Your search keyword '"Donatella Granchi"' showing total 243 results

51. No effect of methacrylate-based bone cement CMW 1 on the plasmatic phase of coagulation, red blood cells and endothelial cells in vitro

Author

Donatella Granchi, Alessandra Corradini, Lucia Savarino, Susanna Stea, Elisabetta Cenni, Gabriela Ciapetti, and Alessandro Di Leo

Subjects

Erythrocytes, Time Factors, Thrombomodulin, Drug Evaluation, Preclinical, Hemolysis, Thromboplastin, Immunoenzyme Techniques, Hemoglobins, Plasma, Tissue factor, Materials Testing, Humans, Polymethyl Methacrylate, Medicine, Orthopedics and Sports Medicine, Endothelium, Blood Coagulation, Chromatography, medicine.diagnostic_test, business.industry, Antithrombin, Bone Cements, Bone cement, Endothelial stem cell, Red blood cell, medicine.anatomical_structure, Biochemistry, Surgery, Human umbilical vein endothelial cell, Blood Coagulation Tests, business, medicine.drug, Partial thromboplastin time

Abstract

The compatibility of a methacrylate-based bone cement (CMW 1, DePuy International Ltd, England) used for the fixation of joint prostheses was evaluated on plasma, an erythrocyte suspension and cultured human endothelial cells. The extract of the cement was tested, following 1 hour and 7 days of curing. After the contact in vitro of the extract with plasma, activated partial thromboplastin time, antithrombin III, thrombin-antithrombin complexes and fibrin degradation products were assayed. Hemolytic activity was tested by adding the cement extracts to a suspension of erythrocytes. After 4 hours of incubation at 37 degrees C, the hemoglobin concentration was determined on the supernatants by the colorimetric method. The effect of the cement on tissue factor and thrombomodulin production was evaluated on human umbilical vein endothelial cell cultures. Tissue factor was determined in cell lysates by enzyme immunoassay, following 4 hours' incubation of cultures with the cement extract. Thrombomodulin was assayed in cell lysates by enzyme immuno assay, after 24 hours' incubation with the cement extract. The response to all trans-retinoic acid (ATRA) was tested. The cement caused no significant modifications of the coagulation tests, had no hemolytic activity, did not determine tissue factor production and did not modify thrombomodulin, compared to the negative control. The response to stimulation with ATRA was similar to that of the negative control. We conclude that the cement extract does not affect the plasmatic phase of coagulation, has no effect on erythrocytes, does not induce the expression of procoagulant activity by endothelial cells and does not impair their antithrombotic property, within the limits of the tests performed.

Published

2001

52. Expression of the CD69 activation antigen on lymphocytes of patients with hip prosthesis

Author

Susanna Stea, Armando Giunti, Federica Filippini, Lucia Savarino, Roberto Rotini, Gabriela Ciapetti, Alessandra Sudanese, and Donatella Granchi

Subjects

Antigens, Differentiation, T-Lymphocyte, Male, medicine.medical_specialty, Lymphocyte, medicine.medical_treatment, CD3, Biophysics, Urology, Bioengineering, Peripheral blood mononuclear cell, Prosthesis, Biomaterials, Antigen, Antigens, CD, medicine, Humans, Hypersensitivity, Delayed, Lectins, C-Type, Lymphocytes, Sensitization, Aged, biology, business.industry, Implant failure, Middle Aged, medicine.anatomical_structure, Mechanics of Materials, Immunology, Ceramics and Composites, biology.protein, Female, Hip Prosthesis, Implant, business

Abstract

The aim of the study was to evaluate the sensitization to metals in patients with Co-Cr hip prosthesis. Peripheral blood mononuclear cells (PBMC) were collected from 14 healthy donors and three groups of patients: 10 candidates for primary total joint replacements, 11 patients with well-fixed implant and 13 patients with aseptic loosening of the hip prosthesis. PBMCs were cultured with the metal ions employed for implant manufacturing and the expression of CD69 activation antigen on CD3/T lymphocytes was detected by flow cytometry. Chromium extract increased significantly the expression of CD3/CD69 phenotype in patients with loosening of hip prosthesis. The chromium-induced 'activation index' was higher in patients with loosening of hip prosthesis than in healthy donors and in pre-implant patients. The cobalt-stimulated PBMC of patients with either well-fixed or loosened prosthesis had an 'activation index' significantly higher than healthy donors. The activation index values were used to graduate the PBMC-response as 'normal' (or = 0.9 and2), 'low' (0.9) and 'high' (or = 2): an high-activation index was observed only in chromium-exposed PBMC of patients with prosthesis. Our data show that chromium released from orthopedic implants could be responsible for the lymphocyte sensitization and flow cytometry is an easy and reliable method for monitoring the hypersensitivity state in patients with metal prostheses. Activated lymphocytes in the peri-implant tissue are likely to elicit a localized immune response and contribute to maintain the inflammatory process evolving in the implant failure.

Published

2000

53. In vitro cytokine production by mononuclear cells exposed to bone cement extracts

Author

Donatella Granchi, Arturo Pizzoferrato, Federica Filippini, Susanna Stea, Aldo Toni, Elisabetta Cenni, and Gabriela Ciapetti

Subjects

medicine.medical_treatment, Biophysics, Biocompatible Materials, Bioengineering, Inflammation, Peripheral blood mononuclear cell, Monocytes, Bone resorption, Biomaterials, Blood cell, Immune system, medicine, Humans, Cells, Cultured, Interleukin-6, business.industry, Bone Cements, Granulocyte-Macrophage Colony-Stimulating Factor, Bone cement, medicine.anatomical_structure, Cytokine, Mechanics of Materials, Immunology, Ceramics and Composites, Cytokines, Tumor necrosis factor alpha, medicine.symptom, business, Interleukin-1

Abstract

The authors evaluated the ability of bone cement to modify the pro"le of pro-in#ammatory cytokines secreted by the immune cells. Peripheral blood mononuclear cells (PBMC) collected from healthy individuals were cultured with cement extracts and tested to assess the release of IL-1b, TNFa, GM-CSF and IL-6 in both unstimulated and PHA-stimulated PBMC. The cytokine release of unstimulated PBMC was very poor, and in particular the IL-1b was undetectable: the addition of cement extract increased both TNFa and GM-CSF release and decreased IL-6, sometimes signi"cantly. The most recurrent observation in PHA-stimulated PBMCs exposed to bone cement extract was the increase in both IL-1b and IL-6 release, while both the mean concentration and the index of release of TNFa and GM-CSF were changeable. In conclusion our results showed that leachable components of some bone cements can induce in vitro the release of pro-in#ammatory cytokines which are known to be involved in the bone resorption associated with aseptic loosening of hip prostheses. These "ndings allowed us to identify materials endowed with the highest in#ammatory power. ( 2000 Elsevier Science Ltd. All rights reserved.

Published

2000

54. Apoptosis in peri-implant tissue

Author

Alessandra Sudanese, Donatella Granchi, Aldo Toni, Elisabetta Cenni, Gabriela Ciapetti, M. Visentin, and S. Stea

Subjects

Male, Ceramics, Programmed cell death, medicine.medical_specialty, Pathology, Materials science, Biopsy, medicine.medical_treatment, Cell, Biophysics, Apoptosis, Bioengineering, DNA Fragmentation, Prosthesis, Biomaterials, medicine, Humans, Aged, medicine.diagnostic_test, Bone Cements, Acetabulum, Bone cement, Prosthesis Failure, Surgery, Corrosion, medicine.anatomical_structure, Terminal deoxynucleotidyl transferase, Metals, Polyethylene, Mechanics of Materials, Ceramics and Composites, Female, Hip Prosthesis, Implant, Plastics, Joint Capsule

Abstract

The authors examined 54 biopsies taken from the tissue surrounding loosened hip joint prostheses. In situ apoptotic cell identification was performed by the detection of single- and double-stranded DNA breaks that occurred in the early stages of apoptosis. Both types of breaks can be revealed by labeling the free 3′-OH termini with modified nucleotides (fluoresceine-dUTP) in an enzymatic reaction catalyzed by terminal deoxynucleotidyl transferase (TdT). Results were correlated with the presence of wear debris in the tissue and with the use of bone cement for prosthesis fixation. Apoptotic cells were present in a higher percentage in tissue sections where metal particles were present (24% apoptotic cells) if compared to areas where no wear (6%), or plastic wear (2.8%) or ceramic wear (1.5%) was observed. Apoptosis is neither related to bone cement, nor to the time it takes for the implant to fail. Cell death by apoptosis may be important in implants which release metal ions by corrosion or wear and may have been underestimated up to now, as it is a `clean’ way of cell death, leading to limited damage in the surrounding tissues.

