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用于鉴定与HIV-1 Gag相关的宿主因子的串联免疫沉淀方法。

Tandem immunoprecipitation approach to identify HIV-1 Gag associated host factors.

作者信息

Gao Wei, Li Min, Zhang Jingxin

机构信息

Liaoning Medical University, First Affiliated Hospital, Jinzhou, Liaoning 121001, China.

Chinese Academy of Medical Sciences & Peking Union Medical College, Beijing 100050, China.

出版信息

J Virol Methods. 2014 Jul;203:116-9. doi: 10.1016/j.jviromet.2014.03.017. Epub 2014 Mar 30.

Abstract

HIV-1 Gag by itself is able to assemble and release from host cells and thus serves as a simplified model to identify host factors involved in this stage of the HIV-1 life cycle. In this study, a tandem immunoprecipitation approach is taken to immunoprecipitate Gag-interacting host proteins from transfected 293T cells. It is demonstrated that with the tandem immunoprecipitation method Gag-interacting host factors can be precipitated more efficiently than by single-step immunoprecipitation. Gag proteins are found to interact with multiple RNA-binding proteins such as hnRNPs, nucleolin, EF1a and ribosomal proteins. Such interactions are mediated by cellular RNAs and the Gag Nuclear Capsid (NC) domain. Deletion of the NC domain results in removal of most of the RNA-binding proteins, as well as a reduction of the Gag releasing capability, which can be restored by replacing the deleted NC domain with another multimerization motif. Importantly, interactions between Gag and host factors are relevant functionally, as evidenced by significantly increased nucleolin protein in the cytoplasm where it is recruited into the Gag complex, and enhanced Gag release when nucleolin is over-expressed.

摘要

HIV-1 Gag自身能够从宿主细胞组装并释放,因此可作为一个简化模型来鉴定参与HIV-1生命周期这一阶段的宿主因子。在本研究中,采用串联免疫沉淀方法从转染的293T细胞中免疫沉淀与Gag相互作用的宿主蛋白。结果表明,与单步免疫沉淀相比,串联免疫沉淀方法能更有效地沉淀与Gag相互作用的宿主因子。发现Gag蛋白与多种RNA结合蛋白相互作用,如hnRNPs、核仁素、EF1a和核糖体蛋白。这种相互作用由细胞RNA和Gag核衣壳(NC)结构域介导。删除NC结构域会导致大多数RNA结合蛋白的去除,以及Gag释放能力的降低,通过用另一个多聚化基序替换缺失的NC结构域可恢复该能力。重要的是,Gag与宿主因子之间的相互作用在功能上是相关的,这一点这一点得到了证实,证据是在细胞质中核仁素蛋白显著增加,它被招募到Gag复合物中,并且当核仁素过表达时Gag释放增强。

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