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基于对与SecY相互作用蛋白Syd的抗性,对大肠杆菌SecY必需细胞质结构域进行的遗传分析。

Genetic analysis of an essential cytoplasmic domain of Escherichia coli SecY based on resistance to Syd, a SecY-interacting protein.

作者信息

Matsuo E, Ito K

机构信息

Department of Cell Biology, Institute for Virus Research, Kyoto University, Japan.

出版信息

Mol Gen Genet. 1998 May;258(3):240-9. doi: 10.1007/s004380050728.

DOI:10.1007/s004380050728
PMID:9645430
Abstract

We previously described a dominant negative secY-d1 allele in Escherichia coli, whose product interferes with protein export, presumably by sequestering SecE, the stabilizing partner of SecY. Syd is the product of a multicopy suppressor of the secY-d1 phenotype, and its overproduction preferentially stabilizes the wild-type SecY protein. In contrast, overproduction of Syd is toxic to the secY24 mutant, which shows a partial defect in SecY-SecE interaction. We isolated Syd-resistant revertants from the secY24 mutant. Pseudo-reversions mapped to sites at or near the secY24 mutation site (Gly240-->Asp). The secY249 mutation (Ala249-->Val) intragenically suppressed Syd sensitivity, but not the temperature-sensitive Sec phenotype of the secY24 mutation. The SecY249 mutant protein shows a reduced capacity to be stabilized by Syd, suggesting that the mutation weakens the SecY-Syd interaction. The other two mutations changed residue 240 (the site of the secY24 alteration) to Asn (secY245) or Ala (secY241) and restored the ability of the cell to export protein. Although the secY245 mutant retained some sensitivity to Syd overproduction, the secY241 mutant was completely Syd-resistant. Furthermore, the secY241 mutation seemed to represent a "hyper reversion" with respect to the SecY-SecE interaction. Protein export in this mutant was no longer sensitive to SecY-d1. When the secY-d1 mutation was combined intragenically with secY241, the resulting double mutant gene (secY-d1-241) showed an increased ability to interfere with protein export. On the basis of our model for SecY-d1, these results suggest that the secY241 alteration enhances SecY-SecE interaction. These results indicate that residue 240 of SecY is crucial for the interaction between the cytosolic domains of SecY and SecE required for the establishment of the translocase complex.

摘要

我们之前描述过大肠杆菌中一种显性负性secY-d1等位基因,其产物可能通过隔离SecY的稳定伴侣SecE来干扰蛋白质输出。Syd是secY-d1表型多拷贝抑制子的产物,其过量表达优先稳定野生型SecY蛋白。相比之下,Syd的过量表达对secY24突变体有毒性,该突变体在SecY-SecE相互作用中存在部分缺陷。我们从secY24突变体中分离出了对Syd有抗性的回复突变体。假回复突变定位在secY24突变位点(甘氨酸240→天冬氨酸)或其附近的位点。secY249突变(丙氨酸249→缬氨酸)在基因内抑制了Syd敏感性,但未抑制secY24突变的温度敏感型Sec表型。SecY249突变体蛋白被Syd稳定的能力降低,这表明该突变削弱了SecY-Syd相互作用。另外两个突变将第240位残基(secY24改变的位点)分别变为天冬酰胺(secY245)或丙氨酸(secY241),并恢复了细胞输出蛋白质的能力。尽管secY245突变体对Syd过量表达仍保留一些敏感性,但secY241突变体对Syd完全有抗性。此外,就SecY-SecE相互作用而言,secY241突变似乎代表一种“超回复”。该突变体中的蛋白质输出不再对SecY-d1敏感。当secY-d1突变与secY241在基因内结合时,产生的双突变基因(secY-d1-241)干扰蛋白质输出的能力增强。基于我们的SecY-d1模型,这些结果表明secY241改变增强了SecY-SecE相互作用。这些结果表明,SecY的第240位残基对于建立转位酶复合物所需的SecY和SecE胞质结构域之间的相互作用至关重要。

