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Publication : Isolating mitotic and meiotic germ cells from male mice by developmental synchronization, staging, and sorting.

First Author  Romer KA Year  2018
Journal  Dev Biol Volume  443
Issue  1 Pages  19-34
PubMed ID  30149006 Mgi Jnum  J:333273
Mgi Id  MGI:6237458 Doi  10.1016/j.ydbio.2018.08.009
Citation  Romer KA, et al. (2018) Isolating mitotic and meiotic germ cells from male mice by developmental synchronization, staging, and sorting. Dev Biol 443(1):19-34
abstractText  Isolating discrete populations of germ cells from the mouse testis is challenging, because the adult testis contains germ cells at every step of spermatogenesis, in addition to somatic cells. We present a novel method for isolating precise, high-purity populations of male germ cells. We first synchronize germ cell development in vivo by manipulating retinoic acid metabolism, and perform histological staging to verify synchronization. We use fluorescence-activated cell sorting to separate the synchronized differentiating germ cells from contaminating somatic cells and undifferentiated spermatogonia. We achieve ~90% purity at each step of development from undifferentiated spermatogonia through late meiotic prophase. Utilizing this "3S" method (synchronize, stage, and sort), we can separate germ cell types that were previously challenging or impossible to distinguish, with sufficient yield for epigenetic and biochemical studies. 3S expands the toolkit of germ cell sorting methods, and should facilitate detailed characterization of molecular and biochemical changes that occur during the mitotic and meiotic phases of spermatogenesis.
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