Published

2000

55. Sister chromatid exchanges and ion release in patients wearing fracture fixation devices

Author

Donatella Granchi, Giuseppe Rollo, Aldo Toni, Lucia Savarino, Arturo Pizzoferrato, M. Elena Donati, Lucio Montanaro, Susanna Stea, Gabriela Ciapetti, M. Visentin, and Gianfranco Zinghi

Subjects

Adult, Chromium, Male, medicine.medical_specialty, Adolescent, Biomedical Engineering, chemistry.chemical_element, Sister chromatid exchange, Bone Nails, medicine.disease_cause, Biomaterials, Nickel, Reference Values, Fracture fixation, medicine, Humans, Lymphocytes, Fixation (histology), Chemistry, Spectrophotometry, Atomic, Radiochemistry, Middle Aged, Stainless Steel, Orthopedic Fixation Devices, Surgery, Toxicity, Female, Implant, Bone Plates, Sister Chromatid Exchange, Quantitative analysis (chemistry), Genotoxicity

Abstract

The quantification of sister chromatid exchange (SCE) during mitosis is a useful index for evaluating genotoxic effects in subjects occupationally or incidentally exposed to potentially toxic substances. The authors investigated the hypothesis that ions released by corrosion from prosthetic components of fracture fixation devices are associated with change in SCE incidence. In the present study, ten patients with implants were examined, and fifteen subjects with no implants were used as controls. SCE and high frequency cell (HFC) numbers were evaluated in circulating lymphocytes. In addition, nickel (Ni) and chromium (Cr) ion values in the serum were measured because, after iron, these metals are major components of stainless steel. A significant increase in SCE numbers was observed in patients compared to the control population (4.9 ± 1.3 vs. 3.5 ± 1.4). Ni concentration was 1.71 ± 1.49 ng/mL in patients and 0.72 ± 0.52 ng/mL in control subjects; Cr concentration was, respectively, 1.01 ± 0.77 ng/mL and 0.19 ± 0.27 ng/mL. The increase of serum Cr and Ni was statistically significant. No correlation was found between the increased Cr concentrations and SCE number while Cr ion levels were found to be significantly correlated to HFC. An inverse correlation between Ni level and SCE numbers was observed. Our findings suggest that Cr release by stainless steel implants could have a genotoxic effect; thus it would be useful to carefully monitor implanted subjects with regard to serum ion dosage, SCE analysis, and HFC evaluation. In any case, it would be appropriate to remove the implant when fracture fixation is reached. © 2000 John Wiley & Sons, Inc. J Biomed Mater Res, 50, 21–26, 2000.

Published

2000

56. Modulation of pro- and anti-apoptotic genes in lymphocytes exposed to bone cements

Author

Donatella Granchi, Elisabettacenni, Aldo Toni, Susanna Stea, Federica Filippini, Gabriela Ciapetti, and Arturo Pizzoferrato

Subjects

Time Factors, Cell Survival, Genes, myc, Biomedical Engineering, Biophysics, Down-Regulation, Apoptosis, Bioengineering, Biology, Polymerase Chain Reaction, Peripheral blood mononuclear cell, Proto-Oncogene Proteins c-myc, Biomaterials, chemistry.chemical_compound, Immune system, Annexin, Humans, Lymphocytes, Viability assay, Propidium iodide, Annexin A5, Phytohemagglutinins, Gene, Reverse Transcriptase Polymerase Chain Reaction, Caspase 1, Bone Cements, Flow Cytometry, Genes, p53, Molecular biology, Genes, bcl-2, Staining, Proto-Oncogene Proteins c-bcl-2, chemistry, RNA, Tumor Suppressor Protein p53, Propidium

Abstract

The ability of bone cements to modify the apoptotic program in activated immune cells and the mechanisms by which they act were evaluated. Mononuclear cells were collected from healthy individuals, cultured for 4 and 24 h with phytohemoagglutinina-P and cement extracts and then tested to assess: (a) cell viability; (b) early apoptotic events, by Annexin V/propidium iodide staining; and (c) the expression of pro- (p53, c-myc, ICE) and anti-apoptotic (bcl-2) genes. After 4 h three cements were able to increase significantly the percentage of apoptotic cells, while after 24 h no differences were found. The proportion of dead cells was not significantly changed at either culture time. The simultaneous expression of both pro-apoptotic (ICE, c-myc, p53) and antiapoptotic genes (bcl-2) was investigated only with regard to the materials which induced significant changes in apoptosis: two cements induced the p53 expression, while the third down-regulated bcl-2. As apoptosis regulates the balance of immune response, the authors recommend that the interaction between materials and immune cells should be assessed, so that the use of pro-apoptotic materials may be avoided in patients with immune defects.

Published

2000

57. Effects of metal ions on white blood cells of patients with failed total joint arthroplasties

Author

Donatella Granchi, Lucio Montanaro, Gianfranco Zinghi, S. Stea, G. Fontanesi, Gabriela Ciapetti, Roberto Rotini, Lucia Savarino, and M. E. Donati

Subjects

Adult, Male, Pathology, medicine.medical_specialty, medicine.medical_treatment, CD3, Biomedical Engineering, Biocompatible Materials, Prosthesis, Gastroenterology, Flow cytometry, Biomaterials, Immune system, Internal medicine, Leukocytes, medicine, Humans, Arthroplasty, Replacement, Aged, CD20, biology, medicine.diagnostic_test, business.industry, Middle Aged, Arthroplasty, Prosthesis Failure, Metals, biology.protein, Female, Joints, Implant, business, CD8

Abstract

In this study twenty-two patients who had revision surgery for aseptic loosening of joint prostheses were examined. The concentration in serum of soluble products of corrosion from the implant, that is, chromium (Cr), cobalt (Co), and nickel (Ni) ions, and the number of white blood cells (leucocytes, myeloid cells, lymphocyte subpopulations) were measured. Twenty patients with no implants were used as controls. The patients who had revision surgery showed normal Ni concentration whereas by statistical analysis that same patient group was shown to have serum Cr and Co levels significantly higher than those of the control. By flow cytometry, a significant decrease of leucocytes, myeloid cells, lymphocytes, and CD16 populations as found in patients versus controls whereas CD3, CD4, CD8, and CD20 positive cells were decreased, but not significantly. In the arthroplasty patients the Cr concentrations were inversely correlated with some of the immunologic parameters while no significant correlation was found between Co levels and decreased lymphocyte subpopulations. Only in revision surgery patients with high Cr concentrations did we find a significant decrease of lymphocytes, namely of CD4 and CD16 positive cells; revision surgery patients with normal Cr concentrations did not show a significant decrease of lymphocyte subpopulations. These data suggest that the presence of metal ions, especially chromium, released from prosthesis components could be associated with changes of lymphocyte subpopulations in patients with loosening of joint prostheses.

Published

1999

58. Established Cell Lines and Primary Cultures in Testing Medical Devices In Vitro

Author

Donatella Granchi, S. Stea, Elisabetta Cenni, Gabriela Ciapetti, Lucia Savarino, Lucio Montanaro, Carla Renata Arciola, and Arturo Pizzoferrato

Subjects

Cell type, Chemistry, medicine.medical_treatment, Osteoblast, General Medicine, Toxicology, Bone resorption, Cell biology, Endothelial stem cell, medicine.anatomical_structure, Cytokine, Cell culture, In vivo, Immunology, medicine, Cytotoxicity

Abstract

In testing for the cytotoxicity of medical devices, crucial parameters are the type of cells, the duration of the exposure, the physical form of the device and the method of evaluation. Using cell cultures the changes of cell functions induced by artificial materials may be evaluated. In screening tests the effect of biomaterials on functions common to all cell types is investigated through both continuous lines and primary cultures. In supplementary tests the effect of biomaterials on specific functions is studied, employing cells of the same type of those which will be in contact with the device in vivo. Osteoblasts, either from primary culture or an established line, are used to study the interaction with materials for bone implants. We evaluated whether dental cements affect the replication cycle of osteoblast-like cells MG63. The S phase was inhibited by the cements with a phenolic group, even though to a different extent. Mononuclear cell cultures are used to investigate the immune response, which is important in the host reaction to implant. We investigated whether the chromium ions released in a biological fluid may induce PBMC to produce cytokines involved in bone resorption. Chromium extract did not impair TNFα release significantly, but inhibited IL-6 release significantly in stimulated PBMC. Endothelial cell cultures are useful to the evaluation of materials for vascular grafts. We studied the influence of some types of Dacron on endothelial functions. Collagen-coated Dacron decreased significantly the production of 6-keto-prostaglandin F1α. Knitted Dacron caused a significant increase of tissue factor, a significant reduction in PECAM-1 and a significant increase in ELAM-1.

