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天冬氨酸化学感受器Tar主要通过疏水相互作用与甲基转移酶结合,从而被有效地甲基化。

The aspartate chemoreceptor Tar is effectively methylated by binding to the methyltransferase mainly through hydrophobic interaction.

作者信息

Shiomi D, Okumura H, Homma M, Kawagishi I

机构信息

Division of Biological Science, Graduate School of Science, Nagoya University, Chikusa-ku, Nagoya 464-8602, Japan.

出版信息

Mol Microbiol. 2000 Apr;36(1):132-40. doi: 10.1046/j.1365-2958.2000.01834.x.

DOI:10.1046/j.1365-2958.2000.01834.x
PMID:10760170
Abstract

In the chemotaxis of Escherichia coli, adaptation requires the methylation and demethylation of transmembrane receptors, which are catalysed by the methyltransferase CheR and the methylesterase CheB respectively. CheR binds to major chemoreceptors through their C-terminal motif NWETF, which is distinct from the methylation sites. In this study, we carried out a systematic mutagenesis of the pentapeptide sequence of Tar. Receptor methylation and adaptation were severely impaired by the alanine substitution of residue W550 and, to a lesser extent, by that of F553. Substitution of residues N549, E551 and T552 had only a slight or little effect. The defects of the W550A and F553A mutations were suppressed by high- and low-level overproduction of CheR respectively. Expression of a fusion protein containing the NWETF sequence, but not its W550A and F553A versions, inhibited chemotaxis of the Che+ strain. In an in vitro assay, CheR bound to the wild-type version but not to the mutant versions. These results and further mutagenesis suggest that the hydrophobicity and the size of residues W550 and F553 are critical in the interaction with CheR, a conclusion that is consistent with the crystal structure of a CheR-NWETF complex. On the other hand, the negatively charged side chain of E551 and the polar side chains of N549 and T552 may not be strictly required, although the presence of a salt bridge and hydrogen bonds between these residues and residues from CheR has been noted in the co-crystal.

摘要

在大肠杆菌的趋化作用中,适应性需要跨膜受体的甲基化和去甲基化,分别由甲基转移酶CheR和甲酯酶CheB催化。CheR通过其C端基序NWETF与主要化学感受器结合,该基序与甲基化位点不同。在本研究中,我们对Tar的五肽序列进行了系统诱变。残基W550的丙氨酸取代严重损害了受体甲基化和适应性,F553的取代在较小程度上也有影响。残基N549、E551和T552的取代只有轻微或几乎没有影响。W550A和F553A突变的缺陷分别被CheR的高水平和低水平过量表达所抑制。含有NWETF序列但不含其W550A和F553A变体的融合蛋白的表达抑制了Che+菌株的趋化作用。在体外试验中,CheR与野生型结合,但不与突变型结合。这些结果和进一步的诱变表明,残基W550和F553的疏水性和大小在与CheR的相互作用中至关重要,这一结论与CheR-NWETF复合物的晶体结构一致。另一方面,尽管在共晶体中已注意到E551的带负电荷侧链以及N549和T552的极性侧链与CheR的残基之间存在盐桥和氢键,但可能并非严格必需。

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