The present study was designed to extensively characterize cell lines derived from porcine blastocysts by several methodical approaches, including morphological observation, cytogenetic analysis, estimation of alkaline phosphatase activity and detection of specific marker expression at the mRNA/protein level. A comparison was made between the properties of cell lines isolated from in vivo- and in vitro-obtained blastocysts. Our results showed that 57.1% of the in vivo-obtained blastocysts attached to the feeder layer and that 33.3% of them started to grow in a monolayer. The percentage of attached in vitro-produced blastocysts was lower (24.6%), and only 6.9% of them started to grow. Outgrowths from the in vitro-produced blastocysts formed mainly trophectoderm or epithelial-like monolayer, whereas the in vivo-obtained blastocysts formed heterogeneous outgrowths that also contained cells with embryonic stem (ES)-like morphology. Detailed analyses showed that the primary outgrowths with ES-like morphology expressed the pluripotency markers OCT-4 and NANOG and revealed intensive alkaline phosphatase staining, while they did not express markers of differentiation. The majority of passaged cells, including those with ES-like morphology, lacked OCT-4 protein and revealed expression of specific differentiation markers (CYTOKERATIN 18, LAMINS A/C, TRANSFERRIN, a-FETOPROTEIN and GATA-4), although they still expressed NANOG and exhibited weak alkaline phosphatase activity. Moreover, these cells spontaneously differentiated into neural, fibroblast or epithelial-like cells, even in the presence of leukaemia inhibitory factor. Our results show that complex analysis of markers of pluripotency as well as differentiation markers is necessary for proper interpretation of data in porcine embryonic stem cell studies.
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Univ CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Univ Antioquia, Grp CENTAURO, Calle 70 52-21, Medellin, ColombiaUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Urrego, R.
Bernal-Ulloa, S. M.
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FLI, Inst Farm Anim Genet, Holtystr 10, D-31535 Neustadt, Germany
Univ Ciencias Aplicadas & Ambientales UDCA, Fac Ciencias Agr, Calle 222 55-37, Bogota, ColombiaUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Bernal-Ulloa, S. M.
Chavarria, N. A.
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Univ CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, ColombiaUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Chavarria, N. A.
Herrera-Puerta, E.
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Univ CES, Grp Biol CES EIA, Calle 10 A 22-04, Medellin, ColombiaUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Herrera-Puerta, E.
Lucas-Hahn, A.
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FLI, Inst Farm Anim Genet, Holtystr 10, D-31535 Neustadt, GermanyUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Lucas-Hahn, A.
Herrmann, D.
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FLI, Inst Farm Anim Genet, Holtystr 10, D-31535 Neustadt, GermanyUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Herrmann, D.
Winkler, S.
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Max Planck Inst Mol Cell Biol & Genet, DNA Sequencing Facil, Pfotenhauerstr 108, D-01307 Dresden, GermanyUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Winkler, S.
Pache, D.
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Max Planck Inst Mol Cell Biol & Genet, DNA Sequencing Facil, Pfotenhauerstr 108, D-01307 Dresden, GermanyUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Pache, D.
Niemann, H.
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FLI, Inst Farm Anim Genet, Holtystr 10, D-31535 Neustadt, GermanyUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia
Niemann, H.
Rodriguez-Osorio, N.
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Univ Antioquia, Grp CENTAURO, Calle 70 52-21, Medellin, ColombiaUniv CES, Fac Med Vet & Zootecnia, Grp INCA CES, Calle 10 A 22-04, Medellin, Colombia