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结核分枝杆菌 M13 金属蛋白酶 Zmp1 开放态的结构分析。

Structural analysis of Mycobacterium tuberculosis M13 metalloprotease Zmp1 open states.

机构信息

Ben May Department for Cancer Research, The University of Chicago, Chicago, IL 60637, USA.

Department of Biochemistry and Molecular Biology, The University of Chicago, Chicago, IL 60637, USA.

出版信息

Structure. 2021 Jul 1;29(7):709-720.e3. doi: 10.1016/j.str.2020.12.002. Epub 2020 Dec 29.

Abstract

Zinc metalloprotease 1 (Zmp1), a Mycobacterium tuberculosis 75 kDa secreted enzyme, mediates key stages of tuberculosis disease progression. The biological activity of Zmp1 presumably stems from its ability to degrade bacterium- and/or host-derived peptides. The crystal structures of Zmp1 and related M13 metalloproteases, such as neprilysin and endothelin-converting enzyme-1 were determined only in the closed conformation, which cannot capture substrates or release proteolytic products. Thus, the mechanisms of substrate binding and selectivity remain elusive. Here we report two open-state cryo-EM structures of Zmp1, revealed by our SAXS analysis to be the dominant states in solution. Our structural analyses reveal how ligand binding induces a conformational switch in four linker regions to drive the rigid body motion of the D1 and D2 domains, which form the sizable catalytic chamber. Furthermore, they offer insights into the catalytic cycle and mechanism of substrate recognition of M13 metalloproteases for future therapeutic innovations.

摘要

锌金属蛋白酶 1(Zmp1)是结核分枝杆菌 75kDa 分泌的酶,介导结核病进展的关键阶段。Zmp1 的生物学活性可能源于其降解细菌和/或宿主来源肽的能力。Zmp1 和相关 M13 金属蛋白酶(如 Neprilysin 和内皮素转换酶-1)的晶体结构仅在封闭构象中确定,无法捕获底物或释放蛋白水解产物。因此,底物结合和选择性的机制仍然难以捉摸。在这里,我们报告了 Zmp1 的两个开放态 cryo-EM 结构,通过我们的 SAXS 分析表明它们是溶液中的主要状态。我们的结构分析揭示了配体结合如何诱导四个连接区的构象转换,从而驱动 D1 和 D2 结构域的刚体运动,形成相当大的催化腔。此外,它们为 M13 金属蛋白酶的催化循环和底物识别机制提供了见解,为未来的治疗创新提供了思路。

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