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青霉素结合蛋白1a和3受损后,表达青霉素结合蛋白1b胞质结构域突变体的大肠杆菌细胞的差异反应。

Differential responses of Escherichia coli cells expressing cytoplasmic domain mutants of penicillin-binding protein 1b after impairment of penicillin-binding proteins 1a and 3.

作者信息

Chalut C, Charpentier X, Remy M H, Masson J M

机构信息

Institut de Pharmacologie et de Biologie Structurale, UMR 5089 du CNRS, Toulouse, France.

出版信息

J Bacteriol. 2001 Jan;183(1):200-6. doi: 10.1128/JB.183.1.200-206.2001.

Abstract

Penicillin-binding protein 1b (PBP1b) is the major high-molecular-weight PBP in Escherichia coli. Although it is coded by a single gene, it is usually found as a mixture of three isoforms which vary with regard to the length of their N-terminal cytoplasmic tail. We show here that although the cytoplasmic tail seems to play no role in the dimerization of PBP1b, as was originally suspected, only the full-length protein is able to protect the cells against lysis when both PBP1a and PBP3 are inhibited by antibiotics. This suggests a specific role for the full-length PBP1b in the multienzyme peptidoglycan-synthesizing complex that cannot be fulfilled by either PBP1a or the shorter PBP1b proteins. Moreover, we have shown by alanine-stretch-scanning mutagenesis that (i) residues R(11) to G(13) are major determinants for correct translocation and folding of PBP1b and that (ii) the specific interactions involving the full-length PBP1b can be ascribed to the first six residues at the N-terminal end of the cytoplasmic domain. These results are discussed in terms of the interactions with other components of the murein-synthesizing complex.

摘要

青霉素结合蛋白1b(PBP1b)是大肠杆菌中主要的高分子量PBP。尽管它由单个基因编码,但通常以三种同工型的混合物形式存在,这三种同工型在其N端细胞质尾巴的长度方面有所不同。我们在此表明,尽管如最初所怀疑的那样,细胞质尾巴似乎在PBP1b的二聚化中不起作用,但当PBP1a和PBP3都被抗生素抑制时,只有全长蛋白能够保护细胞免于裂解。这表明全长PBP1b在多酶肽聚糖合成复合物中具有特定作用,而PBP1a或较短的PBP1b蛋白都无法实现这一作用。此外,我们通过丙氨酸延伸扫描诱变表明:(i)残基R(11)至G(13)是PBP1b正确转运和折叠的主要决定因素,并且(ii)涉及全长PBP1b的特定相互作用可归因于细胞质结构域N端的前六个残基。根据与胞壁质合成复合物其他成分的相互作用对这些结果进行了讨论。

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