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评估黄病毒蛋白酶在埃及伊蚊细胞中对登革病毒2衍生的切割位点的特异性。

Evaluating the specificity of flavivirus proteases in Aedes aegypti cells for dengue virus 2-derived cleavage sites.

作者信息

Dingle Alexius O, Adelman Zach N

机构信息

Department of Entomology, Texas A&M AgriLife, Texas A&M University, College Station, TX, United States of America.

Interdisciplinary Graduate Program in Genetics and Genomics, Texas A&M University, College Station, TX, United States of America.

出版信息

PLoS One. 2024 Dec 3;19(12):e0309095. doi: 10.1371/journal.pone.0309095. eCollection 2024.

Abstract

Flaviviruses are a diverse group of RNA viruses known for their significant impact on human health worldwide. We generated a series of reporters that included cleavage sequences from the dengue virus type 2 polyprotein and co-transfected with plasmids encoding various flavivirus proteases into Aedes aegypti cells, followed by fluorescent imaging and western blot analysis for the determination of proteolytic cleavage. Recombinant flavivirus NS2B3 proteases from medically significant and insect-specific flaviviruses were able to process reporters encoding cleavage sequences from the dengue virus type 2 polyprotein in vitro including proteases from dengue virus types 1-4, Zika virus, yellow fever virus, Aedes flavivirus, and cell-fusing agent virus. Reporters were not cleaved when transfected cells were infected with dengue virus type 2. Endoplasmic reticulum tethered reporters were also cleaved by protease alone but not by infectious virus. These results shed light on the ability of multiple flavivirus proteases to cleave sequences derived from outside of their genome and raise new questions concerning the requirements for effective cleavage by flavivirus proteases in trans.

摘要

黄病毒是一类多样的RNA病毒,因其对全球人类健康的重大影响而闻名。我们构建了一系列报告基因,其中包含登革热病毒2型多聚蛋白的切割序列,并将其与编码各种黄病毒蛋白酶的质粒共转染到埃及伊蚊细胞中,随后进行荧光成像和蛋白质印迹分析以确定蛋白水解切割情况。来自具有医学意义的黄病毒和昆虫特异性黄病毒的重组黄病毒NS2B3蛋白酶能够在体外切割编码登革热病毒2型多聚蛋白切割序列的报告基因,这些蛋白酶包括来自1 - 4型登革热病毒、寨卡病毒、黄热病毒、伊蚊黄病毒和细胞融合剂病毒的蛋白酶。当用2型登革热病毒感染转染细胞时,报告基因未被切割。内质网锚定的报告基因也仅被蛋白酶切割,而不被感染性病毒切割。这些结果揭示了多种黄病毒蛋白酶切割其基因组外序列的能力,并提出了关于黄病毒蛋白酶在反式切割中有效切割所需条件的新问题。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/15ff/11614287/e1c7f13a67b7/pone.0309095.g001.jpg

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