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细胞分裂 amidase AmiC 的晶体结构揭示了 AMIN 结构域的折叠,这是一个新的肽聚糖结合结构域。

The crystal structure of the cell division amidase AmiC reveals the fold of the AMIN domain, a new peptidoglycan binding domain.

机构信息

Centre d'Ingénierie des Protéines, University of Liège, Liège, Belgium.

出版信息

Mol Microbiol. 2013 Oct;90(2):267-77. doi: 10.1111/mmi.12361. Epub 2013 Aug 23.

Abstract

Binary fission is the ultimate step of the prokaryotic cell cycle. In Gram-negative bacteria like Escherichia coli, this step implies the invagination of three biological layers (cytoplasmic membrane, peptidoglycan and outer membrane), biosynthesis of the new poles and eventually, daughter cells separation. The latter requires the coordinated action of the N-acetylmuramyl-L-alanine amidases AmiA/B/C and their LytM activators EnvC and NlpD to cleave the septal peptidoglycan. We present here the 2.5 Å crystal structure of AmiC which includes the first report of an AMIN domain structure, a β-sandwich of two symmetrical four-stranded β-sheets exposing highly conserved motifs on the two outer faces. We show that this N-terminal domain, involved in the localization of AmiC at the division site, is a new peptidoglycan-binding domain. The C-terminal catalytic domain shows an auto-inhibitory alpha helix obstructing the active site. AmiC lacking this helix exhibits by itself an activity comparable to that of the wild type AmiC activated by NlpD. We also demonstrate the interaction between AmiC and NlpD by microscale thermophoresis and confirm the importance of the active site blocking alpha helix in the regulation of the amidase activity.

摘要

二分裂是原核细胞周期的最后一步。在革兰氏阴性菌如大肠杆菌中,这一步意味着三个生物层(细胞质膜、肽聚糖和外膜)的内陷、新极的生物合成,最终是子细胞的分离。后者需要 N-乙酰胞壁酰-L-丙氨酸酰胺酶 AmiA/B/C 及其 LytM 激活剂 EnvC 和 NlpD 的协调作用来切割隔膜肽聚糖。我们在这里展示了 AmiC 的 2.5Å 晶体结构,其中包括 AMIN 结构域结构的首次报告,这是一个由两个对称的四链 β-折叠组成的 β-三明治,在两个外表面暴露高度保守的基序。我们表明,这个参与 AmiC 在分裂部位定位的 N 端结构域是一个新的肽聚糖结合结构域。C 端催化结构域显示出一个自动抑制的α螺旋,阻碍了活性位点。缺少该螺旋的 AmiC 本身就表现出与被 NlpD 激活的野生型 AmiC 相当的活性。我们还通过微尺度热泳法证明了 AmiC 和 NlpD 之间的相互作用,并证实了活性位点阻断α螺旋在调节酰胺酶活性中的重要性。

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