Your search keyword '"Carina Adamzyk"' showing total 6 results

1. Different Culture Media Affect Proliferation, Surface Epitope Expression, and Differentiation of Ovine MSC

Author

Rene Tolba, Tanja Emonds, Wilhelm Jahnen-Dechent, Bernd Lethaus, Carina Adamzyk, Sabine Neuss, and Julia Falkenstein

Subjects

lcsh:Internal medicine, Article Subject, business.industry, Mesenchymal stem cell, Heterologous, Cell Biology, Chondrogenesis, Phenotype, Epitope, Cell biology, Antigen, Adipogenesis, Epidermal growth factor, Immunology, Medicine, lcsh:RC31-1245, business, Molecular Biology, Research Article

Abstract

Orthopedic implants including engineered bone tissue are commonly tested in sheep. To avoid rejection of heterologous or xenogeneic cells, autologous cells are preferably used, that is, ovine mesenchymal stem cells (oMSC). Unlike human MSC, ovine MSC are not well studied regarding isolation, expansion, and characterization. Here we investigated the impact of culture media composition on growth characteristics, differentiation, and surface antigen expression of oMSC. The culture media varied in fetal calf serum (FCS) content and in the addition of supplements and/or additional epidermal growth factor (EGF). We found that FCS strongly influenced oMSC proliferation and that specific combinations of supplemental factors (MCDB-201, ITS-plus, dexamethasone, and L-ascorbic acid) determined the expression of surface epitopes. We compared two published protocols for oMSC differentiation towards the osteogenic, adipogenic, and chondrogenic fate and found (i) considerable donor to donor variations, (ii) protocol-dependent variations, and (iii) variations resulting from the preculture medium composition. Our results indicate that the isolation and culture of oMSC in different growth media are highly variable regarding oMSC phenotype and behaviour. Furthermore, variations from donor to donor critically influence growth rate, surface marker expression, and differentiation.

Published

2013

2. Human Umbilical Cord-Derived Mesenchymal Stem Cells Spontaneously Form 3D Aggregates and Differentiate in an Embryoid Body-Like Manner

Author

Carina Adamzyk, Hoffmann, Fischer J, Rebekka K. Schneider, Sabine Neuss, Ruth Knuechel, Jahnen Dechent W, J. Jaekel, Mareike Hoss, and Norina Labude

Subjects

0301 basic medicine, Mesenchymal stem cell, Clinical uses of mesenchymal stem cells, Hematopoietic stem cell, Embryoid body, Biology, Embryonic stem cell, Molecular biology, Cell biology, 03 medical and health sciences, 030104 developmental biology, medicine.anatomical_structure, Directed differentiation, medicine, Bone marrow, Induced pluripotent stem cell

Abstract

Human adult mesenchymal stem cells hMSC are particularly suitable cells for autologous tissue engineering and cell based therapies They can be isolated from various tissues such as bone marrow adipose tissue dental pulp or umbilical cords Due to their primitive developmental stage umbilical cord derived hMSC are assumed to have a higher proliferation and differentiation capacity than hMSC from adult tissues We isolated hMSC from bone marrow BM and umbilical cords UC and compared the cells regarding their surface epitopes proliferation and differentiation capacity Flow cytometry of specific surface epitopes showed that both BM MSC and UC MSC display the characteristic MSC phenotype Cells from both sources were readily differentiated into adipocytes osteoblasts and chondrocytes according to standard protocols Interestingly only UC MSC spontaneously formed three dimensional aggregates when cultured under post confluent conditions The cells of these aggregates were viable and spontaneously differentiated into several specialized cell types akin to the well known differentiation of embryoid bodies Besides UC MSC expressed the pluripotency associated gene NANOG as well as genes characteristic for the mesodermal and ectodermal fate Thus UC MSC resemble BM MSC but additionally show a spontaneous embryoid body like aggregation and differentiation in vitro These results indicate that UC MSC are less restricted than BM MSC and may thus extend the limits of BM MSC based therapies nbsp

Published

2016

3. Ex vivoexpansion of cord blood-CD34+cells using IGFBP2and Angptl-5 impairs short-term lymphoid repopulationin vivo

Author

Martin Zenke, Carina Adamzyk, Ruth Knüchel, Thomas Hieronymus, Mónica S. Ventura Ferreira, Wolfgang Wagner, Albrecht M. Müller, Sabine Neuss, Norina Labude, Gudrun Walenda, Willi Jahnen-Dechent, and Daniela Piroth

