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从人胚肾293细胞中优化重组寨卡病毒NS1蛋白的分泌

Optimization of recombinant Zika virus NS1 protein secretion from HEK293 cells.

作者信息

Roldán Julieta S, Cassola Alejandro, Castillo Daniela S

机构信息

Instituto de Investigaciones Biotecnológicas "Dr. Rodolfo A. Ugalde" (IIBIO), Universidad Nacional de San Martín (UNSAM) - Consejo Nacional de Investigaciones Científicas y Técnicas (CONICET), San Martín, Buenos Aires, Argentina.

出版信息

Biotechnol Rep (Amst). 2020 Feb 11;25:e00434. doi: 10.1016/j.btre.2020.e00434. eCollection 2020 Mar.

Abstract

Sensitive, accurate and cost-effective diagnostic tests are urgently needed to detect Zika virus (ZIKV) infection. Nonstructural 1 (NS1) glycoprotein is an excellent diagnostic marker since it is released in a hexameric conformation from infected cells into the patient's bloodstream early in the course of the infection. We established a stable rZNS1-His-expression system in HEK293 cells through lentiviral transduction. A novel optimization approach to enhance rZNS1-His protein secretion in the mammalian expression system was accomplished through 50 nM rapamycin incubation followed by serum-free media incubation for 9 days, reaching protein yields of ∼10 mg/l of culture medium. Purified rZNS1-His hexamer was recognized by anti-NS1 antibodies in ZIKV patient's serum, and showed the ability to induce a humoral response in immunized mice. The obtained recombinant protein is a reliable biological tool that can potentially be applied in the development of diagnostic tests to detect ZIKV in infected patients during the acute phase.

摘要

迫切需要灵敏、准确且经济高效的诊断测试来检测寨卡病毒(ZIKV)感染。非结构蛋白1(NS1)糖蛋白是一种出色的诊断标志物,因为在感染过程早期,它会以六聚体构象从受感染细胞释放到患者血液中。我们通过慢病毒转导在HEK293细胞中建立了稳定的rZNS1-His表达系统。通过50 nM雷帕霉素孵育,然后在无血清培养基中孵育9天,实现了一种在哺乳动物表达系统中增强rZNS1-His蛋白分泌的新型优化方法,培养基中的蛋白产量达到约10 mg/l。纯化的rZNS1-His六聚体可被寨卡病毒患者血清中的抗NS1抗体识别,并在免疫小鼠中显示出诱导体液免疫反应的能力。所获得的重组蛋白是一种可靠的生物学工具,有可能应用于开发诊断测试,以在急性期检测感染患者体内的寨卡病毒。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/83e1/7033529/d4458d410f2b/gr1.jpg

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