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微菌素 J25 和卡比斯特林通过套索肽抑制转录的结构机制。

Structural mechanism of transcription inhibition by lasso peptides microcin J25 and capistruin.

机构信息

Laboratory of Molecular Biophysics, The Rockefeller University, New York, NY 10065.

Department of Chemical and Biological Engineering, Princeton University, Princeton, NJ 08544.

出版信息

Proc Natl Acad Sci U S A. 2019 Jan 22;116(4):1273-1278. doi: 10.1073/pnas.1817352116. Epub 2019 Jan 9.

Abstract

We report crystal structures of the antibacterial lasso peptides microcin J25 (MccJ25) and capistruin (Cap) bound to their natural enzymatic target, the bacterial RNA polymerase (RNAP). Both peptides bind within the RNAP secondary channel, through which NTP substrates enter the RNAP active site, and sterically block trigger-loop folding, which is essential for efficient catalysis by the RNAP. MccJ25 binds deep within the secondary channel in a manner expected to interfere with NTP substrate binding, explaining the partial competitive mechanism of inhibition with respect to NTPs found previously [Mukhopadhyay J, Sineva E, Knight J, Levy RM, Ebright RH (2004) 14:739-751]. The Cap binding determinant on RNAP overlaps, but is not identical to, that of MccJ25. Cap binds further from the RNAP active site and does not sterically interfere with NTP binding, and we show that Cap inhibition is partially noncompetitive with respect to NTPs. This work lays the groundwork for structure determination of other lasso peptides that target the bacterial RNAP and provides a structural foundation to guide lasso peptide antimicrobial engineering approaches.

摘要

我们报告了抗菌拉索肽微菌素 J25(MccJ25)和卡皮斯丁(Cap)与天然酶靶标细菌 RNA 聚合酶(RNAP)结合的晶体结构。这两种肽都结合在 RNAP 的二级通道内,NTP 底物通过该通道进入 RNAP 的活性位点,并且空间上阻止了触发环折叠,这对于 RNAP 的高效催化至关重要。MccJ25 以一种预期会干扰 NTP 底物结合的方式深嵌在二级通道中,这解释了先前发现的对 NTP 的部分竞争性抑制机制[Mukhopadhyay J、Sineva E、Knight J、Levy RM、Ebright RH(2004)14:739-751]。Cap 在 RNAP 上的结合决定簇与 MccJ25 的结合决定簇重叠,但并不完全相同。Cap 与 RNAP 的活性位点结合得更远,并且不会在空间上干扰 NTP 的结合,我们表明 Cap 的抑制作用对 NTP 具有部分非竞争性。这项工作为针对细菌 RNA 聚合酶的其他拉索肽的结构测定奠定了基础,并为拉索肽抗菌工程方法提供了结构基础。

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