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1 Department of Neuroscience, Albert Einstein College of Medicine, Bronx, New York 10461; and 2 Department of Anatomy, Hiroshima University School of Medicine, Hiroshima 737-0023, Japan
Primary cultures of
adult mouse hepatocytes are shown here to reexpress differentiated
hepatocyte features following treatment with 2% DMSO and
10
7 M glucagon. To examine the roles of gap junctional
communication during hepatocyte growth and differentiation, we have
compared treated and untreated hepatocytes from connexin
(Cx)32-deficient [Cx32 knockout (KO)] and wild-type mice. In
untreated cultures, DNA replication of Cx32 KO hepatocytes was markedly
higher than of wild types. Although Cx26 mRNA levels remained high at
all time points in wild-type and Cx32 KO hepatocytes, Cx32 mRNA
and protein in wild-type hepatocytes underwent a marked decline, which recovered in 10-day treated cultures. Increased levels of Cx26 protein and junctional conductance were observed in Cx32 KO
hepatocytes at 96 h in culture, a time when cell growth rate was
high. Treatment with DMSO/glucagon highly reinduced Cx26 expression in
Cx32 KO hepatocytes, and such treatment reinduced expression of
both Cx32 and Cx26 expression in wild types. Dye transfer was not
observed following Lucifer yellow injection into DMSO/glucagon-treated Cx32 KO hepatocytes, whereas the spread was extensive in wild types.
Nevertheless, high junctional conductance values were observed in
treated cells from both genotypes. These studies provide a method by
which the differentiated phenotype can be obtained in cultured
mouse hepatocytes and provide in vitro evidence that expression of gap
junctions formed of Cx32 are involved in the regulation of growth
of mouse hepatocytes.
connexin32; connexin26; knockout mice
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