Published

1999

59. Cytokine release in mononuclear cells of patients with Co–Cr hip prosthesis

Author

Alessandra Sudanese, Susanna Stea, Lucio Montanaro, Lucia Savarino, Federica Filippini, Gianfranco Zinghi, Donatella Granchi, and Gabriela Ciapetti

Subjects

Adult, Chromium, Male, medicine.medical_specialty, Lymphocyte, medicine.medical_treatment, Metal Ceramic Alloys, Biophysics, Bioengineering, Lymphocyte Activation, Peripheral blood mononuclear cell, Monocytes, Biomaterials, Blood cell, Reference Values, Internal medicine, medicine, Humans, Lymphocytes, Cells, Cultured, Aged, Interleukin-6, Tumor Necrosis Factor-alpha, business.industry, Monocyte, Granulocyte-Macrophage Colony-Stimulating Factor, Cobalt, Middle Aged, Hypersensitivity reaction, medicine.anatomical_structure, Endocrinology, Cytokine, Mechanics of Materials, Delayed hypersensitivity, Immunology, Ceramics and Composites, Cytokines, Female, Tumor necrosis factor alpha, Hip Prosthesis, business

Abstract

The aim of this study was the evaluation of the release of bone-resorbing cytokines in peripheral blood mononuclear cells (PBMC) of patients with aseptic loosening of Co–Cr hip prostheses. TNF-α, IL-6, and GM-CSF were measured in both unstimulated and PHA-stimulated PBMC, and in PBMC cultured in the presence of chromium and cobalt extracts. Blood samples from healthy donors were used as controls. Serum samples of both patients and healthy donors were tested to determine the concentration of metal ions. The proportion of lymphocyte, monocyte and lympocyte subpopulation in cultured PBMC did not differ in patients and the control group. In unstimulated PBMC the release of TNF was significantly higher in patients than in the control group, while IL-6 was significantly decreased and no change was observed for GM-CSF. When the PBMC were challenged with chromium extract, all the ‘index of cytokine release’ resulted higher in patients than in the control group; cobalt extract increased both the TNF and GM-CSF index, but not the index of IL-6 release. Metal concentrations in serum from patients were significantly increased and correlated with the TNF release in PBMC stimulated with both metal extract. Our results suggest that a CoCr-implant releases a large amount of metal ions which could mediate the priming or the renewal of a cell-mediated hypersensitivity reaction. The prevalence of circulating lymphocytes responsible for the delayed hypersensitivity, namely Th1, would justify both the significant increase of TNF and the significant decrease of IL6 in unstimulated PBMC of patients, as well as the significant increase of the ‘index of cytokine release’ after the challenge with metal ions.

Published

1999

60. Cytotoxicity testing of materials with limitedin vivo exposure is affected by the duration of cell-material contact

Author

Gabriela Ciapetti, E. Verri, Lucia Savarino, Franca Savioli, Susanna Stea, A. Gori, Donatella Granchi, and Lucio Montanaro

Subjects

Neutral red, Materials science, Biocompatibility, Cell Survival, Silicones, Biomedical Engineering, Biocompatible Materials, Pharmacology, Biomaterials, Mice, chemistry.chemical_compound, L Cells, In vivo, Materials Testing, Animals, Cytotoxic T cell, Propidium iodide, Coloring Agents, Cytotoxicity, Dental Impression Materials, Amido Black, Staining, Dental impression, chemistry, Neutral Red, Propidium, Biomedical engineering

Abstract

Silicones for dental impression largely are used to record the geometry of hard and soft dental tissues. They are considered to be medical devices, and the assessment of cytotoxicity is a necessary step in the evaluation of their biocompatibility. Extracts of six addition-type and six condensation-type silicones have been tested with L929 cells according to the ISO 10993-Part 5 standard. The cytotoxicity was evaluated by three different methods: neutral red uptake, propidium iodide (PI) staining, and amido black staining. According to the selected specific assay, contact between cells and material extracts was maintained for 24 h in the first series of experiments; then, considering that in vivo application of these materials is restricted to a few minutes, additional experiments were performed after 1 h of cell/extract contact. Analysis of the results showed that the addition-type silicones are nontoxic even when tested after prolonged exposure of the cells to the materials while the condensation-type silicones were cytotoxic at 24 h of incubation. Nevertheless, harm to the patient actually could be negligible, considering its very short time of exposure in vivo. This is supported by our finding that most are not toxic after 1 h. We suggest that the experimental conditions of cytotoxicity testing have to be relevant to the in vivo situation; accordingly, the time of exposure should be designed carefully.

Published

1998

61. Fluorescent microplate assay for respiratory burst of PMNs challengedin vitro with orthopedic metals

Author

Gabriela Ciapetti, Donatella Granchi, E. Verri, Lucia Savarino, Franca Savioli, Elisabetta Cenni, and Arturo Pizzoferrato

Subjects

inorganic chemicals, Neutrophils, Biomedical Engineering, chemistry.chemical_element, Granulocyte, Biomaterials, Metal, Chromium, medicine, Humans, Respiratory Burst, chemistry.chemical_classification, Reactive oxygen species, Chromatography, Orthopedic Equipment, Reproducibility of Results, Fluoresceins, Fluorescence, In vitro, Respiratory burst, Kinetics, Spectrometry, Fluorescence, medicine.anatomical_structure, chemistry, Metals, visual_art, visual_art.visual_art_medium, Reactive Oxygen Species, Cobalt, Biomedical engineering

Abstract

This report describes a simple, rapid, automated microassay for measuring in vitro changes of oxidative burst of phagocytes following challenge with metals for orthopedic devices. The production of reactive oxygen species (ROS) by polymorphonuclear leukocytes (PMNs) was measured using 2′,7′-dichlorofluorescin-diacetate (DCFH-DA) as fluorescent probe. DCFH-DA enters the cells and is oxidized by ROS to fluorescent DCF. The DCF generated was directly proportional to ROS produced intracellularly: The fluorescence intensity was read and converted to an index of ROS production by cells. In our experimental system, granulocytes (PMNs) were isolated from normal human blood and seeded in microplates. To verify if metals could influence ROS production, chromium, cobalt, nickel, molybdenum, titanium, aluminum, and vanadium prepared as aqueous extracts in phosphate-buffered saline were tested onto PMNs using phorbolmyristate acetate (PMA) as positive control. Molybdenum, aluminum, and vanadium increased ROS generation by PMNs, while signals not different from unstimulated PMNs were recorded for chromium, cobalt, nickel, and titanium. The DCFH-DA microplate-based assay provides an in vitro tool for the detection of oxygen-reactive species generated by PMNs as a response to metals. © 1998 John Wiley & Sons, Inc. J Biomed Mater Res, 41, 455–460, 1998.

Published

1998

62. Flow-cytometric analysis of leukocyte activation induced by polyethylene-terephthalate with and without pyrolytic carbon coating

Author

Donatella Granchi, A. Gori, E. Verri, S. Gamberini, Gabriela Ciapetti, Elisabetta Cenni, and Arturo Pizzoferrato

Subjects

Materials science, biology, medicine.diagnostic_test, Cell adhesion molecule, Biomedical Engineering, CD18, CD11a, Molecular biology, In vitro, Flow cytometry, Biomaterials, chemistry.chemical_compound, Integrin alpha M, Antigen, chemistry, Immunology, biology.protein, medicine, Polyethylene terephthalate

Abstract

Leukocyte activation is one test for the evaluation of blood-materials interaction. The expression of adhesion molecules analyzed by flow cytometry provides a simple method to evaluate leukocyte activation by biomaterials: any change in these molecules can be predictive of the inflammatory activity of the materials. In this study the contact between leukocytes and uncoated polyethylene terephthalate or pyrolytic carbon-coated polyethylene terephthalate (PET and PET-PC, respectively) was inspected by analyzing whether the expression of some adhesion molecules involved in leukocyte activation, namely LFA-1 (CD11a/ CD18), Mac-1/CR3 (CD11b/CD18), and LECAM-1 (CD62L) can be modified. By flow cytometry expression of the adhesion molecules can be studied separately on lymphocytes and myeloid cells. The materials tested reduced the total numbers of both leukocytes and neutrophils, although not significantly. Neither PET nor PET-PC changed the expression of the adhesion molecules in lymphocytes: this suggests that no specific immune response is stimulated. On the contrary, statistically significant changes were observed for monocytes and granulocytes: the percentage of cells expressing Mac-1 and the density of such antigens on cell membranes increased while the percentage of LECAM-1 positive cells decreased. Similar changes were observed when the cells underwent the inflammatory stimulus provided by an in vitro challenge with bacterial endotoxin. Our results demonstrated that polyethylene terephthalate activates leukocytes by modifying the expression in neutrophils of the molecules involved in the early phase of the inflammatory response. Even after coating PET with pyrolytic carbon, the ability of this material to activate circulating leukocytes was maintained.

