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Lrg1p是酵母中高效细胞融合所需的一种Rho1 GTP酶激活蛋白。

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

作者信息

Fitch Pamela G, Gammie Alison E, Lee Debbie J, de Candal Valeria Brizzio, Rose Mark D

机构信息

The Children's Hospital of Philadelphia, Philadelphia, Pennsylvania 19104, USA.

出版信息

Genetics. 2004 Oct;168(2):733-46. doi: 10.1534/genetics.104.028027.

Abstract

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 rvs161Delta. 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 fus2Delta. 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 beta(1-3) glucan in fus2Delta strains. We conclude that Lrg1p is a Rho1p-GAP 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.

摘要

为了鉴定酿酒酵母中其他的细胞融合基因,我们对fus2Δ进行了高拷贝抑制子筛选。三个基因BEM1、LRG1和FUS1的高剂量部分抑制了fus2Δ的细胞融合缺陷。BEM1和FUS1是许多细胞融合缺陷突变的高拷贝抑制子,而LRG1仅抑制fus2Δ和rvs161Δ。Lrg1p包含一个Rho-GAP同源区域。LRG1的完全缺失以及Rho-GAP编码区域的缺失导致细胞融合率和二倍体形成率降低,与fus2Δ相当。此外,lrg1Δ与其他细胞融合突变一起导致更严重的交配缺陷。与参与细胞融合一致,Lrg1p定位于交配突起的顶端。Lrg1p-GAP结构域在体外强烈且特异性地刺激了Rho1p的GTPase活性,Rho1p是β(1-3)-葡聚糖合酶的调节因子。在lrg1Δ菌株中β(1-3)-葡聚糖沉积增加,在fus2Δ菌株中β(1-3)-葡聚糖沉积错位到交配突起的顶端。高拷贝的LRG1抑制了fus2Δ菌株中β(1-3)葡聚糖的错位。我们得出结论,Lrg1p是一种参与细胞融合的Rho1p-GAP,并推测它的作用是局部抑制细胞壁合成,以帮助交配细胞的质膜紧密贴附。

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