Construction of Host Plant Insect‐Resistance Mutant Library by High‐Throughput CRISPR/Cas9 System and Identification of A Broad‐Spectrum Insect Resistance Gene

Author:

Sun Lin12,Alariqi Muna13ORCID,Wang Yaxin1,Wang Qiongqiong1,Xu Zhongping1,Zafar Muhammad Naeem1,Yang Guangqin1,Jia Ruoyu1,Hussain Amjad1,Chen Yilin1,Ding Xiao1,Zhou Jiawei1,Wang Guanying1,Wang Fuqiu1,Li Jianying1,Zou Jiawei1,Zhu Xiangqian1,Yu Lu1,Sun Yiwen1,Liang Sijia1,Hui Fengjiao1,Chen Luo1,Guo Weifeng4,Wang Yanqin4,Zhu Huaguo5,Lindsey Keith6,Nie Xinhui7,Zhang Xianlong1,Jin Shuangxia1

Affiliation:

1. Hubei Hongshan Laboratory National Key Laboratory of Crop Genetic Improvement Huazhong Agricultural University Wuhan Hubei 430070 P. R. China

2. Institute of Industrial Crops Shandong Academy of Agricultural Sciences Jinan Shandong 250100 China

3. Department of Agronomy and Pastures, Faculty of Agriculture Sana’a University Sana’a Yemen

4. Xinjiang Production and Construction Corps Key Laboratory of Protection and Utilization of Biological Resources in Tarim Basin Tarim University Alaer Xinjiang 843300 China

5. College of Biology and Agricultural Resources Huanggang Normal University Huanggang Hubei 438000 China

6. Department of Biosciences Durham University Durham DH1 3LE UK

7. Key Laboratory of Oasis Ecology Agricultural of Xinjiang Bingtuan Agricultural College Shihezi University Shihezi Xinjiang China

Abstract

AbstractInsects pose significant challenges in cotton‐producing regions. Here, they describe a high‐throughput CRISPR/Cas9‐mediated large‐scale mutagenesis library targeting endogenous insect‐resistance‐related genes in cotton. This library targeted 502 previously identified genes using 968 sgRNAs, generated ≈2000 T0 plants and achieved 97.29% genome editing with efficient heredity, reaching upto 84.78%. Several potential resistance‐related mutants (10% of 200 lines) their identified that may contribute to cotton‐insect molecular interaction. Among these, they selected 139 and 144 lines showing decreased resistance to pest infestation and targeting major latex‐like protein 423 (GhMLP423) for in‐depth study. Overexpression of GhMLP423 enhanced insect resistance by activating the plant systemic acquired resistance (SAR) of salicylic acid (SA) and pathogenesis‐related (PR) genes. This activation is induced by an elevation of cytosolic calcium [Ca2+]cyt flux eliciting reactive oxygen species (ROS), which their demoted in GhMLP423 knockout (CR) plants. Protein‐protein interaction assays revealed that GhMLP423 interacted with a human epidermal growth factor receptor substrate15 (EPS15) protein at the cell membrane. Together, they regulated the systemically propagating waves of Ca2+ and ROS, which in turn induced SAR. Collectively, this large‐scale mutagenesis library provides an efficient strategy for functional genomics research of polyploid plant species and serves as a solid platform for genetic engineering of insect resistance.

Publisher

Wiley

Subject

General Physics and Astronomy,General Engineering,Biochemistry, Genetics and Molecular Biology (miscellaneous),General Materials Science,General Chemical Engineering,Medicine (miscellaneous)

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