Published

1998

63. False positive results in cytotoxicity testing due to unexpectedly volatile compounds

Author

S. Stea, A. Gori, Arturo Pizzoferrato, Lucia Savarino, Franca Savioli, E. Verri, Gabriela Ciapetti, and Donatella Granchi

Subjects

Neutral red, Cell Survival, Biomedical Engineering, New materials, Cell Line, Biomaterials, Toxicology, Dental Materials, Mice, chemistry.chemical_compound, Materials Testing, Cytotoxicity testing, Animals, Viability assay, Coloring Agents, Cytotoxicity, Biological evaluation, Chromatography, Chemistry, In vitro, Neutral Red, Toxicity, Volatilization, Artifacts, Plastics, Propidium

Abstract

We investigated the cytotoxicity of different dental materials according to the study protocol adopted by our lab for the screening of new materials. Experimental parameters used in such testing are addressed mainly in documents EN 30993 “Biological evaluation of medical devices, Part 5: Tests for cytotoxicity: in vitro methods” and “Biological evaluation of medical devices, Part 12: Sample preparation and reference materials.” Cells were cultured in microplates and challenged with aqueous extracts of the materials. The assay methods were neutral red- and propidium iodide-uptake assays, both indicative of cell viability and able to provide quantitative data. The observation of contrasting results for one material using the above-mentioned methods raised some concern about the assay system used. With further experimentation, it appeared that a sustained release of volatile substances still present in one extract exerted a toxic effect in neighboring cultures. It is concluded that in the microenvironment of a microplate the distribution of samples cannot be disregarded, as it may be responsible for toxicity cross-contamination. Moreover, the use of more than one single method has to be recommended in cytotoxicity testing, in order to avoid false positive results due to experimental artifacts. © 1998 John Wiley & Sons, Inc. J Biomed Mater Res, 39, 286–291, 1998.

Published

1998

64. [Untitled]

Author

Guglielmo Paganetto, M. E. Donati, Adriana Moroni, A. Pizzoferrato, S. Stea, M. Cervellati, Lucia Savarino, and Donatella Granchi

Subjects

Materials science, Metallurgy, Biomedical Engineering, Biophysics, Bioengineering, Crystal structure, Bone tissue, Apatite, Bone remodeling, Biomaterials, Metal, medicine.anatomical_structure, visual_art, Fracture fixation, X-ray crystallography, visual_art.visual_art_medium, medicine, Implant, Composite material

Abstract

The microstructural characteristics of the newly formed bone tissue at the interface with hydroxyapatite-coated and uncoated stainless steel pins used in an external fracture fixation system have been evaluated. The bone far from the interface was used as a control. Pins were transversally inserted into the diaphyses of sheep tibiae and were loaded in for six weeks. Three sheep received coated pins and two received uncoated pins. Crystallographic habit and mineralization of the implant-facing bone were evaluated. Moreover, lattice parameters of bone apatite were measured and hydroxyapatite (HA) coating degradation was investigated, by means of conventional and microbeam X-ray diffraction (XRD). In coated pins, six weeks after the implantation the newly formed bone tissue at the interface did not reach complete maturation, but the presence of the implant did not alter the apatite lattice structure; the lattice parameters did not show statistically significant variations with respect to those observed in the control bone. In uncoated pins, bone tissue rarely appeared totally mineralized and lattice parameters were significantly different with respect to those observed in the bone far from the implant. HA particles were observed spreading in the bone-facing coated pins; the XRD pattern of bone apatite surrounding HA particles was unmodified. It was concluded that HA coatings improved the bone remodelling process during pin fixation in comparison to uncoated pins and did not alter the crystallographic habit of apatite. © 1998 Chapman & Hall

Published

1998

65. Adhesive protein expression on human endothelial cells after in vitro contact with woven Dacron

Author

A. Di Leo, E. Verri, A. Gori, S. Gamberini, Arturo Pizzoferrato, Gabriela Ciapetti, Elisabetta Cenni, and Donatella Granchi

Subjects

Endothelium, medicine.drug_class, Biophysics, Vascular Cell Adhesion Molecule-1, Biocompatible Materials, Bioengineering, Biology, Monoclonal antibody, Umbilical vein, Flow cytometry, Biomaterials, Antigen, Cell–cell interaction, Blood vessel prosthesis, Cell Adhesion, Leukocytes, medicine, Humans, Cells, Cultured, medicine.diagnostic_test, Flow Cytometry, Intercellular Adhesion Molecule-1, Molecular biology, Blood Vessel Prosthesis, Platelet Endothelial Cell Adhesion Molecule-1, Endothelial stem cell, medicine.anatomical_structure, Mechanics of Materials, cardiovascular system, Ceramics and Composites, Endothelium, Vascular, E-Selectin, Cell Adhesion Molecules

Abstract

In this research adhesive proteins are studied in order to evaluate the interference of woven Dacron in the endothelialization process and in the ability of endothelial cells to bind circulating leucocytes. Endothelial cells from human umbilical vein (HUVEC) were put in contact with woven Dacron for 24 h. PECAM-1, ELAM-1, ICAM-1 and VCAM-1 expression was then evaluated by flow cytometry, using indirect immunofluorescence reaction with monoclonal antibodies. The study of adhesive proteins was completed with the quantitative determination of surface antigens expressed as the antibody binding capacity (ABC). Antigenic density was calculated by the DAKO QFIT calibration system for indirect immunofluorescence. After contact with woven Dacron no significant change was observed in the percentage of positive cells or in the fluorescence intensity of the adhesins. No significant variation was also noted by calculating the surface antigen density by means of calibration fluorospheres. It can be concluded that the material examined does not significantly affect leucocyte adhesion to the endothelium.

Published

1998

66. CD62, thromboxane B2, and beta-thromboglobulin: A comparison between different markers of platelet activation after contact with biomaterials

Author

Donatella Granchi, Elisabetta Cenni, S. Gamberini, E. Verri, G. Falsone, D. Cavedagna, and Arturo Pizzoferrato

Subjects

medicine.medical_specialty, medicine.diagnostic_test, Biocompatibility, Chemistry, Biomedical Engineering, Biomaterial, Radioimmunoassay, Flow cytometry, Biomaterials, Thromboxane B2, chemistry.chemical_compound, Endocrinology, Biochemistry, Beta-thromboglobulin, Internal medicine, medicine, Platelet, Platelet activation

Abstract

The authors examined the modifications of some markers of platelet activation after contact with biomaterials. Glycoprotein GMP-140 (CD62) was evaluated by flow cytometry; β-thromboglobulin (β-TG) and thromboxane B2 (TXB2) were determined by radioimmunoassay. Polyethylene terephthalate (PET) induced a remarkable platelet adhesion and a significant increase in β-TG and TXB2, with no increase in CD62 on the nonadherent platelets. Pyrolytic carbon-coated PET (PC) did not induce platelet adhesion after 15 min of contact, but a significant increase in CD62 was detected. After 30 min a significant increase in platelet adhesion as well as the release of β-TG and TXB2 were noted. The increase was lower than that observed for uncoated PET, and after 30 min of contact with PC the increase no longer was observed. © 1997 John Wiley & Sons, Inc. J Biomed Mater Res, 36, 289–294, 1997.

Published

1997

67. [Untitled]

Author

A. Gori, Elisabetta Cenni, S. Gamberini, P Zucchelli, Gabriela Ciapetti, Donatella Granchi, E. Verri, S. Stea, and Arturo Pizzoferrato

Subjects

chemistry.chemical_classification, Materials science, Biomedical Engineering, Biophysics, Bioengineering, engineering.material, In vitro, Complement system, Biomaterials, chemistry.chemical_compound, Enzyme, chemistry, Coating, Polymer chemistry, Alternative complement pathway, engineering, Polyethylene terephthalate, Pyrolytic carbon, Nuclear chemistry, Whole blood

Abstract

This study was undertaken to evaluate whether the pyrolytic carbon coating of polyethylene terephthalate induces complement activation. Complement activation induced by pyrolytic carbon-coated polyethylene terephthalate (PET+PC) in comparison with uncoated polyethylene terephthalate (PET) was assessed on whole blood collected with heparin. The activation of the classic pathway was evaluated by C4d fragment enzyme immunoassay. The activation of the alternative pathway was evaluated with Bb fragment enzyme immunoassay. The results show that uncoated PET activates the alternative pathway, but not the classic one. PET+PC does not induce complement activation, not even through the alternative pathway. Pyrolytic carbon coating therefore contributes to improving blood compatibility.

