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枯草芽孢杆菌超氧化物歧化酶基因的分子克隆、核苷酸序列及其产物特性

Molecular cloning and nucleotide sequence of the superoxide dismutase gene and characterization of its product from Bacillus subtilis.

作者信息

Inaoka T, Matsumura Y, Tsuchido T

机构信息

Department of Biotechnology, Faculty of Engineering, Kansai University, Suita, Osaka 564, Japan.

出版信息

J Bacteriol. 1998 Jul;180(14):3697-703. doi: 10.1128/JB.180.14.3697-3703.1998.

Abstract

Bacillus subtilis was found to possess one detectable superoxide dismutase (Sod) in both vegetative cells and spores. The Sod activity in vegetative cells was maximal at stationary phase. Manganese was necessary to sustain Sod activity at stationary phase, but paraquat, a superoxide generator, did not induce the expression of Sod. The specific activity of purified Sod was approximately 2, 600 U/mg of protein, and the enzyme was a homodimer protein with a molecular mass of approximately 25,000 per monomer. The gene encoding Sod, designated sodA, was cloned by the combination of several PCR methods and the Southern hybridization method. DNA sequence analysis revealed the presence of one open reading frame consisting of 606 bp. Several putative promoter sites were located in the upstream region of sodA. The deduced amino acid sequence showed high homology with other bacterial manganese Sods. Conserved regions in bacterial manganese Sod could also be seen. The phenotype of double mutant Escherichia coli sodA sodB, which could not grow in minimal medium without supplemental amino acids, was complemented by the expression of B. subtilis sodA.

摘要

已发现枯草芽孢杆菌在营养细胞和孢子中均具有一种可检测到的超氧化物歧化酶(Sod)。营养细胞中的Sod活性在稳定期达到最大值。锰是维持稳定期Sod活性所必需的,但超氧化物产生剂百草枯并未诱导Sod的表达。纯化后的Sod的比活性约为2600 U/mg蛋白质,该酶是一种同型二聚体蛋白,每个单体的分子量约为25000。通过几种PCR方法和Southern杂交方法相结合,克隆了编码Sod的基因,命名为sodA。DNA序列分析显示存在一个由606 bp组成的开放阅读框。在sodA的上游区域发现了几个推定的启动子位点。推导的氨基酸序列与其他细菌的锰Sod具有高度同源性。在细菌锰Sod中也可以看到保守区域。在没有补充氨基酸的基本培养基中无法生长的双突变大肠杆菌sodA sodB的表型,通过枯草芽孢杆菌sodA的表达得到了互补。

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