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质粒介导的对血清杀菌活性的抗性:一种主要外膜蛋白,即traT基因产物,负责大肠杆菌中质粒特异性的血清抗性。

Plasmid-determined resistance to serum bactericidal activity: a major outer membrane protein, the traT gene product, is responsible for plasmid-specified serum resistance in Escherichia coli.

作者信息

Moll A, Manning P A, Timmis K N

出版信息

Infect Immun. 1980 May;28(2):359-67. doi: 10.1128/iai.28.2.359-367.1980.

Abstract

Resistance to the bactericidal activity of serum appears to be an important virulence property of invasive bacteria. The conjugative multiple-antibiotic-resistance plasmid R6-5 was found to confer upon Escherichia coli host bacteria increased resistance against rabbit serum. Gene-cloning techniques were used to localize the serum resistance determinant of R6-5 to a segment of the plasmid that encodes conjugal transfer functions, and a pACYC184 hybrid plasmid, designated pKT107, that contains this segment was constructed. The generation and analysis of deletion and insertion mutant derivatives of the pKT107 plasmid that no longer specify serum resistance permitted precise localization of the serum-resistance cistron on the R6-5 map and demonstrated that this locus is coincident with that of traT, one of the two surface exclusion genes of R6-5. Examination of the proteins synthesized in E. coli minicells of pKT107 and its serum-sensitive mutant derivative plasmids confirmed that the serum-resistance gene product of R6-5 is the traT protein and showed that this protein is a major structural component (about 21,000 copies per cell) of the bacterial outer membrane.

摘要

对血清杀菌活性的抗性似乎是侵袭性细菌的一种重要毒力特性。发现接合型多重抗生素抗性质粒R6 - 5赋予大肠杆菌宿主细菌对兔血清的抗性增强。利用基因克隆技术将R6 - 5的血清抗性决定簇定位到质粒的一个编码接合转移功能的片段上,并构建了一个包含该片段的pACYC184杂交质粒,命名为pKT107。对不再具有血清抗性的pKT107质粒缺失和插入突变衍生物的产生和分析,使得血清抗性顺反子在R6 - 5图谱上得以精确定位,并证明该位点与R6 - 5的两个表面排斥基因之一traT的位点一致。对pKT107及其血清敏感突变体衍生质粒在大肠杆菌微小细胞中合成的蛋白质的检测证实,R6 - 5的血清抗性基因产物是traT蛋白,并表明该蛋白是细菌外膜的一种主要结构成分(每个细胞约21,000个拷贝)。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2079/550942/09ce1068fbf4/iai00173-0060-a.jpg

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