemical_compound, medicine.anatomical_structure, Mafosfamide, chemistry, Stroma, Immunology, medicine, Molecular Medicine, Progenitor cell, Clonogenic assay, Developmental Biology, Chronic myelogenous leukemia

Abstract

Chronic myelogenous leukemia (CML) is a clonal disorder of the hematopoietic stem cell characterized by the co-existence of Philadelphia-negative with Ph-positive progenitors. CML progenitor cells have been shown to be defective in adherence to marrow stroma. The present study investigated at the cytogenetic level marrow-derived CML clonogenic cells generated from the stroma-adherent cell fraction. Mononuclear marrow cells from CML patients (n = 20) were incubated with mafosfamide (100 micrograms/ml) or control medium, seeded onto marrow stromal layers, and allowed to adhere (2 h, 37 degrees C). Following a short-term (3 days) liquid culture, the cells were harvested, incorporated in methylcellulose, and individual colonies were analyzed by single colony karyotyping. On direct cytogenetic analysis, the overall mean (+/- SD) percentage of Ph-negative metaphases was 9 +/- 20%. The mean (+/- SD) percentages of Ph-negative colonies grown from the stroma-adherent and the stroma-adherent mafosfamide-treated fraction were 41 +/- 32% and 62 +/- 40% (p < or = .005), respectively. Single colony transfer experiments revealed that 50 +/- 13% stroma-adherent and 70 +/- 24% stroma-adherent mafosfamide-treated progenitors gave rise to secondary colonies. In conclusion, the present data demonstrate the possibility to select Ph-negative clones that: 1) have a maintained capability of stroma adherence; 2) are mafosfamide resistant; and 3) have high-replating potential.

Published

1993

48. Fractionation of Chronic Myelogenous Leukemia Marrow Cells by Stroma Adherence: Implications for Marrow Purging

Author

Vittorio Rizzoli, Camillo Almici, Giovanna Piovani, Lina Mangoni, D. Garau, Cecilia Caramatti, and Carmelo Carlo-Stella

Subjects

Cancer Research, Pathology, medicine.medical_specialty, Stromal cell, Cells, Bone Marrow Cells, Cell Separation, Biology, Colony-Forming Units Assay, Bone Marrow Purging, Bone Marrow Transplantation, Cell Adhesion, Cultured, Cyclophosphamide, Hematopoietic Stem Cells, Humans, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, Neoplastic Stem Cells, Tumor Cells, Tumor Stem Cell Assay, chemistry.chemical_compound, Mafosfamide, Leukemia, Myelogenous, Chronic, BCR-ABL Positive, Tumor Cells, Cultured, medicine, Progenitor cell, Clonogenic assay, Cells, Cultured, Hematology, medicine.disease, Molecular biology, Bone marrow purging, Oncology, chemistry, Chronic myelogenous leukemia

Abstract

Chronic myelogenous leukemia (CML) progenitor cells have been shown to be defective in their ability to adhere to marrow stroma. It was the aim of the present study to investigate at the cytogenetic level marrow-derived CML clonogenic cells fractionated on the basis of their ability to adhere to preformed, allogeneic, normal marrow-derived stromal layers. Mononuclear marrow cells from CML patients (n = 15) were incubated with mafosfamide (100 micrograms/ml) or control medium, seeded onto marrow stromal layers and allowed to adhere (3 hrs, 37 degrees C). Following a short-term liquid culture, the different cell fractions were harvested and incorporated in methylcellulose cultures. CFU-GM grown from these cultures were analyzed by single colony karyotyping. On direct cytogenetic analysis, the overall mean (+/- SD) percentage of Ph-negative metaphases was 7 +/- 20%. Following stroma adherence and shortterm suspension culture, the mean (+/- SD) percentages of Ph-negative clones were as follows: 33 +/- 25% for adherent CFU-GM, 59 +/- 40% for adherent, mafosfamide-treated CFU-GM, 12 +/- 16% for non-adherent CFU-GM, and 32 +/- 26% for non-adherent-mafosfamide-treated CFU-GM. If only the patients showing a percentage of Ph-negative clones > or = 20% were included in this analysis, the mean (+/- SD) percentages of Ph-negative clones were 47 +/- 19% for adherent CFU-GM, and 81 +/- 21% for adherent-Mafosfamide-treated CFU-GM. In contrast, the majority of pH-positive CFU-GM were detected within the stroma non-adherent cell fraction.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1993

49. Use of recombinant human granulocyte-macrophage colony-stimulating factor in patients with lymphoid malignancies transplanted with unpurged or adjusted-dose mafosfamide-purged autologous marrow

Author

Giovanna Meloni, Carmelo Carlo-Stella, Luca Cottafavi, Camillo Almici, Vittorio Rizzoli, Lina Mangoni, and Franco Mandelli

Subjects

Adult, Male, medicine.medical_specialty, Neutrophils, Microgram, medicine.medical_treatment, Immunology, Antineoplastic Agents, Transplantation, Autologous, Biochemistry, Gastroenterology, law.invention, Leukocyte Count, chemistry.chemical_compound, Mafosfamide, law, Internal medicine, medicine, Humans, Cyclophosphamide, Bone Marrow Transplantation, business.industry, Lymphoma, Non-Hodgkin, Bone Marrow Purging, Granulocyte-Macrophage Colony-Stimulating Factor, Cell Biology, Hematology, Immunotherapy, Precursor Cell Lymphoblastic Leukemia-Lymphoma, Hematopoietic Stem Cells, medicine.disease, Recombinant Proteins, Lymphoma, Transplantation, Granulocyte macrophage colony-stimulating factor, chemistry, Recombinant DNA, Absolute neutrophil count, Female, business, medicine.drug

