ITA
ENG

FIBROBLAST GROWTH-FACTOR-2 (FGF-2) DIFFERENTIALLY REGULATES CONNEXIN (CX) 43 EXPRESSION AND FUNCTION IN ASTROGLIAL CELLS FROM DISTINCT BRAIN-REGIONS

Authors

REUSS B DERMIETZEL R UNSICKER K

Citation

B. Reuss et al., FIBROBLAST GROWTH-FACTOR-2 (FGF-2) DIFFERENTIALLY REGULATES CONNEXIN (CX) 43 EXPRESSION AND FUNCTION IN ASTROGLIAL CELLS FROM DISTINCT BRAIN-REGIONS, Glia, 22(1), 1998, pp. 19-30

Citations number

Categorie Soggetti

Neurosciences

Journal title

Glia → ACNP

ISSN journal

08941491

Volume

Issue

Year of publication

1998

Pages

19 - 30

Database

ISI

SICI code

0894-1491(1998)22:1<19:FG(DRC>2.0.ZU;2-O

Abstract

Fibroblast growth factor (FGF)-2 is a peptide growth factor that promo tes the generation, differentiation, and survival of neurons and glial cells. In the CNS, astroglial cells are coupled in a region-specific manner by gap junctions consisting of connexin 43 (cx43). In the prese nt study we have investigated effects of FGF-2 and of other growth fac tors on the expression and function of cx43 in astroglial cells cultur ed from telencephalic cortex, striatum, and mesencephalon of newborn r ats. Confluent cultures were maintained for two days in low serum, and then exposed to FGF-2 (10 ng/ml) for 48 h. FGF-2 caused a reduction o f cx43-protein, -mRNA, and intercellular communication revealed by dye spreading. These changes occurred in cortical and striatal cells, but not in mesencephalic astroglial cells. Effects of FGF-2 were time-and concentration-dependent, with a minimal effective dose of 1 ng/ml FGF -2, and an onset of effects after 6 h of incubation. The reduction of coupling by FGF-2 was transient, since in cortical and striatal cultur es coupling recovered to control levels 48 h after removal of the grow th factor. Like FGF-2, transforming growth factor-beta 3 (TGF-beta 3) decreased coupling of cortical and striatal, but not mesencephalic ast roglial cells. Astroglial cells from all brain regions showed a slight FGF-mediated increase in 5-bromo-2'-desoxy-uridine (BrdU) incorporati on, which was abolished upon co-treatment with TGF-beta 3. However, TG F-beta 3 did not interfere with the repression of cx43-function by FGF -2. Epidermal growth factor (EGF) that has been demonstrated to influe nce coupling in other cell types had no effect on dye spreading but si gnificantly increased BrdU incorporation. Our results reveal a novel f unction of FGF-2 on cultured astroglial cells which may be relevant to the regulation of astroglial cell connectivity in vivo. (C) 1998 Wile y-Liss, Inc.