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Comparison of helper component-protease RNA silencing suppression activity, subcellular localization, and aggregation of three Korean isolates of Turnip mosaic virus

机译:螺杆组分 - 蛋白酶RNA沉默抑制活性,亚细胞定位和三孔叶片病毒的三个朝鲜分离物的聚集的比较

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摘要

In 2014, we performed a nationwide survey in Korean radish fields to investigate the distribution and variability of Turnip mosaic virus (TuMV). Brassica rapa ssp. pekinensis sap-inoculated with three isolates of TuMV from infected radish tissue showed different symptom severities, whereas symptoms in Raphanus sativus were similar for each isolate. The helper component-protease (HC-Pro) genes of each isolate were sequenced, and phylogenetic analysis showed that the three Korean isolates were clustered into the basal-BR group. The HC-Pro proteins of these isolates were tested for their RNA silencing suppressor (VSR) activity and subcellular localization in Nicotiana benthamiana. A VSR assay by co-agroinfiltration of HC-Pro with soluble-modified GFP (smGFP) showed that HC-Pro of isolate R007 and R041 showed stronger VSR activity than R065. The HC-Pros showed 98.25 % amino acid identity, and weak VSR isolate (R065) has a single variant residue in the C-terminal domain associated with protease activity and self-interaction compared to isolates with strong VSR activity. Formation of large subcellular aggregates of GFP: HC-Pro fusion proteins in N. benthamiana was only observed for HC-Pro from isolates with strong VSR activity, suggesting that R065 'weak' HC-Pro may have diminished self-association; substitution of the variant C-terminal residue largely reversed the HC-Pro aggregation and silencing suppressor characteristics. The lack of correlation between VSR efficiency and induction of systemic necrosis (SN) suggests that differences in viral accumulation due to HC-Pro are not responsible for SN.
机译:2014年,我们在韩国萝卜领域进行了全国范围的调查,探讨了萝卜马扎病毒(Tumv)的分布和变异性。芸苔属rapa ssp。 Pekinensis SAP接种来自来自受感染的萝卜组织的三个分离株的肿瘤株显示出不同的症状剧烈症状,而Raphanus Sativus的症状对于每个分离物类似。测序每个分离物的辅助组分 - 蛋白酶(HC-Pro)基因,并且系统发育分析表明将三个韩国分离物聚集到基础-Br组中。测试这些分离株的HC-Pro蛋白在尼古利亚纳·斯坦氨基裔中的RNA沉默抑制剂(VSR)活性和亚细胞定位。通过具有可溶性改性的GFP(SMGFP)的HC-Pro的共传播的VSR测定表明,分离物R007和R041的HC-Pro显示出比R065更强的VSR活性。 HC-ProS显示出98.25%的氨基酸同一性,弱VSR分离物(R065)在与蛋白酶活性和自相互作用相关的C末端结构域中具有单个变体残留物,与具有强VSR活性的分离物相比。 GFP的大亚细胞聚集体的形成:N型果实蛋白在N必需的N必需蛋白中仅针对具有强大VSR活性的分离株观察到HC-Pro,表明R065'HC-Pro可以减少自我关联;变体C末端残留物的取代在很大程度上反转了HC-Pro聚集和沉默抑制器特性。 VSR效率与系统坏死(SN)诱导之间的相关性表明,HC-Pro引起的病毒累积差异不负责任。

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