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用于研究人类嗜T淋巴细胞病毒1型传播的报告系统。

Reporter Systems to Study HTLV-1 Transmission.

作者信息

Gross Christine, Thoma-Kress Andrea K

机构信息

Institute of Clinical and Molecular Virology, Friedrich-Alexander-Universität Erlangen-Nürnberg, Schlossgarten 4, 91054, Erlangen, Germany.

出版信息

Methods Mol Biol. 2017;1582:33-46. doi: 10.1007/978-1-4939-6872-5_3.

DOI:10.1007/978-1-4939-6872-5_3
PMID:28357660
Abstract

The retrovirus Human T-lymphotropic virus type 1 (HTLV-1) preferentially infects CD4 T-cells via cell-to-cell transmission, while cell-free infection of T-cells is inefficient. Substantial insights into the different routes of transmission have largely been obtained by imaging techniques or by flow cytometry. Recently, strategies to quantify infection events with HTLV-1 improved. In this chapter, we present two different methods to quantitate virus transmission. Both methods are based on measuring gene activity of luciferase with a cost-saving in-house luciferase assay. First, we established a reporter Jurkat T-cell line carrying a luciferase gene under the control of the HTLV-1 core promoter U3R. Upon co-culture with chronically HTLV-1-infected T-cell lines, reporter cells are infected, and upon expression of the viral transactivator Tax, the viral promoter is activated resulting in enhanced luciferase activity. However, this assay as presented here does not exclude cell fusion as the mechanism allowing intracellular Tax-dependent activation of luciferase gene expression. Therefore, we describe a second method, the single-cycle replication-dependent reporter system developed by Mazurov et al. (PLoS Pathog 6:e1000788, 2010) that allows quantitation of HTLV-1 infection in co-cultured cells. Taken together, both methods facilitate quantitation of HTLV-1 transmission and will help to unravel pathways required for cell-to-cell transmission on a quantitative basis.

摘要

逆转录病毒1型人类嗜T淋巴细胞病毒(HTLV-1)通过细胞间传播优先感染CD4 T细胞,而T细胞的游离病毒感染效率较低。通过成像技术或流式细胞术,在很大程度上获得了对不同传播途径的深入了解。最近,量化HTLV-1感染事件的策略有所改进。在本章中,我们介绍两种不同的定量病毒传播的方法。这两种方法均基于用节省成本的内部荧光素酶测定法测量荧光素酶的基因活性。首先,我们建立了一个报告Jurkat T细胞系,该细胞系携带一个在HTLV-1核心启动子U3R控制下的荧光素酶基因。与长期感染HTLV-1的T细胞系共培养时,报告细胞被感染,并且在病毒反式激活因子Tax表达后,病毒启动子被激活,导致荧光素酶活性增强。然而,此处介绍的该测定法并不排除细胞融合作为允许荧光素酶基因表达进行细胞内Tax依赖性激活的机制。因此,我们描述了第二种方法,即由马祖罗夫等人开发的单周期复制依赖性报告系统(《公共科学图书馆·病原体》6:e1000788,2010年),该系统可对共培养细胞中的HTLV-1感染进行定量。综上所述,这两种方法都有助于对HTLV-1传播进行定量,并将有助于在定量基础上揭示细胞间传播所需的途径。

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