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Control of intracellular serine protease expression in Bacillus subtilis.

机译:控制枯草芽孢杆菌中细胞内丝氨酸蛋白酶的表达。

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Expression of the major intracellular serine protease (ISP-1) gene of Bacillus subtilis was studied by using a translational fusion plasmid in which the isp promoter region was fused to the lacZ gene. beta-Galactosidase activity, used to measure transcription from the isp promoter, was produced immediately after the end of exponential growth, whereas intracellular protease activity was not detected until 4 h later. These results are consistent with a previous suggestion that ISP-1 initially accumulates in the cell in an enzymatically inactive form. ISP-1 activity was detected in all of the sporulation-deficient strains examined, and the amount of protease activity always corresponded to the amount of beta-galactosidase activity. These results indicate that the activation of ISP-1 is not dependent on a sporulation-specific gene product. Expression of ISP-1 is regulated by a number of mutations known to affect the expression of extracellular enzymes. In sacU(h) and sacQ(h) mutants, the expression of ISP-1 was 10-fold higher than in the wild-type strain. In catA, hpr, and scoC strains, expression of ISP was stimulated two- to threefold, whereas in sacU mutants the expression of ISP-1 was reduced to less than 10% of the wild-type level. The temporal expression and activation of ISP-1 was not affected by any of these mutations. This is the first evidence that the expression of a native intracellular protein is affected by these hyperproduction mutations.
机译:枯草芽孢杆菌的主要细胞内丝氨酸蛋白酶(ISP-1)基因的表达通过使用翻译融合质粒进行研究,在该质粒中,isp启动子区域与lacZ基因融合。用来衡量从isp启动子转录的β-半乳糖苷酶活性是在指数增长结束后立即产生的,而直到4小时后才检测到细胞内蛋白酶活性。这些结果与以前的建议一致,即ISP-1最初以酶无活性的形式积累在细胞中。在所有检查的孢子形成缺陷菌株中均检测到ISP-1活性,并且蛋白酶活性的量始终与β-半乳糖苷酶活性的量相对应。这些结果表明,ISP-1的激活不依赖于孢子形成特异性基因产物。 ISP-1的表达受许多影响细胞外酶表达的突变调控。在sacU(h)和sacQ(h)突变体中,ISP-1的表达比野生型菌株高10倍。在catA,hpr和scoC菌株中,ISP的表达被刺激了2到3倍,而在sacU突变体中,ISP-1的表达被降低到野生型水平的不到10%。 ISP-1的时间表达和激活不受这些突变的影响。这是第一个证据表明天然细胞内蛋白的表达受这些高产突变的影响。

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