Abstract

The neutropenia-related morbidity and mortality occurring after autologous bone marrow transplantation (ABMT) is increased by marrow purging procedures. While phase I through III clinical trials showed the enhancing activity of recombinant human granulocyte-macrophage colony-stimulating factor (rhGM-CSF) on neutrophil recovery after ABMT with unpurged marrow, controversial results have been reported when purged marrow was used. Therefore, it was the aim of the present study to evaluate the efficacy of rhGM-CSF administration in a group of patients (n = 15) with lymphoid malignancies transplanted in complete remission with mafosfamide-purged (n = 10) or unpurged (n = 5) marrow. Mafosfamide concentrations used for marrow purging were evaluated on an individual basis by means of a recently described technique that destroys the granulocyte-macrophage (granulocyte-macrophage colony- forming units [CFU-GM]) compartment, but spares 50% of the more primitive stroma adherent colony-forming cells (CFU-Blast). rhGM-CSF (10 micrograms/kg/d) was started within 24 hours of ABMT and administered in a 4-hour infusion daily until the absolute neutrophil count (ANC) reached 500 x 10(6)/L and then for 7 more days. Patients receiving mafosfamide-purged or unpurged marrow failed to show any difference in terms of median number of days required to achieve an ANC > or = 500 x 10(6) (13 v 14.0, P > .4) cells/L. As compared with retrospective controls, granulocytic recovery was reduced by a median time of 11 (P < or = .0005) and 5 (P < or = .0005) days for patients grafted with purged and unpurged marrow, respectively. The number of CFU-GM (mean +/- SD) infused per kilogram of body weight was significantly lower in patients who received purged autografts as compared with those receiving unpurged autografts (0.85 +/- 0.79 x 10(4) v 15.7 +/- 9.2 x 10(4), P < or = .0005). The dose of CFU-GM progenitors infused per kilogram of body weight did not correlate (r = .031, P > .05) with the time required to reach an ANC > or = 500 x 10(6) cells/L. The number of CFU-Blast (mean +/- SD) infused per kilogram of body weight was not significantly different between patients who received purged or unpurged autografts (5.05 +/- 2.51 x 10(3)/kg v 6.18 +/- 2.66 x 10(3)/kg, P < or = .375). A statistically significant correlation (r = -.658, P < or = .05) was observed between the number of CFU-Blast infused and the number of days required to reach an ANC > or = 500 x 10(6) cells/L.(ABSTRACT TRUNCATED AT 400 WORDS)

Published

1992

50. Trapianti da donatore a cuore fermo: il caso del paziente pediatrico

Author

Paola Delbon, Mirella Marini, Adelaide Conti, and Camillo Almici

Subjects

Philosophy, Issues, ethics and legal aspects, Health Policy, Medicine (miscellaneous)

Abstract

In presenza di grave insufficienza d’organo, il trapianto è la sola e unica soluzione per salvare la vita del paziente. Si stima che, attualmente, in Italia oltre 9.000 persone siano in lista d’attesa per un trapianto di organo: anche se vi è stato un incremento del numero di donazioni negli ultimi decenni, il gap tra donatori e pazienti in attesa è in continua crescita. Secondo la maggior parte delle società di trapiantologia, i donatori a cuore non battente (NHBD) possono essere una fonte di reperimento degli organi. Quanto la donazione da NHBD può ampliare il pool dei donatori? Quali sono i rischi legati al prelievo di organi da NHBD non solo per il donatore ma anche per il ricevente? Nel tentativo di chiarire almeno alcuni di tali interrogativi abbiamo condotto un’analisi della letteratura scientifica internazionale. Per valutare, poi, la possibilità di ampliamento del pool di donatori con l’introduzione di un protocollo da NHBD nella popolazione pediatrica del Policlinico “A. Gemelli” in Roma, abbiamo condotto uno studio retrospettivo sui pazienti pediatrici deceduti nel corso del triennio 2004-2007. I risultati sembrano indicare la possibilità di raddoppiare il potenziale pool di donatori; questi dati richiedono poi una valutazione attenta, innanzitutto alla luce delle percentuali di opposizione alla donazione che nell’età pediatrica sono ancora più significative che nell’adulto. I risultati ottenuti sono solo il punto di partenza per un’analisi più approfondita sui problemi relativi ai trapianti e alla donazione di organi. ---------- In case of end stage organ failure, organ transplantation is the one and only solution to save patient’s life. Currently, in Italy, more than 9.000 people are awaiting for an organ transplantation; even though the number of organ donation has been increasing during last decades, gap between organ demand and transplantation is still wide. According to ideas of most society of transplantation, non heart beating donors (NHBD) could be a solution to the shortage of organs. How much NHBD could widen donors pool? Which ones and how many risks involve NHBD, even for donors or transplantation recipients? Trying to answer these questions, we led an analysis on NHBD data in international literature. To evaluate the potential of NHBD to expand the pool of donors in pediatric population of “Policlinico Gemelli” in Rome, we studied all deceased pediatric patients in the years 2004-2007. Results showed that the potential pool of donors could be twice as much, but these data should esteem about parental opposition, in particular in pediatric age. These data represent only a starting point for a deeper analysis of transplantation and donation related problems.

Published

2009