Published

1997

68. Low toxicity and unprecedented anti-osteoclast activity of a simple sulfur-containing gem-bisphosphonate: A comparative study

Author

Alessandro Scarso, Giulio Bianchini, Rino A. Michelin, Andrea Chiminazzo, Giorgio Strukul, Sofia Avnet, Gemma Di Pompo, Donatella Granchi, Alberto Minto, Paolo Sgarbossa, Granchi D., Scarso A., Bianchini G., Chiminazzo A., Minto A., Sgarbossa P., Michelin R.A., Di Pompo G., Avnet S., and Strukul G.

Subjects

Cytotoxicity, medicine.medical_treatment, Osteoclasts, Apoptosis, urologic and male genital diseases, Settore CHIM/04 - Chimica Industriale, Bone resorption, bisphosphonates S coumpounds osteoclast inhibition, Mice, Structure-Activity Relationship, Osteoclast, Drug Discovery, medicine, Animals, Bisphosphonate, Structure–activity relationship, bisphosphonates, cytotoxicity, Cells, Cultured, Pharmacology, Diphosphonates, Dose-Response Relationship, Drug, Molecular Structure, Animal, Chemistry, Organic Chemistry, Apoptosi, Biological activity, General Medicine, Settore CHIM/06 - Chimica Organica, S-containing drug, Molecular Weight, medicine.anatomical_structure, Diphosphonate, Biochemistry, Michael reaction, Collagen, Sulfur, hormones, hormone substitutes, and hormone antagonists

Abstract

Bisphosphonates (BPs) are key drugs for the treatment of bone resorption diseases like osteoporosis, Paget's disease and some forms of tumors. Recent findings underlined the importance of lipophilic N-containing BPs to ensure high biological activity. Herein we present some unprecedented results concerning the low toxicity and good anti-osteoclast activity of low molecular weight hydrophilic S-containing BPs. A series of S and N-containing BPs bearing aromatic and aliphatic substitution were prepared through Michael addition reaction between vinylidenebisphosphonate tetraethyl ester and the proper nucleophile under basic catalysis. S-containing BPs showed a generally low toxicity, determined with the neutral-red assay using the L929 cell line, and, in particular for an aliphatic one, a good biological activity assessed on primary cultures of human osteoclasts. © 2013 Elsevier Masson SAS. All rights reserved.

Published

2013

69. Preparation method and growth factor content of platelet concentrate influence the osteogenic differentiation of bone marrow stromal cells

Author

Donatella Granchi, Erminia Mariani, Valentina Devescovi, Loredana Pratelli, Nicola Baldini, Elizaveta Kon, Annarita Cenacchi, Maurilio Marcacci, Francesca Perut, Giuseppe Filardo, Andrea Facchini, Perut F, Filardo G, Mariani E, Cenacchi A, Pratelli L, Devescovi V, Kon E, Marcacci M, Facchini A, Baldini N, and Granchi D

Subjects

Male, Cancer Research, medicine.medical_treatment, Cellular differentiation, Basic fibroblast growth factor, Cell Culture Techniques, chemistry.chemical_compound, 0302 clinical medicine, Osteogenesis, Leukocytes cytology/metabolism, Leukocytes, Immunology and Allergy, Platelet, platelet concentrate, Genetics (clinical), 0303 health sciences, Chemistry, Platelet-Rich Plasma, Osteogenesi, Cell Differentiation, 3. Good health, medicine.anatomical_structure, Oncology, 030220 oncology & carcinogenesis, Intercellular Signaling Peptides and Proteins, Blood Platelets cytology/metabolism, Cell Culture Technique, Mesenchymal Stromal Cells cytology/metabolism, Human, Blood Platelets, Adult, Intercellular Signaling Peptides and Proteins metabolism, Stromal cell, Immunology, osteogenic differentiation, Bone healing, Andrology, 03 medical and health sciences, medicine, Humans, 030304 developmental biology, Transplantation, Growth factor, Mesenchymal Stem Cells, Cell Biology, Platelet-Rich Plasma metabolism, Platelet-rich plasma, preparation method, Bone marrow

Abstract

BACKGROUND AIMS: An extensive debate about the clinical benefits of autologous platelet concentrates used as a treatment option for patients with orthopedic injuries is ongoing. The aim of this study was to determine whether different compositions of platelet concentrates may affect the osteogenic differentiation of bone marrow stromal cells (BMSC). METHODS: Pure platelet-rich plasma (P-PRP) and leukocyte-PRP (L-PRP) were characterized for platelet and leukocyte content. As an indicative marker of the delivery of growth factors (GFs), the release of basic fibroblast growth factor (bFGF) from platelet gel (PG) was measured at 1, 18, 48 and 72 h and at 7 d. The ability of different PGs to induce proliferation and differentiation of BMSC was evaluated by using bioactivity assays. RESULTS: The platelet recovery was significantly higher in L-PRP, either fresh or frozen. PGs derived from L-PRP and P-PRP showed significant differences in terms of bFGF release and biological activity. bFGF release was faster both in fresh and frozen L-PRP preparations. Moreover, L-PRP samples were able to induce a significantly higher proliferation of BMSC compared with P-PRP or PPP samples. Even though all PG preparations allowed the deposition of mineral nodules in BMSC cultures, the mineralization activity correlated significantly with bFGF levels. CONCLUSIONS: The biological activity of platelet concentrates differs according to preparation technique, which affects platelet and leukocyte content and GF availability. Because GF levels are not always optimal in subjects with defective bone healing, composition and bioactivity of PRP should be analyzed to test the reliability and potential effectiveness of the regenerative treatment. Copyright © 2013 International Society for Cellular Therapy. Published by Elsevier Inc. All rights reserved

Published

2013

70. Application of a combination of neutral red and amido black staining for rapid, reliable cytotoxicity testing of biomaterials

Author

Gabriela Ciapetti, Lucia Savarino, and Donatella Granchi

Subjects

Biomaterials, Mechanics of Materials, Biophysics, Ceramics and Composites, Bioengineering

Published

1996

71. In vitro assessment of phagocytosis of bovine collagen by human monocytes/ macrophages using a spectrophotometric method

Author

Donatella Granchi, Gabriela Ciapetti, Arturo Pizzoferrato, E. Verri, S. Gamberini, Elisabetta Cenni, M. Mian, and D. Benetti

Subjects

Lipopolysaccharides, Surgical Sponges, Phagocytosis, Biophysics, Bioengineering, Cell Separation, Biology, Monocytes, Biomaterials, chemistry.chemical_compound, Picrates, medicine, Animals, Humans, Macrophage, Coloring Agents, Sirius Red, Cells, Cultured, Analysis of Variance, Wound Healing, Histocytochemistry, Macrophages, Monocyte, Biomaterial, Molecular biology, In vitro, medicine.anatomical_structure, chemistry, Mechanics of Materials, Cell culture, Immunology, Ceramics and Composites, Cattle, Indicators and Reagents, Spectrophotometry, Ultraviolet, Collagen, Wound healing, Azo Compounds

Abstract

The use of a wound dressing with covering and haemostatic properties significantly improves wound healing. In this study, a lyophilized bovine collagen sponge used for the treatment of wounds and ulcerae has been tested in a cell culture system. Phagocytosis of collagen fragments by human blood monocytes/macrophages has been investigated. For the assessment of collagen ingestion by mononuclear phagocytes, a picrosirius dye specific for collagen molecules has been used. By adapting this histochemical technique to microplate cell culture system, replicate monocyte cultures are assayed. Collagen content is determined by evaluating spectrophotometrically at 540 nm the absorbance of a sirius red/picric acid solution. Using this simple and sensitive method, the phagocytosis of bovine collagen by LPS-stimulated monocytes/macrophages has been ascertained.

Published

1996

72. In vitro effects of bone cements on the cell cycle of osteoblast-like cells

Author

D. Cavedagna, Lucia Savarino, Donatella Granchi, S. Stea, Gabriela Ciapetti, and Arturo Pizzoferrato

Subjects

Materials science, Biophysics, Bone Neoplasms, Bioengineering, Flow cytometry, Biomaterials, chemistry.chemical_compound, Tumor Cells, Cultured, medicine, Humans, Propidium iodide, Osteosarcoma, Osteoblasts, medicine.diagnostic_test, Cell growth, Cell Cycle, Bone Cements, Osteoblast, Cell cycle, Flow Cytometry, Molecular biology, In vitro, medicine.anatomical_structure, chemistry, Polymerization, Mechanics of Materials, Toxicity, Ceramics and Composites, Cell Division, Biomedical engineering

Abstract

The effects of orthopaedic cements on the proliferation and cell cycle of in vitro cultured MG63 osteoblast-like cells were examined. Five different cements were mixed and extracted at different time intervals (15 and 60 min, 6, 24 and 48 h). Cell proliferation inhibition (CPI) was evaluated after 72 h culture as the toxicity parameter. As for the toxicity degree, the extracts were considered to have ‘high toxicity’ (CPI ⩾ 50%), ‘medium toxicity’ (50% > CPI > 25%), ‘slow toxicity’ (CPI ⩽ 25%) and ‘no toxicity’ (CPI = 0). Cell cycle phases of MG63 cells were evaluated at 24, 48 and 72 h by flow cytometry; the DNA content was assessed using the propidium iodide uptake and the percentage of cells in the S phase was determined using 5′-bromodeoxyuridine uptake. According to our results, the toxicity is inversely correlated with the time interval between polymerization and extract preparation, and is different according to the cement type. For some cements the effects are still observed 48 h after polymerization. The damaging effect is not linked to a specific phase of the cell cycle, nor does it hamper the restarting of cell proliferation at 72 h.

