Sequencing 4.3 million mutations in wheat promoters to understand and modify gene expression

Author:

Zhang Junli1,Xiong Hongchun12,Burguener Germán F.13,Vasquez-Gross Hans14,Liu Qiujie13ORCID,Debernardi Juan M.13,Akhunova Alina5,Garland-Campbell Kimberly6,Kianian Shahryar F.7,Brown-Guedira Gina8,Pozniak Curtis9ORCID,Faris Justin D.10,Akhunov Eduard5,Dubcovsky Jorge13ORCID

Affiliation:

1. Department of Plant Sciences, University of California, Davis, CA 95616

2. Institute of Crop Sciences, Chinese Academy of Agricultural Sciences, Beijing 100081, China

3. HHMI, Chevy Chase, MD 20815

4. Nevada Bioinformatics Center, University of Nevada, Reno, NV 89557

5. Department of Plant Pathology, Kansas State University, Manhattan, KS 66506

6. United States Department of Agriculture - Agricultural Research Service, Wheat Health, Genetics and Quality Research Unit, Pullman, WA 99164

7. United States Department of Agriculture - Agricultural Research Service, Cereal Disease Laboratory, Saint Paul, MN 55108-6086

8. United States Department of Agriculture - Agricultural Research Service, Plant Science Research Unit, Raleigh, NC 27695

9. Crop Development Centre, University of Saskatchewan, Saskatoon S7N 5A8, Canada

10. United States Department of Agriculture - Agricultural Research Service, Cereal Crops Research Unit, Northern Crop Science Laboratory, Fargo, ND 58102

Abstract

Wheat is an important contributor to global food security, and further improvements are required to feed a growing human population. Functional genetics and genomics tools can help us to understand the function of different genes and to engineer beneficial changes. In this study, we used a promoter capture assay to sequence 2-kb regions upstream of all high-confidence annotated genes from 1,513 mutagenized plants from the tetraploid wheat variety Kronos. We identified 4.3 million induced mutations with an accuracy of 99.8%, resulting in a mutation density of 41.9 mutations per kb. We also remapped Kronos exome capture reads to Chinese Spring RefSeq v1.1, identified 4.7 million mutations, and predicted their effects on annotated genes. Using these predictions, we identified 59% more nonsynonymous substitutions and 49% more truncation mutations than in the original study. To show the biological value of the promoter dataset, we selected two mutations within the promoter of the VRN-A1 vernalization gene. Both mutations, located within transcription factor binding sites, significantly altered VRN-A1 expression, and one reduced the number of spikelets per spike. These publicly available sequenced mutant datasets provide rapid and inexpensive access to induced variation in the promoters and coding regions of most wheat genes. These mutations can be used to understand and modulate gene expression and phenotypes for both basic and commercial applications, where limited governmental regulations can facilitate deployment. These mutant collections, together with gene editing, provide valuable tools to accelerate functional genetic studies in this economically important crop.

Funder

USDA | National Institute of Food and Agriculture

Howard Hughes Medical Institute

International Atomic Energy Agency

Publisher

Proceedings of the National Academy of Sciences

Subject

Multidisciplinary

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