Proteomics Analysis Identifies IRSp53 and Fascin as Critical for PRV Egress and Direct Cell–Cell Transmission

聚束蛋白 生物 细胞生物学 细胞骨架 CDC42型 蛋白质组 丝状体 蛋白质组学 细胞外 肌动蛋白 细胞 基因 生物化学
作者
Fei‐Long Yu,Huan Miao,Jinjin Xia,Fan Jia,Huadong Wang,Fuqiang Xu,Lin Guo
出处
期刊:Proteomics [Wiley]
卷期号:19 (23) 被引量:6
标识
DOI:10.1002/pmic.201900009
摘要

Abstract Pseudorabies virus (PRV) has been widely used as a live trans‐synaptic tracer for mapping neuronal circuits. Systematically identifying mature PRV virion proteomes and defining co‐purified host proteins are necessary to fully understand the detailed mechanism underlying PRV transmission processes. Here, a PRV virion purification strategy based on sorting with flow cytometry is developed and the mature extracellular and intracellular PRV virion proteomes using LC coupled with MS/MS are characterized. In addition to viral proteins, a large number of host proteins are also identified, including proteins related to actin cytoskeletal dynamics and membrane protrusion. How many of these host proteins are true virion components are unknown and the majority of these may not be. Through functional analysis, it is found that IRSp53 and fascin are critical for the egress process and play a role in direct cell–cell transmission. Moreover, it is shown that CDC42 and Rac1 are also involved in the production of mature extracellular virions. The results suggest that the formation of the filopodia‐like cytoskeleton and the rearrangement of the membrane, which are both associated with IRSp53 and fascin, may be important for the transmission of viruses used in neuronal tracing.
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