相似文献

1
Genetic analysis of an essential cytoplasmic domain of Escherichia coli SecY based on resistance to Syd, a SecY-interacting protein.基于对与SecY相互作用蛋白Syd的抗性,对大肠杆菌SecY必需细胞质结构域进行的遗传分析。
Mol Gen Genet. 1998 May;258(3):240-9. doi: 10.1007/s004380050728.
2
Product of a new gene, syd, functionally interacts with SecY when overproduced in Escherichia coli.新基因syd的产物在大肠杆菌中过量表达时与SecY发生功能相互作用。
J Biol Chem. 1995 Mar 10;270(10):5519-26. doi: 10.1074/jbc.270.10.5519.
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Syd, a SecY-interacting protein, excludes SecA from the SecYE complex with an altered SecY24 subunit.Syd是一种与SecY相互作用的蛋白质,它通过改变SecY24亚基,将SecA排除在SecYE复合物之外。
J Biol Chem. 1998 Jul 24;273(30):18835-40. doi: 10.1074/jbc.273.30.18835.
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A cytoplasmic domain is important for the formation of a SecY-SecE translocator complex.细胞质结构域对于SecY - SecE转运体复合物的形成很重要。
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Characterization of a mutant form of SecA that alleviates a SecY defect at low temperature and shows a synthetic defect with SecY alteration at high temperature.一种SecA突变形式的特性,该突变形式在低温下可缓解SecY缺陷,并在高温下与SecY改变表现出合成缺陷。
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Subunit interactions in the Escherichia coli protein translocase: SecE and SecG associate independently with SecY.大肠杆菌蛋白质转运酶中的亚基相互作用:SecE和SecG分别与SecY独立结合。
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FtsH is required for proteolytic elimination of uncomplexed forms of SecY, an essential protein translocase subunit.FtsH是蛋白水解清除未复合形式的SecY(一种必需的蛋白质转运酶亚基)所必需的。
Proc Natl Acad Sci U S A. 1995 May 9;92(10):4532-6. doi: 10.1073/pnas.92.10.4532.
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SecY variants that interfere with Escherichia coli protein export in the presence of normal secY.在正常SecY存在的情况下干扰大肠杆菌蛋白质输出的SecY变体。
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9
Preferential interaction of Sec-G with Sec-E stabilizes an unstable Sec-E derivative in the Escherichia coli cytoplasmic membrane.Sec-G与Sec-E的优先相互作用稳定了大肠杆菌细胞质膜中一种不稳定的Sec-E衍生物。
Biochem Biophys Res Commun. 1995 Dec 5;217(1):217-23. doi: 10.1006/bbrc.1995.2766.
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The Cs sec mutants of Escherichia coli reflect the cold sensitivity of protein export itself.大肠杆菌的Cs sec突变体反映了蛋白质输出本身的冷敏感性。
Genetics. 1993 Apr;133(4):763-73. doi: 10.1093/genetics/133.4.763.

引用本文的文献

1
Structure, binding, and activity of Syd, a SecY-interacting protein.Syd(一种与SecY相互作用的蛋白质)的结构、结合及活性
J Biol Chem. 2009 Mar 20;284(12):7897-902. doi: 10.1074/jbc.M808305200. Epub 2009 Jan 12.
2
Interfering mutations provide in vivo evidence that Escherichia coli SecE functions in multimeric states.干扰性突变提供了体内证据,表明大肠杆菌SecE以多聚体状态发挥功能。
Mol Genet Genomics. 2003 Mar;268(6):808-15. doi: 10.1007/s00438-003-0803-9. Epub 2003 Feb 11.
3
A SecE mutation that modulates SecY-SecE translocase assembly, identified as a specific suppressor of SecY defects.
一种调节SecY-SecE转位酶组装的SecE突变,被鉴定为SecY缺陷的特异性抑制因子。
J Bacteriol. 2003 Feb;185(3):948-56. doi: 10.1128/JB.185.3.948-956.2003.
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Roles of the C-terminal end of SecY in protein translocation and viability of Escherichia coli.SecY蛋白C末端在大肠杆菌蛋白质转运及生存能力中的作用
J Bacteriol. 2002 Apr;184(8):2243-50. doi: 10.1128/JB.184.8.2243-2250.2002.
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An essential amino acid residue in the protein translocation channel revealed by targeted random mutagenesis of SecY.通过SecY的靶向随机诱变揭示的蛋白质转运通道中的一个必需氨基酸残基。
Proc Natl Acad Sci U S A. 2001 Apr 24;98(9):5128-33. doi: 10.1073/pnas.081617398. Epub 2001 Apr 17.