Literature DB >> 16425235

Establishment of an in vitro culture system for chicken preblastodermal cells.

Hyun Jeong Park1, Tae Sub Park, Tae Min Kim, Jin Nam Kim, Sang Su Shin, Jeong Mook Lim, Jae Yong Han.   

Abstract

To develop an alternative source for chicken pluripotent cells, we examined (1) whether undifferentiated preblastodermal cells could be subcultured in vitro for an extended period and (2) how subculturing affected the physiological properties of preblastodermal cells. The average number of preblastodermal cells was 2,397 in stage V embryos and 36,345 in stage VII embryos; stage X embryos had an average of 53,857 blastodermal cells. The average cell size decreased significantly (70.63-18.83 microm in diameter; P < 0.0001) as the embryo grew; this was closely related to a reduction in the size and number of lipid vesicles in the cell cytoplasm. The culture conditions were optimized for the stage V preblastodermal cells and the control stage X blastodermal cells. On STO feeder cells, the preblastodermal cells achieved stable growth in vitro only in HES medium or a mixed medium of the Knockout DMEM and HES media. However, more than 10 passages of preblastodermal cells at intervals of 3-4 days was possible only by using the Knockout/HES mixed medium and BRL cell-conditioned HES medium for the primary cultures and subcultures, respectively. Colony-forming preblastodermal cells had well-delineated cytoplasm, which was positively stained for stem cell-specific markers by anti-stage-specific embryo antigen-1 antibody, periodic acid-Schiff's solution, and alkaline phosphatase. When preblastodermal cells with or without culturing were transferred into the blastodermal cavity of stage X embryos, only in vitro-cultured preblastodermal cells at stage V (4/5 = 80%) and stage VII (2/8 = 25%) induced somatic chimerism in recipient chickens. In conclusion, undifferentiated preblastodermal cells could be subcultured, and only the colony-forming preblastodermal cells that stained positively for stem cell markers could induce somatic chimerism. Copyright 2006 Wiley-Liss, Inc.

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Year:  2006        PMID: 16425235     DOI: 10.1002/mrd.20441

Source DB:  PubMed          Journal:  Mol Reprod Dev        ISSN: 1040-452X            Impact factor:   2.609


  8 in total

1.  Gamma-irradiation depletes endogenous germ cells and increases donor cell distribution in chimeric chickens.

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2.  Basic fibroblast growth factor activates MEK/ERK cell signaling pathway and stimulates the proliferation of chicken primordial germ cells.

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3.  Cellular analysis of cleavage-stage chick embryos reveals hidden conservation in vertebrate early development.

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6.  The first whole transcriptomic exploration of pre-oviposited early chicken embryos using single and bulked embryonic RNA-sequencing.

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7.  Cleavage events and sperm dynamics in chick intrauterine embryos.

Authors:  Hyung Chul Lee; Hee Jung Choi; Tae Sub Park; Sang In Lee; Young Min Kim; Deivendran Rengaraj; Hiroki Nagai; Guojun Sheng; Jeong Mook Lim; Jae Yong Han
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Review 8.  Current Approaches and Applications in Avian Genome Editing.

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Journal:  Int J Mol Sci       Date:  2020-05-30       Impact factor: 5.923

  8 in total

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