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通过丙氨酸延伸扫描诱变对大肠杆菌青霉素结合蛋白1b进行拓扑学和功能研究。

Topographical and functional investigation of Escherichia coli penicillin-binding protein 1b by alanine stretch scanning mutagenesis.

作者信息

Lefèvre F, Rémy M H, Masson J M

机构信息

Institut de Pharmacologie et de Biologie Structurale, UPR 9062 du CNRS, Toulouse, France.

出版信息

J Bacteriol. 1997 Aug;179(15):4761-7. doi: 10.1128/jb.179.15.4761-4767.1997.

Abstract

Penicillin-binding proteins (PBPs) are the targets of beta-lactam antibiotics. We have used a systematic five-alanine substitution method (called ASS [alanine stretch scanning] mutagenesis) to investigate the functional or structural role of various stretches of amino acids in the PBP1b of Escherichia coli. To probe the specific activity of each variant, the antibiotic discs assay was used with strain QCB1 (delta ponB) in the presence of cefaloridine, which totally inhibits the complementing action of PBP1a. This in vivo test has been combined with a quick and efficient in vitro test of the penicillin-binding activity of each of these variants with fluorescent penicillin. This approach has enabled us to show an unexpected role of the N-terminal and C-terminal tails of PBP1b. Moreover, we have established the correct position in PBP1b of the SMN motif that, with the SXXK and the KTG motifs, constitutes the signature of the penicilloyl serine transferases family. Finally, we have shown that the transglycosylase and the transpeptidase domains are separated by an inert linker region, where substitutions and insertions can be made without hindering the in vivo and in vitro activity of the protein.

摘要

青霉素结合蛋白(PBPs)是β-内酰胺类抗生素的作用靶点。我们采用了一种系统性的五丙氨酸取代方法(称为ASS[丙氨酸延伸扫描]诱变)来研究大肠杆菌PBP1b中不同氨基酸片段的功能或结构作用。为了探究每个变体的比活性,在头孢洛林存在的情况下,使用抗生素纸片法对QCB1菌株(ponB缺失株)进行检测,头孢洛林可完全抑制PBP1a的互补作用。这种体内试验与对这些变体中的每一个与荧光青霉素结合的青霉素结合活性进行快速有效的体外试验相结合。这种方法使我们能够揭示PBP1b的N端和C端尾巴出人意料的作用。此外,我们确定了SMN基序在PBP1b中的正确位置,该基序与SXXK和KTG基序一起构成了青霉素酰丝氨酸转移酶家族的特征。最后,我们表明转糖基酶结构域和转肽酶结构域由一个惰性连接区隔开,在该区域进行取代和插入不会妨碍该蛋白的体内和体外活性。

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