Understanding spatiotemporal coupling of gene expression using single molecule RNA imaging technologies.

IF 3.6 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY Transcription-Austin Pub Date : 2023-06-01 Epub Date: 2023-04-12 DOI:10.1080/21541264.2023.2199669
Alan Gerber, Sander van Otterdijk, Frank J Bruggeman, Evelina Tutucci
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Abstract

Across all kingdoms of life, gene regulatory mechanisms underlie cellular adaptation to ever-changing environments. Regulation of gene expression adjusts protein synthesis and, in turn, cellular growth. Messenger RNAs are key molecules in the process of gene expression. Our ability to quantitatively measure mRNA expression in single cells has improved tremendously over the past decades. This revealed an unexpected coordination between the steps that control the life of an mRNA, from transcription to degradation. Here, we provide an overview of the state-of-the-art imaging approaches for measurement and quantitative understanding of gene expression, starting from the early visualizations of single genes by electron microscopy to current fluorescence-based approaches in single cells, including live-cell RNA-imaging approaches to FISH-based spatial transcriptomics across model organisms. We also highlight how these methods have shaped our current understanding of the spatiotemporal coupling between transcriptional and post-transcriptional events in prokaryotes. We conclude by discussing future challenges of this multidisciplinary field.Abbreviations: mRNA: messenger RNA; rRNA: ribosomal rDNA; tRNA: transfer RNA; sRNA: small RNA; FISH: fluorescence in situ hybridization; RNP: ribonucleoprotein; smFISH: single RNA molecule FISH; smiFISH: single molecule inexpensive FISH; HCR-FISH: Hybridization Chain-Reaction-FISH; RCA: Rolling Circle Amplification; seqFISH: Sequential FISH; MERFISH: Multiplexed error robust FISH; UTR: Untranslated region; RBP: RNA binding protein; FP: fluorescent protein; eGFP: enhanced GFP, MCP: MS2 coat protein; PCP: PP7 coat protein; MB: Molecular beacons; sgRNA: single guide RNA.

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利用单分子 RNA 成像技术了解基因表达的时空耦合。
在所有生命领域,基因调控机制都是细胞适应不断变化的环境的基础。基因表达的调控可调整蛋白质的合成,进而影响细胞的生长。信使 RNA 是基因表达过程中的关键分子。过去几十年来,我们定量测量单细胞中 mRNA 表达的能力有了极大提高。这揭示了控制 mRNA 从转录到降解的各个步骤之间意想不到的协调性。在此,我们概述了用于测量和定量了解基因表达的最先进成像方法,从早期的电子显微镜单基因可视化到目前基于荧光的单细胞方法,包括活细胞 RNA 成像方法和基于 FISH 的模式生物空间转录组学。我们还重点介绍了这些方法如何塑造了我们目前对原核生物中转录和转录后事件之间时空耦合的理解。最后,我们将讨论这一多学科领域的未来挑战。缩略语:mRNA:信使 RNA;rRNA:核糖体 rDNA;tRNA:转运 RNA;sRNA:小 RNA;FISH:荧光原位杂交;RNP:核糖核蛋白;smFISH:单 RNA 分子 FISH;smiFISH:单分子廉价 FISH;HCR-FISH:杂交链反应-FISH;RCA:seqFISH:顺序 FISH;MERFISH:多重错误稳健 FISH;UTR:非翻译区;RBP:RNA 结合蛋白;FP:荧光蛋白;eGFP:增强型 GFP;MCP:MS2 衣壳蛋白;PCP:PP7 衣壳蛋白;MB:分子信标;sgRNA:单导向 RNA。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Transcription-Austin
Transcription-Austin BIOCHEMISTRY & MOLECULAR BIOLOGY-
CiteScore
6.50
自引率
5.60%
发文量
9
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