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在大肠杆菌中添加利福平诱导的rRNA损失反映的是提取假象而非体内降解。

rRNA loss induced by rifampicin addition in Escherichia coli reflects extraction artifacts rather than in vivo degradation.

作者信息

Burck Mathilde, Nouaille Sébastien, Carpousis Agamemnon J, Cocaign-Bousquet Muriel, Girbal Laurence

机构信息

TBI, Université de Toulouse, CNRS, INRAE, INSA, Toulouse, 31077, France.

出版信息

Sci Rep. 2025 Aug 22;15(1):30833. doi: 10.1038/s41598-025-14966-1.

DOI:10.1038/s41598-025-14966-1
PMID:40841809
Abstract

When measuring RNA stability in Escherichia coli, RNA synthesis is usually stopped using rifampicin. Although rRNAs are considered stable in vivo, Hamouche et al. Ribosomal RNA degradation induced by the bacterial RNA polymerase inhibitor rifampicin. RNA 27, 946-958 (2021) recently presented experimental evidence that rifampicin treatment leads to a 50% decrease in total RNA levels due to degradation of 23S and 16S rRNA. Since most mRNA decay in E. coli is initiated by RNase E, which also contributes to the degradation of 23S and 16S rRNA, this suggests that mRNA and rRNA may compete for RNase E in vivo, potentially affecting cell physiology. Here, we show that in exponential growing cells, the decrease in 23S and 16S rRNA levels is an artefact of the RNA extraction protocol. We measured rRNA levels after rifampicin addition using four different protocols. Whereas the gentle lysis employed by Hamouche et al. did indeed lead to loss of rRNA, rRNA levels were stable under stronger lysis. We also measured mRNA levels after rifampicin addition with the different protocols. Our results indicate that 23S, 16S and 5S rRNAs are not degraded during the mRNA degradation period in rifampicin-treated cells. In exponential growing cells therefore, rRNAs are stable in vivo and do not compete with other RNAs for degradation by RNase E. Whether rRNA is degraded and competes with RNA for RNase E under other physiological conditions, particularly stress, remains an open question.

摘要

在测量大肠杆菌中的RNA稳定性时,通常使用利福平来停止RNA合成。尽管核糖体RNA(rRNA)在体内被认为是稳定的,但哈穆什等人(《RNA》27卷,946 - 958页,2021年)最近提供的实验证据表明,利福平处理会导致总RNA水平因23S和16S rRNA的降解而降低50%。由于大肠杆菌中大多数mRNA的衰变是由核糖核酸酶E(RNase E)启动的,而RNase E也参与23S和16S rRNA的降解,这表明mRNA和rRNA在体内可能会竞争RNase E,从而可能影响细胞生理功能。在这里,我们表明,在指数生长的细胞中,23S和16S rRNA水平的降低是RNA提取方案造成的假象。我们使用四种不同的方案测量了添加利福平后的rRNA水平。虽然哈穆什等人采用的温和裂解确实导致了rRNA的损失,但在更强的裂解条件下rRNA水平是稳定的。我们还使用不同的方案测量了添加利福平后的mRNA水平。我们的结果表明,在利福平处理的细胞中,23S、16S和5S rRNA在mRNA降解期间不会被降解。因此,在指数生长的细胞中,rRNA在体内是稳定的,不会与其他RNA竞争被RNase E降解。在其他生理条件下,特别是在应激状态下,rRNA是否会被降解并与RNA竞争RNase E,仍然是一个悬而未决的问题。

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