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通过全基因组表达谱分析确定马立克氏病病毒在淋巴母细胞系中自发裂解转换过程中的差异表达基因。

Differentially expressed genes during spontaneous lytic switch of Marek's disease virus in lymphoblastoid cell lines determined by global gene expression profiling.

作者信息

Mwangi William N, Vasoya Deepali, Kgosana Lydia B, Watson Mick, Nair Venugopal

机构信息

Avian Viral Diseases Programme, UK-China Centre of Excellence on Avian Disease Research, The Pirbright Institute, Pirbright, Surrey, UK.

Division of Genetics and Genomics, The Roslin Institute, R(D)SVS, University of Edinburgh, Easter Bush, Midlothian, UK.

出版信息

J Gen Virol. 2017 Apr;98(4):779-790. doi: 10.1099/jgv.0.000744.

Abstract

Marek's disease virus (MDV), an alphaherpesvirus of poultry, causes Marek's disease and is characterized by visceral CD4+TCRαβ+ T-cell lymphomas in susceptible hosts. Immortal cell lines harbouring the viral genome have been generated from ex vivo cultures of MD tumours. As readily available sources of large numbers of cells, MDV-transformed lymphoblastoid cell lines (LCLs) are extremely valuable for studies of virus-host interaction. While the viral genome in most cells is held in a latent state, minor populations of cells display spontaneous reactivation identifiable by the expression of lytic viral genes. Spontaneous reactivation in these cells presents an opportunity to investigate the biological processes involved in the virus reactivation. For detailed characterization of the molecular events associated with reactivation, we used two lymphoblastoid cell lines derived from lymphomas induced by pRB1B-UL47eGFP, a recombinant MDV engineered to express enhanced green fluorescent protein (EGFP) fused with the UL47. We used fluorescence-activated cell sorting to purify the low-frequency EGFP-positive cells with a spontaneously activating viral genome from the majority EGFP-negative cells and analysed their gene expression profiles by RNA-seq using Illumina HiSeq2500. Ingenuity pathway analysis on more than 2000 differentially expressed genes between the lytically infected (EGFP-positive) and latently infected (EGFP-negative) cell populations identified the biological pathways involved in the reactivation. Virus-reactivating cells exhibited differential expression of a significant number of viral genes, with hierarchical differences in expression levels. Downregulation of a number of host genes including those directly involved in T-cell activation, such as CD3, CD28, ICOS and phospholipase C, was also noticed in the LCL undergoing lytic switch.

摘要

马立克氏病病毒(MDV)是一种家禽α疱疹病毒,可引起马立克氏病,其特征是在易感宿主中引发内脏CD4+TCRαβ+ T细胞淋巴瘤。已从MD肿瘤的体外培养物中产生了携带病毒基因组的永生细胞系。作为大量细胞的现成来源,MDV转化的淋巴母细胞系(LCL)对于病毒-宿主相互作用的研究极具价值。虽然大多数细胞中的病毒基因组处于潜伏状态,但少数细胞群体表现出可通过裂解性病毒基因的表达来识别的自发激活。这些细胞中的自发激活为研究病毒激活所涉及的生物学过程提供了机会。为了详细表征与激活相关的分子事件,我们使用了两种源自pRB1B-UL47eGFP诱导的淋巴瘤细胞的淋巴母细胞系,pRB1B-UL47eGFP是一种经工程改造以表达与UL47融合的增强型绿色荧光蛋白(EGFP)的重组MDV。我们使用荧光激活细胞分选技术从大多数EGFP阴性细胞中纯化出具有自发激活病毒基因组的低频EGFP阳性细胞,并使用Illumina HiSeq2500通过RNA测序分析它们的基因表达谱。对裂解感染(EGFP阳性)和潜伏感染(EGFP阴性)细胞群体之间2000多个差异表达基因进行的 Ingenuity 通路分析确定了激活过程中涉及的生物学通路。病毒激活细胞表现出大量病毒基因的差异表达,表达水平存在层次差异。在经历裂解转换的LCL中还注意到许多宿主基因的下调,包括那些直接参与T细胞激活的基因,如CD3、CD28、ICOS和磷脂酶C。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8647/5657026/e9492d9cc135/jgv-98-779-g001.jpg

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