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一种简化的 qPCR 方法揭示了基因型 3 型肝炎病毒感染时 tRNAome 的重塑。

A simplified qPCR method revealing tRNAome remodeling upon infection by genotype 3 hepatitis E virus.

机构信息

Institute of Preventive Veterinary Medicine, Sichuan Agricultural University, Chengdu, China.

Department of Gastroenterology and Hepatology, Erasmus MC - University Medical Center Rotterdam, The Netherlands.

出版信息

FEBS Lett. 2020 Jun;594(12):2005-2015. doi: 10.1002/1873-3468.13764. Epub 2020 Mar 21.

Abstract

The landscape of tRNA-viral codons regulates viral adaption at the translational level, presumably through adapting to host codon usage or modulating the host tRNAome. We found that the major zoonotic genotype of hepatitis E virus (HEV) has not adapted to host codon usage, prompting exploration of the effects of HEV infection on the host tRNAome. However, tRNAome quantification is largely impeded by the extremely short sequences of tRNAs and redundancy of tRNA genes. Here, we present a length-extension and stepwise simplified qPCR method that utilizes a universal DNA/RNA hybrid tRNA adaptor and degenerate primers. Using this novel methodology, we observe that HEV infection dramatically reprograms the hepatic tRNAome, which is likely to facilitate translation of viral RNAs. This tRNAome quantification method bears broad implications for future tRNA research and possibly tRNA-based diagnostics.

摘要

tRNA-病毒密码子景观在翻译水平上调节病毒适应,可能通过适应宿主密码子使用或调节宿主 tRNA 组。我们发现,主要的人畜共患基因型戊型肝炎病毒(HEV)尚未适应宿主密码子使用,促使我们探索 HEV 感染对宿主 tRNA 组的影响。然而,tRNA 组的定量受到 tRNA 序列极短和 tRNA 基因冗余的极大阻碍。在这里,我们提出了一种长度扩展和逐步简化的 qPCR 方法,该方法利用通用的 DNA/RNA 杂交 tRNA 接头和简并引物。使用这种新方法,我们观察到 HEV 感染极大地重编程了肝脏的 tRNA 组,这可能有助于病毒 RNA 的翻译。这种 tRNA 组定量方法对未来的 tRNA 研究和可能基于 tRNA 的诊断具有广泛的意义。

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