Subjects

medicine.medical_treatment, Biomedical Engineering, CD34, Medicine (miscellaneous), Biology, Biomaterials, Transplantation, Haematopoiesis, Cytokine, In vivo, Cord blood, Immunology, Cancer research, medicine, Stem cell, Ex vivo

Abstract

Cord blood-derived haematopoietic stem cells (CB-HSCs) are an attractive source for transplantation in haematopoietic disorders. However, the yield of CB-HSCs per graft is limited and often insufficient, particularly for the treatment of adult patients. Here we compare the capacity of three cytokine cocktails to expand CB-CD34+ cells. Cells were cultured for 5 or 14 days in media supplemented with: (a) SCF, FL, IL-3 and IL-6 (SFLIL3/6); (b) SCF, TPO, FGF-1 and IL-6 (STFIL6); and (c) SCF, TPO, FGF-1, IGFBP2 and Angptl-5 (STFAI). We observed that STFAI-culture expansion sustained the most vigorous cell proliferation, maintenance of CD34+ phenotype and colony-forming unit counts. In addition, STFAI-cultured cells had a potent ex vivo migration activity. STFAI-expanded cells were able to engraft NSG mice. However, no significant difference in overall engraftment was observed among the expansion cocktails. Assessment of short-term reconstitution using multilineage markers demonstrated that the STFAI cocktail for HSCs expansion greatly improved total cell expansion but may impair short-term lymphoid repopulation. Copyright © 2012 John Wiley & Sons, Ltd.

Published

2012

4. Bone tissue engineering using polyetherketoneketone scaffolds combined with autologous mesenchymal stem cells in a sheep calvarial defect model

Author

Ali Modabber, Carina Adamzyk, Sabine Neuss, Mareike Hoss, Rene Tolba, Felix Gremse, Paul Kachel, Bernd Lethaus, Frank Hölzle, MUMC+: MA Mondzorg Kaak Aangezicht Chirurgie (9), RS: FHML non-thematic output, and RS: GROW - R3 - Innovative Cancer Diagnostics & Therapy

Subjects

0301 basic medicine, Scaffold, Bone Regeneration, Polymers, Cell, Bone healing, Mesenchymal Stem Cell Transplantation, Bone tissue engineering, Biomaterials, 03 medical and health sciences, chemistry.chemical_compound, Benzophenones, Tissue engineering, Osseointegration, Bone reconstruction, medicine, Animals, Humans, Calvarial defect, Sheep, Tissue Engineering, Tissue Scaffolds, business.industry, Mesenchymal stem cell, Skull, Polyetherketoneketone, Anatomy, Disease Models, Animal, 030104 developmental biology, medicine.anatomical_structure, Otorhinolaryngology, chemistry, Models, Animal, Mesenchymal stem cells, Surgery, Oral Surgery, business, Biomedical engineering

Abstract

Polyetherketoneketone (PEKK) a high performance thermoplastic polymer that is FDA-approved for cranio- and maxillo-facial as well as spineal surgery. We studied the viability, growth and osteogenic differentiation of bone marrow-derived human and sheep mesenchymal stem cells (MSC) in combination with a 3D scaffold made of PEKK using different cell-based assays. To investigate if autologous MSC, either undifferentiated or osteogenically pre-differentiated, augmented bone formation after implantation, we implanted cell-seeded 3D PEKK scaffolds into calvarial defects in sheep for 12 weeks. The volume and quality of newly formed bone were investigated using micro-computer tomography (micro-CT) and histological stainings. Our results show that the 3D PEKK scaffolds were cyto- and bio-compatible. They allowed for adherence, growth and osteogenic differentiation of human and ovine MSC. However, bone healing seemed unaffected by whether the scaffolds were seeded with MSC. Considerable amounts of newly formed bone were found in all PEKK treated groups, but a fibrous capsule was formed around the implants regardless of cell seeding with MSC. European Association for Cranio-Maxillo-Facial Surgery.

