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体外感染倍数和 RNA 耗竭方法在感染上皮细胞中的 Chlamydia 的 Dual RNA-seq 分析。

Dual RNA-seq analysis of in vitro infection multiplicity and RNA depletion methods in Chlamydia-infected epithelial cells.

机构信息

The iThree Institute, Faculty of Science, University of Technology Sydney, Sydney, Australia.

Helmholtz Centre for Infection Research (HZI), Helmholtz Institute for RNA-based Infection Research (HIRI), Würzburg, Germany.

出版信息

Sci Rep. 2021 May 17;11(1):10399. doi: 10.1038/s41598-021-89921-x.

Abstract

Dual RNA-seq experiments examining viral and bacterial pathogens are increasing, but vary considerably in their experimental designs, such as infection rates and RNA depletion methods. Here, we have applied dual RNA-seq to Chlamydia trachomatis infected epithelial cells to examine transcriptomic responses from both organisms. We compared two time points post infection (1 and 24 h), three multiplicity of infection (MOI) ratios (0.1, 1 and 10) and two RNA depletion methods (rRNA and polyA). Capture of bacterial-specific RNA were greatest when combining rRNA and polyA depletion, and when using a higher MOI. However, under these conditions, host RNA capture was negatively impacted. Although it is tempting to use high infection rates, the implications on host cell survival, the potential reduced length of infection cycles and real world applicability should be considered. This data highlights the delicate nature of balancing host-pathogen RNA capture and will assist future transcriptomic-based studies to achieve more specific and relevant infection-related biological insights.

摘要

越来越多的研究采用 Dual RNA-seq 技术同时检测病毒和细菌病原体,但实验设计差异较大,例如感染率和 RNA 耗尽方法。本研究采用 Dual RNA-seq 技术检测沙眼衣原体感染的上皮细胞,以同时分析两种生物的转录组反应。我们比较了感染后 1 小时和 24 小时两个时间点、三种感染复数(MOI)比值(0.1、1 和 10)和两种 RNA 耗尽方法(rRNA 和 polyA)。rRNA 和 polyA 耗尽联合使用以及采用高 MOI 时,细菌特异性 RNA 的捕获效果最佳。然而,在这些条件下,宿主 RNA 的捕获受到负面影响。尽管使用高感染率很有吸引力,但应考虑到对宿主细胞存活的影响、潜在缩短感染周期以及实际应用的影响。本研究数据突出了平衡宿主-病原体 RNA 捕获的微妙性质,将有助于未来基于转录组的研究获得更具体和相关的感染相关生物学见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cd8f/8128910/37a38d0d6903/41598_2021_89921_Fig1_HTML.jpg

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