Characterization and Immunomodulation of Canine Amniotic Membrane Stem Cells

Characterization and Immunomodulation of Canine Amniotic Membrane Stem Cells

Amniotic membrane stem cells have a high capacity of proliferation, cell expansion, and plasticity, as well as immunomodulatory properties that contribute to maternal-fetal tolerance. Owing to the lack of research on human amniotic membrane at different gestational stages, the canine model is consid...

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Veröffentlicht in:Stem cells and cloning 2020-01, Vol.13, p.43-55
Hauptverfasser: de Oliveira Pinheiro, Alessandra, Lara, Valéria M, Souza, Aline F, Casals, Juliana B, Bressan, Fabiana F, Fantinato Neto, Paulo, Oliveira, Vanessa C, Martins, Daniele S, Ambrosio, Carlos E
Format: Artikel
Sprache:eng
Schlagworte:
Amniotic membrane
canine stem cells
CD105 antigen
CD34 antigen
CD45 antigen
CD90 antigen
Cell culture
Cell differentiation
Cell lineage
Cell proliferation
Colonies
Cryopreservation
Cytokines
Cytology
fetal annexes
Fetuses
Flow cytometry
Gene expression
Gestation
Immunological tolerance
Immunomodulation
Interleukin 10
Lymphocytes
Membranes
Mesenchyme
Original Research
Plasticity
Pluripotency
Polymerase chain reaction
Pregnancy
Prostaglandin E2
Stem cells
Tumor necrosis factor-TNF
γ-Interferon
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Zusammenfassung:Amniotic membrane stem cells have a high capacity of proliferation, cell expansion, and plasticity, as well as immunomodulatory properties that contribute to maternal-fetal tolerance. Owing to the lack of research on human amniotic membrane at different gestational stages, the canine model is considered ideal because of its genetic and physiological similarities. We aimed to characterize the canine amniotic membrane (CAM) cell lineage in different gestational stages and evaluate the expression of immunomodulatory genes. Twenty CAMs from early (20-30 days) (n=7), mid- (31-45 days) (n=7), and late gestation (46-63 days) (n=6) stages were studied. The cell features were assessed by cell viability tests, growth curve, colony-forming units, in vitro differentiation, cell labeling for different immunophenotypes, and pluripotent potential markers. The cells were subjected to RT-PCR and qPCR analysis to determine the expression of , and genes. CAM cells exhibited a fibroblastoid morphology and adherence to plastic with an average cell viability of 78.5%. The growth curve indicated a growth peak in the second passage and we obtained an average of 138.2 colonies. Osteogenic, chondrogenic, and adipogenic lineages were confirmed by in vitro differentiation assays. Cellular immunophenotyping experiments confirmed the presence of positive mesenchymal markers (CD90 and CD105) and the low or negative expression of hematopoietic markers (CD45 and CD34). Qualitative analysis of the immunomodulatory functions indicated the expression of the , and genes. When stimulated by interferon-gamma, CAM cells exhibited higher IDO levels throughout gestation. The CAMs from different gestational stages presented features consistent with mesenchymal stem cell lineage; better results were observed during the late gestation stage. Therefore, the gestational stage is a key factor that may influence the functionality of therapies when using fetal membrane tissues from different periods of pregnancy.
ISSN:1178-6957
1178-6957
DOI:10.2147/SCCAA.S237686