Regulation of mRNA decay in E. coli.

IF 6.2 2区 生物学 Q1 BIOCHEMISTRY & MOLECULAR BIOLOGY Critical Reviews in Biochemistry and Molecular Biology Pub Date : 2022-02-01 Epub Date: 2021-09-21 DOI:10.1080/10409238.2021.1968784
Bijoy K Mohanty, Sidney R Kushner
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Abstract

Detailed studies of the Gram-negative model bacterium, Escherichia coli, have demonstrated that post-transcriptional events exert important and possibly greater control over gene regulation than transcription initiation or effective translation. Thus, over the past 30 years, considerable effort has been invested in understanding the pathways of mRNA turnover in E. coli. Although it is assumed that most of the ribonucleases and accessory proteins involved in mRNA decay have been identified, our understanding of the regulation of mRNA decay is still incomplete. Furthermore, the vast majority of the studies on mRNA decay have been conducted on exponentially growing cells. Thus, the mechanism of mRNA decay as currently outlined may not accurately reflect what happens when cells find themselves under a variety of stress conditions, such as, nutrient starvation, changes in pH and temperature, as well as a host of others. While the cellular machinery for degradation is relatively constant over a wide range of conditions, intracellular levels of specific ribonucleases can vary depending on the growth conditions. Substrate competition will also modulate ribonucleolytic activity. Post-transcriptional modifications of transcripts by polyadenylating enzymes may favor a specific ribonuclease activity. Interactions with small regulatory RNAs and RNA binding proteins add additional complexities to mRNA functionality and stability. Since many of the ribonucleases are found at the inner membrane, the physical location of a transcript may help determine its half-life. Here we discuss the properties and role of the enzymes involved in mRNA decay as well as the multiple factors that may affect mRNA decay under various in vivo conditions.

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大肠杆菌中 mRNA 的衰变调控。
对革兰氏阴性模式菌大肠杆菌(Escherichia coli)的详细研究表明,转录后事件对基因调控的控制非常重要,甚至可能比转录启动或有效翻译的控制更大。因此,在过去 30 年中,人们投入了大量精力来了解大肠杆菌中 mRNA 的转换途径。虽然参与 mRNA 降解的大多数核糖核酸酶和辅助蛋白都已被鉴定,但我们对 mRNA 降解调控的了解仍不全面。此外,绝大多数关于 mRNA 衰变的研究都是在指数增长的细胞中进行的。因此,目前概述的 mRNA 降解机制可能无法准确反映细胞在各种应激条件下发生的情况,如营养饥饿、pH 值和温度的变化以及其他许多情况。虽然细胞降解机制在各种条件下相对稳定,但细胞内特定核糖核酸酶的水平会因生长条件的不同而变化。底物竞争也会调节核糖核酸分解活性。多聚腺苷酸化酶对转录本的转录后修饰可能有利于特定核糖核酸酶的活性。与小调控 RNA 和 RNA 结合蛋白的相互作用也会增加 mRNA 功能和稳定性的复杂性。由于许多核糖核酸酶存在于内膜,转录本的物理位置可能有助于决定其半衰期。在此,我们将讨论参与 mRNA 降解的酶的特性和作用,以及在各种体内条件下可能影响 mRNA 降解的多种因素。
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来源期刊
CiteScore
14.90
自引率
0.00%
发文量
6
期刊介绍: As the discipline of biochemistry and molecular biology have greatly advanced in the last quarter century, significant contributions have been made towards the advancement of general medicine, genetics, immunology, developmental biology, and biophysics. Investigators in a wide range of disciplines increasingly require an appreciation of the significance of current biochemical and molecular biology advances while, members of the biochemical and molecular biology community itself seek concise information on advances in areas remote from their own specialties. Critical Reviews in Biochemistry and Molecular Biology believes that well-written review articles prove an effective device for the integration and meaningful comprehension of vast, often contradictory, literature. Review articles also provide an opportunity for creative scholarship by synthesizing known facts, fruitful hypotheses, and new concepts. Accordingly, Critical Reviews in Biochemistry and Molecular Biology publishes high-quality reviews that organize, evaluate, and present the current status of high-impact, current issues in the area of biochemistry and molecular biology. Topics are selected on the advice of an advisory board of outstanding scientists, who also suggest authors of special competence. The topics chosen are sufficiently broad to interest a wide audience of readers, yet focused enough to be within the competence of a single author. Authors are chosen based on their activity in the field and their proven ability to produce a well-written publication.
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