首页> 外文期刊>The Journal of General and Applied Microbiology >Efficient export of alkaline phosphatase overexpressed from a multicopy plasmid requires degP, a gene encoding a periplasmic protease of Escherichia coli
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Efficient export of alkaline phosphatase overexpressed from a multicopy plasmid requires degP, a gene encoding a periplasmic protease of Escherichia coli

机译:从多拷贝质粒中过表达的碱性磷酸酶的有效输出需要degP,该基因编码大肠杆菌的周质蛋白酶

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摘要

Escherichia coli DegP is an inducible serine protease which is involved in the breakdown of abberant proteins arising in the periplasmic compartment. Overexpression of alkaline phosphatase (PhoA) increased transcription of degP by twofold. To examine the significance of its induction, we overexpressed PhoA in a mutant strain deficient in the degP gene. Upon PhoA overexpression, the degP mutant produced a smaller amount of active PhoA, about one half of the enzymatic activity of its isogenic wild-type strain, and accumulated a larger amount of its precursor, indicating that degP is required for efficient export of overexpressed PhoA. Pulse-chase experiment showed that PhoA overexpression in the absence of degP causes a severe defect in the export of several proteins tested. Examination of the synthesis and the accumulation of the phoA gene products revealed that a part of them, synthesized in the wild-type strain, undergoes relatively rapid proteolysis and that degP is necessary for such a process. From these results, we discuss a possible role of DegP in facilitating protein export under stress conditions.
机译:大肠杆菌DegP是一种可诱导的丝氨酸蛋白酶,参与周质区室中异常蛋白的降解。碱性磷酸酶(PhoA)的过表达使degP的转录增加了两倍。为了检查其诱导的重要性,我们在degP基因缺陷的突变株中过表达了PhoA。在PhoA过表达后,degP突变体产生的活性PhoA量较小,约为同基因野生型菌株酶活性的一半,并且积累了大量的前体,表明degP是有效输出过表达的PhoA所必需的。脉冲追踪实验表明,在没有degP的情况下PhoA过表达会导致几种测试蛋白质输出的严重缺陷。对phoA基因产物的合成和积累的检查表明,其中的一部分(在野生型菌株中合成)经历了相对较快的蛋白水解,而degP对于这种过程是必需的。从这些结果,我们讨论了DegP在促进应激条件下蛋白质输出中的可能作用。

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