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未折叠蛋白反应途径在酿酒酵母分泌应激及INO1表达调控中的作用

Role of the unfolded protein response pathway in secretory stress and regulation of INO1 expression in Saccharomyces cerevisiae.

作者信息

Chang Hak J, Jesch Stephen A, Gaspar Maria L, Henry Susan A

机构信息

Department of Biological Sciences, Carnegie Mellon University, Pittsburgh, Pennsylvania 15213, USA.

出版信息

Genetics. 2004 Dec;168(4):1899-913. doi: 10.1534/genetics.104.032961. Epub 2004 Sep 15.

Abstract

The unfolded protein response pathway (UPR) enables the cell to cope with the buildup of unfolded proteins in the endoplasmic reticulum (ER). UPR loss-of-function mutants, hac1Delta and ire1Delta, are also inositol auxotrophs, a phenotype associated with defects in expression of INO1, the most highly regulated of a set of genes encoding enzymes of phospholipid metabolism. We now demonstrate that the UPR plays a functional role in membrane trafficking under conditions of secretory stress in yeast. Mutations conferring a wide range of membrane trafficking defects exhibited negative genetic interaction when combined with ire1Delta and hac1Delta. At semipermissive temperatures, carboxypeptidase Y transit time to the vacuole was slower in Sec(-) cells containing an ire1Delta or hac1Delta mutation than in Sec(-) cells with an intact UPR. The UPR was induced in Sec(-) cells defective in subcellular membrane trafficking events ranging from ER vesicle trafficking to distal secretion and in erg6Delta cells challenged with brefeldin A. However, the high levels of UPR induction observed under these conditions were not correlated with elevated INO1 expression. Indeed, many of the Sec(-) mutants that had elevated UPR expression at semipermissive growth temperatures failed to achieve wild-type levels of INO1 expression under these same conditions.

摘要

未折叠蛋白反应途径(UPR)使细胞能够应对内质网(ER)中未折叠蛋白的积累。UPR功能丧失突变体hac1Δ和ire1Δ也是肌醇营养缺陷型,这种表型与INO1表达缺陷有关,INO1是一组编码磷脂代谢酶的基因中调控程度最高的。我们现在证明,在酵母分泌应激条件下,UPR在膜运输中发挥功能作用。与ire1Δ和hac1Δ结合时,赋予广泛膜运输缺陷的突变表现出负向遗传相互作用。在半允许温度下,与具有完整UPR的Sec(-)细胞相比,含有ire1Δ或hac1Δ突变的Sec(-)细胞中羧肽酶Y转运到液泡的时间更慢。UPR在亚细胞膜运输事件存在缺陷的Sec(-)细胞中被诱导,这些事件范围从内质网囊泡运输到远端分泌,并且在受到布雷菲德菌素A挑战的erg6Δ细胞中也被诱导。然而,在这些条件下观察到的高水平UPR诱导与INO1表达升高无关。实际上,许多在半允许生长温度下UPR表达升高的Sec(-)突变体在相同条件下未能达到野生型INO1表达水平。

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