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毒素介导的核糖体停滞重编程结核分枝杆菌的蛋白质组。

Toxin-mediated ribosome stalling reprograms the Mycobacterium tuberculosis proteome.

机构信息

Department of Biochemistry and Molecular Biology, Rutgers University, Robert Wood Johnson Medical School, Piscataway, NJ, 08854, USA.

Division of Infectious Diseases, Boston Children's Hospital and Harvard Medical School, Boston, MA, 02115, USA.

出版信息

Nat Commun. 2019 Jul 10;10(1):3035. doi: 10.1038/s41467-019-10869-8.

Abstract

Mycobacterium tuberculosis readily adapts to survive a wide range of assaults by modifying its physiology and establishing a latent tuberculosis (TB) infection. Here we report a sophisticated mode of regulation by a tRNA-cleaving toxin that enlists highly selective ribosome stalling to recalibrate the transcriptome and remodel the proteome. This toxin, MazF-mt9, exclusively inactivates one isoacceptor tRNA, tRNA, through cleavage at a single site within its anticodon (UU↓U). Because wobble rules preclude compensation for loss of tRNA by the second M. tuberculosis lysine tRNA, tRNA, ribosome stalling occurs at in-frame cognate AAA Lys codons. Consequently, the transcripts harboring these stalled ribosomes are selectively cleaved by specific RNases, leading to their preferential deletion. This surgically altered transcriptome generates concomitant changes to the proteome, skewing synthesis of newly synthesized proteins away from those rich in AAA Lys codons toward those harboring few or no AAA codons. This toxin-mediated proteome reprogramming may work in tandem with other pathways to facilitate M. tuberculosis stress survival.

摘要

结核分枝杆菌(Mycobacterium tuberculosis)通过改变其生理学并建立潜伏性结核(TB)感染,从而轻松适应多种攻击并存活下来。在这里,我们报告了一种由 tRNA 切割毒素介导的复杂调控模式,该模式通过高度选择性的核糖体停滞来重新校准转录组并重塑蛋白质组。这种毒素 MazF-mt9 通过在其反密码子(UU↓U)内的单一位置切割,专门使一种同工受体 tRNA(tRNA)失活。由于摆动规则排除了第二个结核分枝杆菌赖氨酸 tRNA(tRNA)对 tRNA 损失的补偿,因此核糖体在框内同源 AAA Lys 密码子处停滞。因此,含有这些停滞核糖体的转录本被特定的核糖核酸酶选择性切割,导致它们优先被删除。这种经过手术改变的转录组会导致蛋白质组发生相应变化,使新合成的富含 AAA Lys 密码子的蛋白质的合成偏向于那些富含 AAA 密码子的蛋白质。这种毒素介导的蛋白质组重编程可能与其他途径协同作用,促进结核分枝杆菌的应激生存。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0730/6620280/89bda63f1e11/41467_2019_10869_Fig1_HTML.jpg

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