Published

1995

73. Assessment of viability and proliferation ofin vivo silicone-primed lymphocytes afterin vitro re-exposure to silicone

Author

Gabriela Ciapetti, P. Schiavon, R. Giuliani, Elisabetta Cenni, Arturo Pizzoferrato, Donatella Granchi, and Susanna Stea

Subjects

Adult, medicine.medical_specialty, Pathology, Cell Survival, Breast Implants, Lymphocyte, Population, Silicones, Biomedical Engineering, Tetrazolium Salts, Biomaterials, Andrology, chemistry.chemical_compound, Silicone, In vivo, medicine, Humans, MTT assay, Breast, Dimethylpolysiloxanes, Lymphocytes, education, Breast augmentation, education.field_of_study, business.industry, technology, industry, and agriculture, Middle Aged, In vitro, Plastic surgery, medicine.anatomical_structure, chemistry, Female, Lymphocyte Culture Test, Mixed, business, Cell Division

Abstract

The functional response of peripheral blood lymphocytes isolated from 22 patients with silicone gel-filled breast implants was assessed after in vitro re-exposure to silicone. Using cell culture test methods to quantify proliferation and viability and/or activation of lymphocyte microcultures, i.e., the uptake of tritiated thymidine (3H-TdR uptake test) and the reduction of formazan salts (MTT assay), interesting data were obtained. Peripheral blood lymphocytes purified from patients wearing silicone gel-filled breast implants react in vitro to silicone showing a statistically significant increase of both proliferation and viability, while healthy subjects do not respond on in vitro exposure to silicone. Differences resulted even more statistically significant when patients were divided into two groups depending on the type of surgery they underwent: patients with breast augmentation for aesthetic reasons seem to have an increased responsiveness in vitro to silicone compared to patients who experienced a reconstructive surgery of the breast. Although they are still preliminary, being referred to a limited population, these results suggest that the lymphocytes of patients with silicone gel-filled breast implants could be sensitized in vivo toward silicone; the re-exposure of these cells to silicone leads to a higher functional response which could be looked for by using quantitative in vitro test methods. © 1995 John Wiley & Sons, Inc.

Published

1995

74. Endodontic cements induce alterations in the cell cycle of in vitro cultured osteoblasts

Author

S. Stea, Donatella Granchi, D. Cavedagna, Susanna Stea, Arturo Pizzoferrato, and Gabriela Ciapetti

Subjects

Root canal, Dental Cements, Dentistry, Biology, Cell Line, Flow cytometry, Calcium Hydroxide, Root Canal Filling Materials, chemistry.chemical_compound, medicine, Humans, Propidium iodide, Zinc Oxide-Eugenol Cement, General Dentistry, Analysis of Variance, Osteoblasts, medicine.diagnostic_test, Cell growth, business.industry, Cell Cycle, Osteoblast, DNA, Cell cycle, Flow Cytometry, Molecular biology, In vitro, medicine.anatomical_structure, Otorhinolaryngology, chemistry, Cell culture, Surgery, Oral Surgery, business, Periapical Granuloma, Cell Division

Abstract

The effects of endodontic cements on the cell cycle of MG63 osteoblasts cultured in vitro have been examined. Three groups of compounds were tested. Group I encompassed zinc oxide- and eugenol-based cements (Tubliseal, Argoseal, N2), group II consisted of cements with a phenol group other than eugenol (AH26, Forfenan, Methode R/R), and group III included CaOH-based cements (Biocalex, Endocalex). The cell cycle of MG63 cells was analyzed by flow cytometry; the DNA content was evaluated by means of the propidium iodide uptake method, whereas the proportion of cells in the S phase was defined by the incorporation of bromodeoxyuridine later revealed by a specific antibody. The results showed that some root canal sealers could hamper the periapex healing processes by inhibiting the cell proliferation through a selective action on different phases of the cell cycle.

Published

1995

75. Adhesive protein expression on endothelial cells after contact in vitro with polyethylene terephthalate coated with pyrolytic carbon

Author

Elisabetta Cenni, Donatella Granchi, Lucia Savarino, D. Cavedagna, Arturo Pizzoferrato, Carla Renata Arciola, S. Stea, A. Di Leo, and Gabriela Ciapetti

Subjects

Materials science, Endothelium, Biophysics, Antigens, Differentiation, Myelomonocytic, Vascular Cell Adhesion Molecule-1, Biocompatible Materials, Bioengineering, In Vitro Techniques, Umbilical vein, Flow cytometry, Biomaterials, Blood vessel prosthesis, Materials Testing, Cell Adhesion, medicine, Humans, Cell adhesion, Cells, Cultured, medicine.diagnostic_test, Polyethylene Terephthalates, Adhesion, Intercellular Adhesion Molecule-1, Molecular biology, Carbon, Blood Vessel Prosthesis, Platelet Endothelial Cell Adhesion Molecule-1, Endothelial stem cell, Kinetics, medicine.anatomical_structure, Biochemistry, Mechanics of Materials, Cell culture, cardiovascular system, Ceramics and Composites, Endothelium, Vascular, E-Selectin, Cell Adhesion Molecules

Abstract

This research aims at evaluating the expression of some adhesive proteins on endothelial cell surface after contact with polyethylene terephthalate coated with pyrolytic carbon (PET + PC). Twenty-two different cultures of human umbilical vein endothelial cells (HUVECs) were put in contact with PET + PC. Both HUVECs grown without the biomaterial and HUVECs incubated with endotoxin were used as control. After 24 h, platelet endothelial cell adhesion molecule-1 (PECAM-1), endothelial leucocyte adhesion molecule-1 (ELAM-1), intercellular adhesion molecule-1 (ICAM-1) and vascular cell adhesion molecule-1 (VCAM-1) were evaluated on the cells by monoclonal antibodies and flow cytometry. In agreement with the literature, after 24 h the culture incubated with endotoxin determined a significant increase in the percentage of positive cells for ELAM-1, a significant increase in fluorescence intensity for ICAM-1, and a significant increase in the percentage of positive cells and fluorescence intensity for VCAM-1. After 24 h of culture with PET + PC, no significant variations in the antigens examined were observed. This demonstrates that such material does not activate in vitro the proteins involved in the adhesion between leucocytes and endothelium or in the adhesion between endothelial cells themselves.

Published

1995

76. Metal hypersensitivity testing in patients undergoing joint replacement: a systematic review

Author

Nicola Baldini, Elisabetta Cenni, Armando Giunti, Donatella Granchi, Granchi D, Cenni E, Giunti A, and Baldini N

Subjects

joint replacement, medicine.medical_specialty, Allergy, Joint replacement, medicine.medical_treatment, Joint Prosthesis, MEDLINE, Metal hypersensitivity, Internal medicine, Hypersensitivity, Medicine, Humans, Orthopedics and Sports Medicine, Arthroplasty, Replacement, Skin Tests, business.industry, Implant failure, Odds ratio, medicine.disease, Arthroplasty, Confidence interval, Surgery, Prosthesis Failure, Metals, Meta-analysis, Preoperative Period, business

Abstract

We report a systematic review and meta-analysis of the peer-reviewed literature focusing on metal sensitivity testing in patients undergoing total joint replacement (TJR). Our purpose was to assess the risk of developing metal hypersensitivity post-operatively and its relationship with outcome and to investigate the advantages of performing hypersensitivity testing. We undertook a comprehensive search of the citations quoted in PubMed and EMBASE: 22 articles (comprising 3634 patients) met the inclusion criteria. The frequency of positive tests increased after TJR, especially in patients with implant failure or a metal-on-metal coupling. The probability of developing a metal allergy was higher post-operatively (odds ratio (OR) 1.52 (95% confidence interval (CI) 1.06 to 2.31)), and the risk was further increased when failed implants were compared with stable TJRs (OR 2.76 (95% CI 1.14 to 6.70)). Hypersensitivity testing was not able to discriminate between stable and failed TJRs, as its predictive value was not statistically proven. However, it is generally thought that hypersensitivity testing should be performed in patients with a history of metal allergy and in failed TJRs, especially with metal-on-metal implants and when the cause of the loosening is doubtful.

