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本文引用的文献

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Protein translocation across the ER membrane.蛋白质跨内质网膜易位。
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Yet1p and Yet3p, the yeast homologs of BAP29 and BAP31, interact with the endoplasmic reticulum translocation apparatus and are required for inositol prototrophy.Yet1p和Yet3p是BAP29和BAP31的酵母同源物,它们与内质网转运装置相互作用,是肌醇原养型所必需的。
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A conserved docking surface on calcineurin mediates interaction with substrates and immunosuppressants.钙调神经磷酸酶上保守的对接表面介导其与底物及免疫抑制剂的相互作用。
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Nonapoptotic death of Saccharomyces cerevisiae cells that is stimulated by Hsp90 and inhibited by calcineurin and Cmk2 in response to endoplasmic reticulum stresses.酿酒酵母细胞的非凋亡性死亡,这种死亡由热休克蛋白90(Hsp90)刺激,并在应对内质网应激时受到钙调神经磷酸酶和Cmk2的抑制。
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Voa1p functions in V-ATPase assembly in the yeast endoplasmic reticulum.Voa1p在酵母内质网的V-ATP酶组装过程中发挥作用。
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Hph1和Hph2是Sec63/Sec62翻译后易位复合体的新组分,有助于液泡质子ATP酶的生物合成。

Hph1 and Hph2 are novel components of the Sec63/Sec62 posttranslational translocation complex that aid in vacuolar proton ATPase biogenesis.

作者信息

Piña Francisco J, O'Donnell Allyson F, Pagant Silvere, Piao Hai Lan, Miller John P, Fields Stanley, Miller Elizabeth A, Cyert Martha S

机构信息

Department of Biology, 371 Serra Drive, Stanford University, Stanford, CA 94305-5020, USA.

出版信息

Eukaryot Cell. 2011 Jan;10(1):63-71. doi: 10.1128/EC.00241-10. Epub 2010 Nov 19.

DOI:10.1128/EC.00241-10
PMID:21097665
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3019806/
Abstract

Hph1 and Hph2 are homologous integral endoplasmic reticulum (ER) membrane proteins required for Saccharomyces cerevisiae survival under environmental stress conditions. To investigate the molecular functions of Hph1 and Hph2, we carried out a split-ubiquitin-membrane-based yeast two-hybrid screen and identified their interactions with Sec71, a subunit of the Sec63/Sec62 complex, which mediates posttranslational translocation of proteins into the ER. Hph1 and Hph2 likely function in posttranslational translocation, as they interact with other Sec63/Sec62 complex subunits, i.e., Sec72, Sec62, and Sec63. hph1Δ hph2Δ cells display reduced vacuole acidification; increased instability of Vph1, a subunit of vacuolar proton ATPase (V-ATPase); and growth defects similar to those of mutants lacking V-ATPase activity. sec71Δ cells exhibit similar phenotypes, indicating that Hph1/Hph2 and the Sec63/Sec62 complex function during V-ATPase biogenesis. Hph1/Hph2 and the Sec63/Sec62 complex may act together in this process, as vacuolar acidification and Vph1 stability are compromised to the same extent in hph1Δ hph2Δ and hph1Δ hph2Δ sec71Δ cells. In contrast, loss of Pkr1, an ER protein that promotes posttranslocation assembly of Vph1 with V-ATPase subunits, further exacerbates hph1Δ hph2Δ phenotypes, suggesting that Hph1 and Hph2 function independently of Pkr1-mediated V-ATPase assembly. We propose that Hph1 and Hph2 aid Sec63/Sec62-mediated translocation of specific proteins, including factors that promote efficient biogenesis of V-ATPase, to support yeast cell survival during environmental stress.

摘要

Hph1和Hph2是同源的内质网(ER)整合膜蛋白,在环境应激条件下对酿酒酵母的生存至关重要。为了研究Hph1和Hph2的分子功能,我们进行了基于分裂泛素膜的酵母双杂交筛选,并确定了它们与Sec71的相互作用,Sec71是Sec63/Sec62复合物的一个亚基,介导蛋白质的翻译后转运到内质网中。Hph1和Hph2可能在翻译后转运中发挥作用,因为它们与其他Sec63/Sec62复合物亚基,即Sec72、Sec62和Sec63相互作用。hph1Δ hph2Δ细胞显示液泡酸化降低;液泡质子ATP酶(V-ATPase)亚基Vph1的稳定性增加;以及与缺乏V-ATPase活性的突变体相似的生长缺陷。sec71Δ细胞表现出类似的表型,表明Hph1/Hph2和Sec63/Sec62复合物在V-ATPase生物合成过程中发挥作用。Hph1/Hph2和Sec63/Sec62复合物可能在这个过程中共同发挥作用,因为在hph1Δ hph2Δ和hph1Δ hph2Δ sec71Δ细胞中,液泡酸化和Vph1稳定性受到的损害程度相同。相比之下,促进Vph1与V-ATPase亚基进行转运后组装的内质网蛋白Pkr1的缺失,进一步加剧了hph1Δ hph2Δ的表型,表明Hph1和Hph2的功能独立于Pkr-1介导的V-ATPase组装。我们提出,Hph1和Hph2有助于Sec63/Sec62介导的特定蛋白质的转运,包括促进V-ATPase高效生物合成的因子,以支持酵母细胞在环境应激期间的生存。