βA- and βC-activin, follistatin, activin receptor mRNA and βC-activin peptide expression during rat liver regeneration

E. J. Gold, X. Zhang, A. M. Wheatley, S. L. Mellor, M. Cranfield, G. P. Risbridger, N. P. Groome, Jean S. Fleming

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51 Citations (Scopus)

Abstract

The mRNA expression of two activin growth factor subunits (βA- and βC-activin), activin receptor subunits (ActRIIA, ActRIIB) and the activin-binding protein follistatin, and peptide expression of βA-activin and βC-activin subunits, were examined in regenerating rat liver after partial hepatectomy (PHx). Liver samples were collected from adult, male Sprague-Dawley rats, 12-240 h (n=3-5 rats per time point) after PHx or from sham-operated controls at the same time points. Hepatocyte mitosis and apoptosis were assessed histologically and by in situ cell death detection. RT and PCR were used to assess relative gene expression. βA- and βC-activin peptide immunoreactivity was assessed in liver and serum samples by western blotting, whereas cellular expression was investigated by immunohistochemistry, using specific monoclonal antibodies. βA- and βC-activin mRNA dropped to <50% of sham control values 12 h after PHx and remained at this level until 168 h post-PHx, when βA-activin expression increased to three times sham control values and βC-activin mRNA returned to pre-PHx levels. A peak in follistatin expression was observed 24-48 h post-PHx, coincident with an increase in hepatocyte mitosis. No changes were observed in ActRIIA mRNA, whereas ActRIIB expression paralleled that of βA-activin mRNA. βC-activin immunoreactive homo- and heterodimers were observed in regenerating liver and serum. Mitotic hepatocytes frequently contained βC-activin immunoreactivity, whereas apoptotic hepatocytes were often immunoreactive for βA-activin. We conclude that βA- and βC-activin subunit proteins are autocrine growth regulators in regenerating liver and when expressed independently lead to hepatocyte apoptosis or mitosis in a subset of hepatocytes.

Original languageEnglish
Pages (from-to)505-515
Number of pages11
JournalJournal of Molecular Endocrinology
Volume34
Issue number2
DOIs
Publication statusPublished - Apr 2005
Externally publishedYes

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