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. 2010 Sep;46(8):657-63.
doi: 10.1007/s11626-010-9321-3. Epub 2010 Jun 22.

SREBP isoform and SREBP target gene expression during rat primary hepatocyte culture

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SREBP isoform and SREBP target gene expression during rat primary hepatocyte culture

Jiakai Wu et al. In Vitro Cell Dev Biol Anim. 2010 Sep.

Abstract

Expression of mRNA encoding sterol regulatory element binding protein (SREBP) isoforms (SREBP-1a, -1c, -2) and seven SREBP target genes decreased dramatically as a result of isolation and subsequent culture of primary rat hepatocytes. In standard maintenance medium (MM) expression remained low but when cultured in HepatoZYME (HZM), there was a selective increase in mRNA encoding SREBP-2 and a subset of SREBP target genes, a group characterised by promoters containing adjacent sterol regulatory element and nuclear factor Y (NF-Y) binding sequences. Quantification of all three NF-Y transcripts showed that expression of nuclear factor Y alpha subunit and nuclear factor Y beta subunit mRNA increased during culture in HZM (in contrast to the situation with MM) whilst specificity protein 1, liver-x-receptor and hepatocyte nuclear factor-4 alpha mRNA exhibited equivalent decreased expression in both HZM and MM. Our data indicate that HZM exerts a selective preservation of hepatocyte phenotype through actions on NF-Y expression directly or via an effect secondary to actions on SREBP-2 expression. These data add to the molecular dissection of the causes of hepatocyte dedifferentiation during culture and address means to develop approaches to prevent/limit phenotype change.

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