A robust high‐throughput functional screening assay for plant pathogen effectors using the TMV‐GFP vector

生物 效应器 绿色荧光蛋白 高通量筛选 病菌 吞吐量 载体(分子生物学) 病毒学 计算生物学 细胞生物学 微生物学 遗传学 基因 重组DNA 电信 计算机科学 无线
作者
Peng Cao,Haotian Shi,Shuangxi Zhang,Jialan Chen,Rongbo Wang,Peiqing Liu,Yingfang Zhu,Yuyan An,Meixiang Zhang
出处
期刊:Plant Journal [Wiley]
标识
DOI:10.1111/tpj.16774
摘要

SUMMARY Uncovering the function of phytopathogen effectors is crucial for understanding mechanisms of pathogen pathogenicity and for improving our ability to protect plants from diseases. An increasing number of effectors have been predicted in various plant pathogens. Functional characterization of these effectors has become a major focus in the study of plant–pathogen interactions. In this study, we designed a novel screening system that combines the TMV (tobacco mosaic virus)‐GFP vector and Agrobacterium ‐mediated transient expression in the model plant Nicotiana benthamiana . This system enables the rapid identification of effectors that interfere with plant immunity. The biological function of these effectors can be easily evaluated by observing the GFP fluorescence signal using a UV lamp within just a few days. To evaluate the TMV‐GFP system, we initially tested it with well‐described virulence and avirulence type III effectors from the bacterial pathogen Ralstonia solanacearum . After proving the accuracy and efficiency of the TMV‐GFP system, we successfully screened a novel virulence effector, RipS1, using this approach. Furthermore, using the TMV‐GFP system, we reproduced consistent results with previously known cytoplasmic effectors from a diverse array of pathogens. Additionally, we demonstrated the effectiveness of the TMV‐GFP system in identifying apoplastic effectors. The easy operation, time‐saving nature, broad effectiveness, and low technical requirements of the TMV‐GFP system make it a promising approach for high‐throughput screening of effectors with immune interference activity from various pathogens.
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