Published

2012

77. Enhancing Osteoconduction of PLLA-Based Nanocomposite Scaffolds for Bone Regeneration Using Different Biomimetic Signals to MSCs

Author

Elisa Leonardi, Gabriela Ciapetti, Maria Jesus Jurado, Serena Rubina Baglìo, Donatella Granchi, Frank Walboomers, Desiree Martini, Nicola Baldini, Valentina Devescovi, Jose Inaki Marquinez Alava, Ilaria Armentano, Jose Maria Kenny, Beatriz Olalde, Pathology, Amsterdam Neuroscience - Cellular & Molecular Mechanisms, AII - Cancer immunology, Ciapetti G, Granchi D, Devescovi V, Baglio SR, Leonardi E, Martini D, Jurado MJ, Olalde B, Armentano I, Kenny JM, Walboomers FX, Alava JI, and Baldini N.

Subjects

Male, Bone Regeneration, Polymers, Cellular differentiation, Cell Culture Techniques, Biomimetic signal, Osteoconduction, Nanocomposites, lcsh:Chemistry, Tissue engineering, Biomimetic Materials, Osteogenesis, bone tissue engineering, lcsh:QH301-705.5, Spectroscopy, Cells, Cultured, mesenchymal stem cell, Nanocomposite, Tissue Scaffolds, Chemistry, Cell Differentiation, General Medicine, Middle Aged, Computer Science Applications, medicine.anatomical_structure, Female, biomimetic nanocomposites, Signal Transduction, Polyesters, Nanotechnology, Bone morphogenetic protein 2, Catalysis, Article, Inorganic Chemistry, medicine, Humans, Lactic Acid, Physical and Theoretical Chemistry, Bone regeneration, Molecular Biology, Aged, Cell Proliferation, Osteoblasts, Tissue Engineering, Guided Tissue Regeneration, Organic Chemistry, Mesenchymal stem cell, Mesenchymal Stem Cells, In vitro, lcsh:Biology (General), lcsh:QD1-999, Cell culture, Biophysics, Bone marrow

Abstract

In bone engineering, the adhesion, proliferation and differentiation of mesenchymal stromal cells rely on signaling from chemico-physical structure of the substrate, therefore prompting the design of mimetic “extracellular matrix”-like scaffolds. In this study, three-dimensional porous poly-L-lactic acid (PLLA)-based scaffolds have been mixed with different components, including single walled carbon nanotubes (CNT), micro-hydroxyapatite particles (HA), and BMP2, and treated with plasma (PT), to obtain four different nanocomposites: PLLA + CNT, PLLA + CNTHA, PLLA + CNT + HA + BMP2 and PLLA + CNT + HA + PT. Adult bone marrow mesenchymal stromal cells (MSCs) were derived from the femur of orthopaedic patients, seeded on the scaffolds and cultured under osteogenic induction up to differentiation and mineralization. The release of specific metabolites and temporal gene expression profiles of marrow-derived osteoprogenitors were analyzed at definite time points, relevant to in vitro culture as well asin vivo differentiation. As a result, the role of the different biomimetic components added to the PLLA matrix was deciphered, with BMP2-added scaffolds showing the highest biomimetic activity on cells differentiating to mature osteoblasts. The modification of a polymeric scaffold with reinforcing components which also work as biomimetic cues for cells can effectively direct osteoprogenitor cells differentiation, so as to shorten the time required for mineralization. EU STRP516943

Published

2012

78. The Combined Use of Mesenchymal Stromal Cells and Scaffolds for Bone Repair

Author

Nicola Baldini, Gabriela Ciapetti, Donatella Granchi, Ciapetti G, Granchi D, and Baldini N.

Subjects

Adult, BONE TISSUE ENGINEERING, Pathology, medicine.medical_specialty, medicine.medical_treatment, Clinical uses of mesenchymal stem cells, SCAFFOLDS, Bone and Bones, Cell therapy, Osteogenesis, Drug Discovery, Medicine, Humans, Progenitor cell, Bone regeneration, Pharmacology, Tissue Engineering, Tissue Scaffolds, business.industry, Regeneration (biology), Mesenchymal stem cell, Mesenchymal Stem Cells, Stem-cell therapy, mesenchymal stromal cell, Cancer research, Stem cell, business

Abstract

A general principle of stem cell therapy is to exploit the natural ability of the human body to heal through the process of regeneration. Here, we review the current status of cell therapy based on adult mesenchymal stem cells (MSC) with emphasis on therapeutic application in bone-related diseases. The main issues for an effective bone engineering strategy include: - A sufficient number of bone-forming cells, where cell yield, separation, expansion, commitment, as well as patient age, are all variables to be considered; - An ECM-like scaffold conductive for and informative to cells, where structural/physico-chemical/mechanical parameters, administration form (injectable or free-form), and degradation rate have to be tuned according to the clinical application; - Biochemical signals, such as growth factors/cytokines to induce osteogenic differentiation, where the choice between autogenous or exogenous sourcing, dose, timing, etc. are critical; - An adequate blood supply, provided by angiogenetic factors, pre-vascularization, pre-implant co-culture of vessel and bone progenitors. We also discuss the safety and efficacy of different approaches, as well as bottlenecks hampering rapid translation of adult MSC therapy from the laboratories to the clinics. A central paradigm for the effective regeneration of bone tissue is the re-creation at the site of injury of a microenvironment as close as possible to the natural MSC repository in the body. This would allow adult MSC to serve as cellular factories, i.e. to express paracrine activity in situ by secretion of inflammatory and reparative cytokines and to cooperate with other cells. The results from a wide array of in vitro and in vivo studies, as well as from some clinical trials, are expanding the range of clinical protocols for bone repair, that is the ultimate goal of orthopaedics.

Published

2012

79. The Effect of Poly(d,l-Lactide-co-Glycolide)-Alendronate Conjugate Nanoparticles on Human Osteoclast Precursors

Author

Caterina Fotia, Elisabetta Cenni, Dorotea Micieli, Donatella Granchi, Maria Grazia Sarpietro, Francesco Castelli, Sofia Avnet, Nicola Baldini, Manuela Salerno, Rosario Pignatello, Cenni E, Avnet S, Granchi D, Fotia C, Salerno M, Micieli D, Sarpietro MG, Pignatello R, Castelli F, and Baldini N

Subjects

inorganic chemicals, Materials science, Stereochemistry, medicine.medical_treatment, Proton Magnetic Resonance Spectroscopy, Biomedical Engineering, Biophysics, Nanoparticle, Osteoclasts, Bioengineering, Apoptosis, Bone Neoplasms, macromolecular substances, Conjugated system, Collagen Type I, Biomaterials, chemistry.chemical_compound, l-Lactide-co-Glycolide), Polylactic Acid-Polyglycolic Acid Copolymer, bone metastases, Osteoclast, medicine, NANOPARTICLES, Humans, Doxorubicin, Lactic Acid, Poly(d, ALENDRONATE, Cells, Cultured, health care economics and organizations, Bone Density Conservation Agents, Dose-Response Relationship, Drug, technology, industry, and agriculture, Bisphosphonate, respiratory system, Actins, PLGA, medicine.anatomical_structure, chemistry, Proteolysis, Polyglycolic Acid, medicine.drug, Conjugate

Abstract

Nanoparticles (NPs) formed from polymers conjugated with bisphosphonates (BPs) allow the bone targeting of loaded drugs, such as doxorubicin, for the treatment of skeletal tumours. The additional antiosteoclastic effect of the conjugated BP could contribute to the inhibition of tumour-associated bone degradation. With this aim, we have produced NPs made of poly(d,l-lactide-co-glycolide) (PLGA) conjugated with alendronate (ALE). To show if ALE retained the antiosteoclastic properties after the conjugation with PLGA and the production of NPs, we treated human osteoclasts, derived from circulating precursors, with PLGA-ALE NPs and compared the effects on actin ring generation, apoptosis and type-I collagen degradation with those of free ALE and with NPs made of pure PLGA. PLGA-ALE NPs disrupted actin ring, induced apoptosis and inhibited collagen degradation. Unexpectedly, also NPs made of pure PLGA showed similar effects. Therefore, we cannot exclude that in addition to the observed antiosteoclastic activity dependent on ALE in PLGA-ALE NPs, there was also an effect due to pure PLGA. Still, as PLGA-ALE NPs are intended for the loading with drugs for the treatment of osteolytic bone metastases, the additional antiosteoclastic effect of PLGA-ALE NPs, and even of PLGA, may contribute to the inhibition of the disease-associated bone degradation.

