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酵母Skn7p在真核双组分调控途径中发挥作用。

Yeast Skn7p functions in a eukaryotic two-component regulatory pathway.

作者信息

Brown J L, Bussey H, Stewart R C

机构信息

Department of Biology, McGill University, Montreal, Quebec, Canada.

出版信息

EMBO J. 1994 Nov 1;13(21):5186-94. doi: 10.1002/j.1460-2075.1994.tb06849.x.

Abstract

Previous analysis of the amino acid sequence of Skn7p, the product of the yeast SKN7 gene, revealed a potential 'receiver motif' homologous to that found in bacterial response regulators (signal-transducing effector proteins regulated by phosphorylation at a conserved aspartate residue corresponding to position D427 in Skn7p). We determined the effects of D427N and D427E mutations in Skn7p. The D427N substitution resulted in diminished activity in four independent in vivo assays of Skn7p function, while the D427E mutation enhanced Skn7p activity in these assays. Our results are consistent with predictions based on the bacterial two-component paradigm and provide experimental evidence that a receiver motif functions in regulating the activity of Skn7p in a eukaryote. Skn7p suppressed growth defects associated with a pkc1 delta mutation, raising the possibility that PKC1 might play a role in regulating Skn7p. However, epistasis experiments indicate that Skn7p does not appear to function directly downstream of the PKC1-MAP kinase pathway. Rather, Skn7p may function in a two-component signal transduction pathway that acts in parallel with the PKC1 cascade to regulate growth at the cell surface. We present evidence suggesting that Skn7p serves as a transcription factor in such a signaling pathway.

摘要

先前对酵母SKN7基因产物Skn7p氨基酸序列的分析揭示了一个潜在的“受体基序”,它与细菌应答调节因子中发现的基序同源(信号转导效应蛋白通过在对应于Skn7p中D427位置的保守天冬氨酸残基处磷酸化来调节)。我们确定了Skn7p中D427N和D427E突变的影响。D427N替代导致在四个独立的Skn7p功能体内试验中活性降低,而D427E突变在这些试验中增强了Skn7p活性。我们的结果与基于细菌双组分模式的预测一致,并提供了实验证据,证明受体基序在真核生物中调节Skn7p的活性。Skn7p抑制了与pkc1δ突变相关的生长缺陷,这增加了PKC1可能在调节Skn7p中发挥作用的可能性。然而,上位性实验表明,Skn7p似乎不直接在PKC-MAP激酶途径的下游起作用。相反,Skn7p可能在与PKC1级联平行起作用以调节细胞表面生长速率的双组分信号转导途径中发挥作用。我们提供的证据表明,Skn7p在这样的信号通路中作为转录因子发挥作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/818e/395467/d092f5068d7f/emboj00069-0181-a.jpg

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