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非结构蛋白 1 G53D 取代降低了一种经临床测试的活型登革热疫苗效力。

A Non-structural 1 Protein G53D Substitution Attenuates a Clinically Tested Live Dengue Vaccine.

机构信息

Programme in Emerging Infectious Diseases, Duke-NUS Medical School, Singapore 169857, Singapore.

Programme in Emerging Infectious Diseases, Duke-NUS Medical School, Singapore 169857, Singapore; Department of Infectious Diseases, Singapore General Hospital, Singapore 169108, Singapore.

出版信息

Cell Rep. 2020 May 12;31(6):107617. doi: 10.1016/j.celrep.2020.107617.

Abstract

The molecular basis of dengue virus (DENV) attenuation remains ambiguous and hampers a targeted approach to derive safe but nonetheless immunogenic live vaccine candidates. Here, we take advantage of DENV serotype 2 PDK53 vaccine strain, which recently and successfully completed a phase-3 clinical trial, to identify how this virus is attenuated compared to its wild-type parent, DENV2 16681. Site-directed mutagenesis on a 16681 infectious clone identifies a single G53D substitution in the non-structural 1 (NS1) protein that reduces 16681 infection and dissemination in both Aedes aegypti, as well as in mammalian cells to produce the characteristic phenotypes of PDK53. Mechanistically, NS1 G53D impairs the function of a known host factor, the endoplasmic reticulum (ER)-resident ribophorin 1 protein, to properly glycosylate NS1 and thus induce a host antiviral gene through ER stress responses. Our findings provide molecular insights on DENV attenuation on a clinically tested strain.

摘要

登革热病毒(DENV)减毒的分子基础仍不清楚,这阻碍了针对衍生安全但仍具有免疫原性的活疫苗候选物的靶向方法。在这里,我们利用最近成功完成 3 期临床试验的登革热病毒 2 型 PDK53 疫苗株,来确定与野生型亲本 DENV2 16681 相比,该病毒是如何减毒的。在 16681 感染性克隆上进行的定点诱变鉴定出 NS1 蛋白中的单个 G53D 取代,该取代降低了 16681 在埃及伊蚊以及哺乳动物细胞中的感染和传播,从而产生 PDK53 的特征表型。从机制上讲,NS1 G53D 会损害一种已知的宿主因子(内质网驻留的核糖体蛋白 1 蛋白)的功能,从而无法正确糖基化 NS1,因此通过内质网应激反应诱导宿主抗病毒基因。我们的研究结果为在经过临床测试的毒株上进行的 DENV 减毒提供了分子见解。

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