Published

2012

80. The natural compound Alizarin as an osteotropic drug for the treatment of bone tumors

Author

Donatella Granchi, Sofia Avnet, Nicola Baldini, Caterina Fotia, Fotia C, Avnet S, Granchi D, and Baldini N.

Subjects

MAP Kinase Signaling System, Anthraquinones, Bone Marrow Cells, Bone Neoplasms, Breast Neoplasms, Alizarin, medicine.disease_cause, chemistry.chemical_compound, Breast cancer, Cell Line, Tumor, medicine, Humans, Orthopedics and Sports Medicine, Bone tumor, Osteosarcoma, Bone cancer, Cell growth, Carcinoma, Cell Cycle, Cell cycle, medicine.disease, Cell Transformation, Neoplastic, chemistry, Cell culture, Immunology, Cancer research, osteotropism, sense organs, Drug Screening Assays, Antitumor, Carcinogenesis

Abstract

Despite significant clinical improvements, conventional therapies for bone cancer treatment are limited by significant systemic toxicity and lack of specific targeting. In this study, we considered Alizarin, a natural hydroxyanthraquinone derived from madder root with high affinity to calcium and remarkable osteotropic features, as a novel approach for bone cancer treatment. Due to its antitumor properties, as demostrated in colon cancer cells, and to its tropism to bone, Alizarin may be an ideal drug to reduce bone tumor growth. We demonstrated that low dosages of Alizarin strongly inhibited the osteosarcoma (IC50 for Saos-2, MG-63, and U-2 OS cells, 27.5, 29.0, and 69.9 µg/ml, respectively) and breast carcinoma (IC50 for MDA-MB-231 cells, 62.1 µg/ml) cell proliferation in vitro. Importantly, Alizarin had a significantly lower inhibitory activity on normal cells (IC50 for MSC, 828.6 µg/ml), thereby revealing a selective activity towards malignant cells. Furthermore, we found that Alizarin acted through the inhibition of ERK phosphorylation and cell cycle arrest in the S-phase. Finally, Alizarin significantly and strongly impaired both osteosarcoma and breast cancer tumorigenesis. Our results highlight a selective and effective inhibitory activity of Alizarin towards cancerous cells, laying the basis for further studies to investigate its application in bone cancer therapy. © 2012 Orthopaedic Research Society. Published by Wiley Periodicals, Inc. J Orthop Res 30:1486–1492, 2012

Published

2012

81. In vitro assessment of lymphocytes response following re-exposure to silicone

Author

R. Giuliani, M. E. Donati, P. Schiavon, Arturo Pizzoferrato, S. Stea, Elisabetta Cenni, Donatella Granchi, and Gabriela Ciapetti

Subjects

Pathology, medicine.medical_specialty, Materials science, medicine.diagnostic_test, Lymphocyte, technology, industry, and agriculture, Biomedical Engineering, Biophysics, Bioengineering, In vitro, Flow cytometry, Biomaterials, chemistry.chemical_compound, Silicone, medicine.anatomical_structure, Antigen, chemistry, In vivo, medicine, Breast reconstruction, Whole blood

Abstract

Currently, the use of silicone-filled devices, mainly in plastic surgery for breast reconstruction or augmentation, is being debated by the scientific community in connection with the risk to the patient. In this study the response of whole blood or isolated peripheral blood lymphocytes from patients with silicone-gel-filled breast implants was assessed in vitro, in order to verify the hypothesis of silicone material acting in vivo as a sensitizing agent. Both quantitative and qualitative changes of lymphocyte subpopulations of patients carrying silicone devices were assessed and compared with healthy subjects. Upon 24–72 h in vitro re-exposure of patients' lymphocytes to silicone extract, lymphocyte surface antigen expression was monitored by flow cytometry, and the functional response of lymphocytes was measured by radioactive tracer uptake and biochemical changes.

Published

1994

82. Gene expression patterns related to osteogenic differentiation of bone marrow-derived mesenchymal stem cells during ex vivo expansion

Author

Gorka Ochoa, Valentina Devescovi, Donatella Granchi, Nicola Baldini, Elisa Leonardi, Serena Rubina Baglìo, Gabriela Ciapetti, Lourdes Osaba, Granchi D, Ochoa G, Leonardi E, Devescovi V, Baglio SR, Osaba L, Baldini N, Ciapetti G, Pathology, Amsterdam Neuroscience - Cellular & Molecular Mechanisms, and AII - Cancer immunology

Subjects

Pathology, medicine.medical_specialty, Reverse Transcriptase Polymerase Chain Reaction, Cellular differentiation, Gene Expression Profiling, Mesenchymal stem cell, Biomedical Engineering, Wnt signaling pathway, Medicine (miscellaneous), Bioengineering, Cell Differentiation, Mesenchymal Stem Cells, Biology, Hematopoietic Stem Cells, Bone and Bones, Cell biology, Gene expression profiling, medicine.anatomical_structure, Bone cell, medicine, Humans, Bone marrow, Bone regeneration, Stem cell transplantation for articular cartilage repair

Abstract

Bone marrow is commonly used as a source of adult multipotent mesenchymal stem cells (MSCs), defined for their ability to differentiate in vitro into multiple lineages. The ex vivo-expanded MSCs are currently being evaluated as a strategy for the restoration of function in damaged skeletal tissue, both in cell therapy and tissue engineering applications. The aim of this study was to define gene expression patterns underlying the differentiation of MSCs into mature osteoblasts during the expansion in vitro, and to explore a variety of cell functions that cannot be easily evaluated using morphological, cytochemical, and biochemical assays. Cell cultures were obtained from bone marrow samples of six individuals undergoing total hip replacement, and a large-scale transcriptome analysis, using Affymetrix HG-U133A Plus 2.0 array (Affymetrix((R)), Santa Clara, CA), was performed at the occurrence of specific events, including the appearance of MSC surface markers, formation of colonies, and deposition of mineral nodules. We focused our attention on 213 differentially upregulated genes, some belonging to well-known pathways and some having one or more Gene Ontology annotations related to bone cell biology, including angiogenesis, bone-related genes, cell communication, development and morphogenesis, transforming growth factor-beta signaling, and Wnt signaling. Twenty-nine genes, whose role in bone cell pathophysiology has not been described yet, were found. In conclusion, gene expression patterns that characterize the early, intermediate, and late phases of the osteogenic differentiation process of ex vivo-expanded MSCs were defined. These signatures represent a useful tool to monitor the osteogenic process, and to analyze a broad spectrum of functions of MSCs cultured on scaffolds, especially when the constructs are conceived for releasing growth factors or other signals to promote bone regeneration.

Published

2009

83. Osteopoikilosis

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

84. Overproduction of Eosinophils

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

85. Oral Crohn’s Disease

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

86. Overriding Aorta

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

87. Over-Breathing

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

88. Otitis Media, Acute

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

89. Opioid Dependence

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

90. Orthodeoxia-Platypnea Syndrome

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

91. Ornithine Transcarbamylase

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

92. Outer Membrane Carnitine Palmitoyl Transferase

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

93. Orthostatic Hypotensive Disorder, Familial, Streeten Type

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

94. Ocular Coloboma-Imperforate Anus Syndrome

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

95. Ophthalmoplegia, Chronic Progressive External and Kearns Sayre Syndrome

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

96. OCTN2 Transporter Deficiency

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

97. Ogilvie's Syndrome

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

98. Outlet Obstruction

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

99. Osteoarthritis: Developmental Dysplasia of the Hip

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009

100. Osteogenesis Imperfecta

Author

Marc Slawik, Felix Beuschlein, Katrina Light, Roger Mulder, Gordon Dent, Mark G. Buckley, Stephen T. Holgate, Rosalia Misseri, Kirstan K. Meldrum, Massimiliano Mirabella, Gabriella Silvestri, Thomas Frieling, Alexander K. C. Leung, Andrew L. Wong, Marcus Schmitt, Jürgen Kohlhase, Sevan Hopyan, William Lane M. Robson, Maria Judit Molnar, Andrew J. Saxon, Simone Schimpf, Stefan R. Bornstein, Regina Ensenauer, Arno Fuchshuber, Carlo Nunes, Michael Escudier, Jo Spencer, Miranda Lomer, Stephen Challacombe, Jeremy Sanderson, Manish Suneja, Christie P. Thomas, Donatella Granchi, Nicola Baldini, George E. Ehrlich, Matthew B. Dobbs, Yasuaki Nakagawa, James Hyland, Roland Staud, Rajiv Kumar, Mary H. Hohenhaus, Nananda F. Col, Miep Helfrich, Anna Villa, Jan Hellemans, Geert Mortier, Minrong Ai, Matthew L. Warman, Markus Pfister, Hans-Peter Zenner, and Stefan K. Plontke

Published

2009