In‐locus gene silencing in plants using genome editing

Author:

Shen Rundong123ORCID,Yao Qi13ORCID,Tan Xinhang3ORCID,Ren Wendan1ORCID,Zhong Dating13,Zhang Xuening1,Li Xinbo2ORCID,Dong Chao2ORCID,Cao Xuesong4ORCID,Tian Yifu12ORCID,Zhu Jian‐Kang24ORCID,Lu Yuming1ORCID

Affiliation:

1. Shanghai Collaborative Innovation Center of Agri‐Seeds, Joint Center for Single Cell Biology, School of Agriculture and Biology Shanghai Jiao Tong University Shanghai 200240 China

2. Institute of Crop Sciences/National Nanfan Research Institute, Chinese Academy of Agricultural Sciences (CAAS), and Key Laboratory of Gene Editing Technologies (Hainan), Ministry of Agriculture and Rural Affairs Sanya 572024 China

3. Shanghai Center for Plant Stress Biology, Center for Excellence in Molecular Plant Sciences, Chinese Academy of Sciences Shanghai 201602 China

4. Institute of Advanced Biotechnology, and School of Life Sciences Southern University of Science and Technology Shenzhen 518055 China

Abstract

Summary Gene silencing is crucial in crop breeding for desired trait development. RNA interference (RNAi) has been used widely but is limited by ectopic expression of transgenes and genetic instability. Introducing an upstream start codon (uATG) into the 5′untranslated region (5′UTR) of a target gene may ‘silence’ the target gene by inhibiting protein translation from the primary start codon (pATG). Here, we report an efficient gene silencing method by introducing a tailor‐designed uATG‐containing element (ATGE) into the 5′UTR of genes in plants, occupying the original start site to act as a new pATG. Using base editing to introduce new uATGs failed to silence two of the tested three rice genes, indicating complex regulatory mechanisms. Precisely inserting an ATGE adjacent to pATG achieved significant target protein downregulation. Through extensive optimization, we demonstrated this strategy substantially and consistently downregulated target protein expression. By designing a bidirectional multifunctional ATGE4, we enabled tunable knockdown from 19% to 89% and observed expected phenotypes. Introducing ATGE into Waxy, which regulates starch synthesis, generated grains with lower amylose, revealing the value for crop breeding. Together, we have developed a programmable and robust method to knock down gene expression in plants, with potential for biological mechanism exploration and crop enhancement.

Funder

China Postdoctoral Science Foundation

National Natural Science Foundation of China

National Key Research and Development Program of China

Publisher

Wiley

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