Lrg1p is a Rho1 GTPase-activating protein required for efficient cell fusion in yeast

被引:22
|
作者
Fitch, PG
Gammie, AE
Lee, DJ
de Candal, VB
Rose, MD [1 ]
机构
[1] Princeton Univ, Dept Mol Biol, Princeton, NJ 08544 USA
[2] Childrens Hosp Philadelphia, Philadelphia, PA 19104 USA
[3] Harvard Univ, Sch Med, Boston, MA 02115 USA
[4] Lifecodes Corp, Stamford, CT 06902 USA
关键词
D O I
10.1534/genetics.104.028027
中图分类号
Q3 [遗传学];
学科分类号
071007 ; 090102 ;
摘要
To identify additional cell fusion genes in Saccharomyces cerevisiae, we performed a high-copy suppressor screen of fus2Delta. Higher dosage of three genes, BEM1, LRG1, and FUS1, partially suppressed the fus2Delta cell fusion defect. BEM1 and FUS1 were high-copy suppressors of many cell-fusion-defective mutations, whereas LRG1 suppressed only fus2Delta and rus161Delta. Lrg1p contains a Rho-GAP homologous region. Complete deletion of LRG1, as well as deletion of the Rho-GAP coding region, caused decreased rates of cell fusion and diploid formation comparable to that of Jas2Delta. Furthermore, lrg1Delta caused a more severe mating defect in combination with other cell fusion mutations. Consistent with an involvement in cell fusion, Lrg1p localized to the tip of the mating projection. Lrg1p-GAP domain strongly and specifically stimulated the GTPase activity of Rho1p, a regulator of beta(1-3)-glucan synthase in vitro. beta(1-3)-glucan deposition was increased in lrg1Delta strains and mislocalized to the tip of the mating projection in fus2Delta strains. High-copy LRG1 suppressed the mislocalization of P(1-3) glucan in fus2Delta strains. We conclude that Lrg1p is a Rho1pGAP involved in cell fusion and speculate that it acts to locally inhibit cell wall synthesis to aid in the close apposition of the plasma membranes of mating cells.
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页码:733 / 746
页数:14
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