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首页> 美国卫生研究院文献>PLoS Pathogens >Interaction of the Trans-Frame Potyvirus Protein P3N-PIPO with Host Protein PCaP1 Facilitates Potyvirus Movement
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Interaction of the Trans-Frame Potyvirus Protein P3N-PIPO with Host Protein PCaP1 Facilitates Potyvirus Movement

机译:跨框架杯状病毒蛋白P3N-PIPO与宿主蛋白PCaP1的相互作用促进杯状病毒运动。

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A small open reading frame (ORF), pipo, overlaps with the P3 coding region of the potyviral polyprotein ORF. Previous evidence suggested a requirement for pipo for efficient viral cell-to-cell movement. Here, we provide immunoblotting evidence that the protein PIPO is expressed as a trans-frame protein consisting of the amino-terminal half of P3 fused to PIPO (P3N-PIPO). P3N-PIPO of Turnip mosaic virus (TuMV) fused to GFP facilitates its own cell-to-cell movement. Using a yeast two-hybrid screen, co-immunoprecipitation assays, and bimolecular fluorescence complementation (BiFC) assays, we found that P3N-PIPO interacts with host protein PCaP1, a cation-binding protein that attaches to the plasma membrane via myristoylation. BiFC revealed that it is the PIPO domain of P3N-PIPO that binds PCaP1 and that myristoylation of PCaP1 is unnecessary for interaction with P3N-PIPO. In PCaP1 knockout mutants (pcap1) of Arabidopsis, accumulation of TuMV harboring a GFP gene (TuMV-GFP) was drastically reduced relative to the virus level in wild-type plants, only small localized spots of GFP were visible, and the plants showed few symptoms. In contrast, TuMV-GFP infection in wild-type Arabidopsis yielded large green fluorescent patches, and caused severe stunting. However, viral RNA accumulated to high level in protoplasts from pcap1 plants indicating that PCaP1 is not required for TuMV RNA synthesis. In contrast to TuMV, the tobamovirus Oilseed rape mosaic virus did not require PCaP1 to infect Arabidopsis plants. We conclude that potyviral P3N-PIPO interacts specifically with the host plasma membrane protein PCaP1 to participate in cell-to-cell movement. We speculate that PCaP1 links a complex of viral proteins and genomic RNA to the plasma membrane by binding P3N-PIPO, enabling localization to the plasmodesmata and cell-to-cell movement. The PCaP1 knockout may contribute to a new strategy for recessive resistance to potyviruses.
机译:一个小的开放阅读框(ORF)pipo与杯状病毒多蛋白ORF的P3编码区重叠。先前的证据表明需要pipo才能有效地实现病毒在细胞间的移动。在这里,我们提供了免疫印迹证据,表明PIPO蛋白表达为跨框架蛋白,由与PIPO(P3N-PIPO)融合的P3氨基末端一半组成。与GFP融合的芜菁花叶病毒(TuMV)的P3N-PIPO促进了其自身的细胞间移动。使用酵母双杂交筛选,免疫共沉淀测定法和双分子荧光互补(BiFC)测定法,我们发现P3N-PIPO与宿主蛋白PCaP1相互作用,后者是一种通过肉豆蔻酰化作用附着在质膜上的阳离子结合蛋白。 BiFC揭示了结合PCaP1的是P3N-PIPO的PIPO域,而PCaP1的豆蔻酰化对于与P3N-PIPO的相互作用是不必要的。在拟南芥的PCaP1基因敲除突变体(pcap1)中,相对于野生型植物中的病毒水平,带有GFP基因(TuMV-GFP)的TuMV的积累量大大减少,只有GFP的局部小斑点可见,并且植物显示很少症状。相反,野生型拟南芥中的TuMV-GFP感染会产生大的绿色荧光斑,并导致严重的发育迟缓。但是,病毒RNA在pcap1植物的原生质体中积累了很高的水平,这表明TuMV RNA合成不需要PCaP1。与TuMV相比,烟草花叶病毒油菜籽花叶病毒不需要PCaP1感染拟南芥植物。我们得出结论,potyviral P3N-PIPO与宿主质膜蛋白PCaP1特异性相互作用,参与细胞间的运动。我们推测PCaP1通过结合P3N-PIPO将病毒蛋白和基因组RNA的复合体连接到质膜上,从而定位到质膜和细胞间移动。 PCaP1基因敲除可能有助于对马铃薯病毒的隐性抗性的新策略。

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