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利用 RT-qPCR 和质谱法测量病毒 RNA 的直接和间接光化学反应。

Direct and Indirect Photochemical Reactions in Viral RNA Measured with RT-qPCR and Mass Spectrometry.

机构信息

Department of Civil and Environmental Engineering, University of Michigan , Ann Arbor, Michigan 48109, United States.

出版信息

Environ Sci Technol. 2016 Dec 20;50(24):13371-13379. doi: 10.1021/acs.est.6b04281. Epub 2016 Dec 1.

DOI:10.1021/acs.est.6b04281
PMID:27993065
Abstract

RNA carries the genetic instructions for many viruses to replicate in their host cells. The photochemical reactions that take place in RNA and affect viral infectivity in natural and engineered environments, however, remain poorly understood. We exposed RNA oligomer segments from the genome of bacteriophage MS2 to UV, simulated sunlight, and singlet oxygen (O) and analyzed the oligomer reaction kinetics with reverse transcription quantitative PCR (RT-qPCR) and quantitative matrix-assisted laser desorption-ionization time-of-flight (MALDI-TOF) mass spectrometry (MS). Following UV exposure, quantitative MALDI-TOF-MS detected significantly more RNA modifications than did RT-qPCR, suggesting that certain chemical modifications in the RNA were not detected by the reverse transcriptase enzyme. In contrast, MALDI-TOF-MS tracked as much O-induced RNA damage as RT-qPCR. After 5 h of simulated sunlight exposure (5100 J/m UVB and 1.2 × 10 J/m UVA), neither MALDI-TOF-MS nor RT-qPCR detected significant decreases in the oligomer concentrations. High-resolution electrospray ionization (ESI)-Orbitrap MS analyses identified pyrimidine photohydrates as the major UV products, which likely contributed to the discrepancy between the MS- and RT-qPCR-based results. Reactions between RNA oligomers and O resulted in an unidentified major product with a mass change of +6 Da. These results shed light on the photochemical reactions that take place in RNA and suggest that the analytical techniques used to detect RNA reactivity could bias the observed reaction kinetics.

摘要

RNA 携带了许多病毒在宿主细胞中复制所需的遗传指令。然而,在自然和工程环境中,影响病毒感染力的 RNA 光化学反应仍知之甚少。我们将噬菌体 MS2 基因组的 RNA 寡聚物片段暴露于 UV、模拟阳光和单线态氧 (O) 下,并通过反转录定量 PCR (RT-qPCR) 和定量基质辅助激光解吸电离飞行时间 (MALDI-TOF) 质谱 (MS) 分析寡聚物反应动力学。在 UV 暴露后,定量 MALDI-TOF-MS 检测到的 RNA 修饰比 RT-qPCR 多得多,这表明逆转录酶并未检测到 RNA 中的某些化学修饰。相比之下,MALDI-TOF-MS 跟踪到的 O 诱导的 RNA 损伤与 RT-qPCR 一样多。在模拟阳光暴露 5 小时后(5100 J/m UVB 和 1.2×10 J/m UVA),无论是 MALDI-TOF-MS 还是 RT-qPCR 都未检测到寡聚物浓度的显著降低。高分辨率电喷雾电离 (ESI)-轨道阱 MS 分析鉴定出嘧啶光水合产物为主要的 UV 产物,这可能是 MS 和 RT-qPCR 结果之间存在差异的原因。RNA 寡聚物与 O 之间的反应产生了一种未知的主要产物,其质量变化为+6 Da。这些结果揭示了 RNA 中发生的光化学反应,并表明用于检测 RNA 反应性的分析技术可能会影响观察到的反应动力学。

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