Published

2015

5. Fluorescent SNAP-tag galectin fusion proteins as novel tools in glycobiology

Author

Gerhard Müller-Newen, Tobias Recker, Christiane E. Kupper, Carina Adamzyk, Sophia Böcker, Lothar Elling, Sabine Neuss, Hulong Liu, Julia van de Kamp, Willi Jahnen-Dechent, Bernd Lethaus, MUMC+: CONC Poli Mondzorg Kaak Aangezicht Chirurgie (9), and RS: GROW - School for Oncology and Reproduction

Subjects

Glycan, Galectins, Asialoglycoproteins, Chromatography, Affinity, Drug Discovery, Galectin-1, galectin-3, fusion protein, fluorescent protein, Humans, Fetuins, Cells, Cultured, Galectin, Pharmacology, chemistry.chemical_classification, SNAP-tag, biology, Glycobiology, Transferrin, Mesenchymal Stem Cells, Fusion protein, Recombinant Proteins, Molecular Imaging, stomatognathic diseases, Luminescent Proteins, chemistry, Biochemistry, Galectin-3, biology.protein, Glycoprotein, Protein Binding

Abstract

Galectins,β -galactoside binding proteins, function in several physiological and pathological processes. The further evaluation of these processes as well as possible applications of galectins in diagnosis and therapy has raised high scientific interest. Therefore, easy and reliable test systems are necessary. Here we present the simple and cost-efficient production of recombinant human galectins as fusion proteins with SNAP-tag and fluorescent proteins. These constructs show binding specificities and oligomerisation properties generally comparable to recombinant galectins. Their direct fluorescence signal was utilised by ELISA-type assay and flow cytometry analysis with human and ovine mesenchymal stem cells (MSC). Flow cytometry demonstrated glycan mediated binding of His 6 -SNAP-YFP-Gal- 3 to both MSC types, which was specifically inhibited by lactose. Moreover, directed immobilisation by SNAP-tag technology onto benzylguanine- activated sepharose was utilised to prepare galectin affinity columns for glycoprotein analysis and purification. The SNAPtag directed coupling yielded up to three-fold higher binding capacities for the glycoprotein standard asialofetuin compared to nondirected coupled galectin suggesting improved functionality following directed coupling.

Published

2013

6. Ex vivo expansion of cord blood-CD34(+) cells using IGFBP2 and Angptl-5 impairs short-term lymphoid repopulation in vivo

Author

Mónica S, Ventura Ferreira, Norina, Labude, Gudrun, Walenda, Carina, Adamzyk, Wolfgang, Wagner, Daniela, Piroth, Albrecht M, Müller, Ruth, Knüchel, Thomas, Hieronymus, Martin, Zenke, Willi, Jahnen-Dechent, and Sabine, Neuss

Subjects

Stem Cell Factor, Cell Polarity, Antigens, CD34, Bone Marrow Cells, Cell Differentiation, Mice, SCID, Fetal Blood, Clone Cells, Colony-Forming Units Assay, Insulin-Like Growth Factor Binding Protein 2, Mice, Thrombopoietin, Cell Movement, Mice, Inbred NOD, Animals, Cytokines, Humans, Leukocyte Common Antigens, Lymphocytes, Angiopoietins, Cells, Cultured, Spleen, Cell Proliferation

Abstract

Cord blood-derived haematopoietic stem cells (CB-HSCs) are an attractive source for transplantation in haematopoietic disorders. However, the yield of CB-HSCs per graft is limited and often insufficient, particularly for the treatment of adult patients. Here we compare the capacity of three cytokine cocktails to expand CB-CD34(+) cells. Cells were cultured for 5 or 14 days in media supplemented with: (a) SCF, FL, IL-3 and IL-6 (SFLIL3/6); (b) SCF, TPO, FGF-1 and IL-6 (STFIL6); and (c) SCF, TPO, FGF-1, IGFBP2 and Angptl-5 (STFAI). We observed that STFAI-culture expansion sustained the most vigorous cell proliferation, maintenance of CD34(+) phenotype and colony-forming unit counts. In addition, STFAI-cultured cells had a potent ex vivo migration activity. STFAI-expanded cells were able to engraft NSG mice. However, no significant difference in overall engraftment was observed among the expansion cocktails. Assessment of short-term reconstitution using multilineage markers demonstrated that the STFAI cocktail for HSCs expansion greatly improved total cell expansion but may impair short-term lymphoid repopulation.

Published

2012