首页> 外文期刊>Journal of Molecular Biology >NMR Structure of Citrobacter freundii AmpD, Comparison with Bacteriophage T7 Lysozyme and Homology with PGRP Domains.
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NMR Structure of Citrobacter freundii AmpD, Comparison with Bacteriophage T7 Lysozyme and Homology with PGRP Domains.

机译:弗氏柠檬酸杆菌AmpD的NMR结构,与噬菌体T7溶菌酶的比较以及具有PGRP域的同源性。

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摘要

AmpD is a bacterial amidase involved in the recycling of cell-wall fragments in Gram-negative bacteria. Inactivation of AmpD leads to derepression of beta-lactamase expression, presenting a major pathway for the acquisition of constitutive antibiotic resistance. Here, we report the NMR structure of AmpD from Citrobacter freundii (PDB accession code 1J3G). A deep substrate-binding pocket explains the observed specificity for low molecular mass substrates. The fold is related to that of bacteriophage T7 lysozyme. Both proteins bind zinc at a conserved site and require zinc for amidase activity, although the enzymatic mechanism seems to differ in detail. The structure-based sequence alignment identifies conserved features that are also conserved in the eukaryotic peptidoglycan recognition protein (PGRP) domains, including the zinc-coordination site in several of them. PGRP domains thus belong to the same fold family and, where zinc-binding residues are conserved, may have amidase activity. This hypothesisis supported by the observation that human serum N-acetylmuramyl-L-alanine amidase seems to be identical with a soluble form of human PGRP-L.
机译:AmpD是一种细菌酰胺酶,参与革兰氏阴性细菌中细胞壁片段的回收。 AmpD的失活导致β-内酰胺酶表达的抑制,为获得组成型抗生素抗性提供了主要途径。在这里,我们报道了来自弗氏柠檬酸杆菌的AmpD的NMR结构(PDB登录号1J3G)。较深的底物结合袋可解释观察到的对低分子量底物的特异性。该折叠与噬菌体T7溶菌酶的折叠有关。两种蛋白质都在一个保守位点结合锌,并且需要锌才能发挥酰胺酶活性,尽管酶促机制似乎在细节上有所不同。基于结构的序列比对可鉴定在真核肽聚糖识别蛋白(PGRP)域中也保守的保守特征,其中包括多个锌协同位点。 PGRP结构域因此属于相同的折叠家族,并且在其中锌结合残基被保守的地方可以具有酰胺酶活性。这一假设得到了以下观察的支持:人血清N-乙酰村mura基-L-丙氨酸酰胺酶似乎与人PGRP-L的可溶形式相同。

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