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Department of Physiology and Institute for Environmental Medicine, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104
We examined phenotype-specific changes in gap
junction protein [connexin (Cx)] expression and function by
cultured rat alveolar type II cells. Type II cells cultured on
extracellular matrix in medium containing keratinocyte growth factor
(KGF) and 2% fetal bovine serum (FBS; KGF/2) retained expression of
surfactant protein C and the 180-kDa lamellar body membrane protein
(lbm180). These markers were lost when cells were cultured in medium
containing 10% FBS (MEM/10). With RT-PCR, cells cultured in MEM/10
showed transient increases in Cx43 and Cx46 mRNA expression, whereas Cx32 and Cx26 decreased and Cx30.3 and Cx37 were unchanged. Transient changes in Cx32, Cx43, and Cx46 protein expression were confirmed by
immunoblot. In contrast, cells cultured in KGF/2 retained expression of
Cx32 and showed increased expression of Cx30.3 and Cx46 mRNAs, compared
with that in day
0 cells. With immunofluorescence
microscopy, Cx32 and Cx43 were at the plasma membrane of cells grown in
KGF/2, whereas Cx46 was exclusively intracellular. Type II cells
cultured in MEM/10 showed ~3- to 4-fold more intercellular transfer
of microinjected lucifer yellow through gap junctions than cells grown
in 2% FBS. Thus type II cells dynamically alter gap junctional communication, and distinct alveolar epithelial cell phenotypes express
different connexins.
connexin; epithelium; intercellular communication; keratinocyte growth factor
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