Lysine 2‐hydroxyisobutyrylation proteomics analyses reveal the regulatory mechanism of CaMYB61‐CaAFR1 module in regulating stem development in Capsicum annuum L.

Author:

Li Qing12ORCID,Fu Canfang12,Hu Bowen12,Yang Bozhi12,Yu Huiyang12,He Huan12,Xu Qing12,Chen Xuejun3,Dai Xiongze12,Fang Rong3,Xiong Xingyao4,Zhou Kunhua3,Yang Sha12,Zou Xuexiao12,Liu Zhoubin12ORCID,Ou Lijun12

Affiliation:

1. Engineering Research Center of Education, Ministry for Germplasm Innovation and Breeding New Varieties of Horticultural Crops, Key Laboratory for Vegetable Biology of Hunan Province, College of Horticulture Hunan Agricultural University Changsha 410125 China

2. Yuelushan Lab Changsha 410128 China

3. Vegetable and Flower Institute, Jiangxi Academy of Agricultural Sciences Nanchang 330200 China

4. Shenzhen Branch, Guangdong Laboratory for Lingnan Modern Agriculture, Key Laboratory of Synthetic Biology, Ministry of Agriculture and Rural Affairs, Agricultural Genomics Institute at Shenzhen Chinese Academy of Agricultural Sciences Shenzhen 518000 China

Abstract

SUMMARYPlant stems constitute the most abundant renewable resource on earth. The function of lysine (K)‐2‐hydroxyisobutyrylation (Khib), a novel post‐translational modification (PTM), has not yet been elucidated in plant stem development. Here, by assessing typical pepper genotypes with straight stem (SS) and prostrate stem (PS), we report the first large‐scale proteomics analysis for protein Khib to date. Khib‐modifications influenced central metabolic processes involved in stem development, such as glycolysis/gluconeogenesis and protein translation. The high Khib level regulated gene expression and protein accumulation associated with cell wall formation in the pepper stem. Specially, we found that CaMYB61 knockdown lines that exhibited prostrate stem phenotypes had high Khib levels. Most histone deacetylases (HDACs, e.g., switch‐independent 3 associated polypeptide function related 1, AFR1) potentially function as the “erasing enzymes” involved in reversing Khib level. CaMYB61 positively regulated CaAFR1 expression to erase Khib and promote cellulose and hemicellulose accumulation in the stem. Therefore, we propose a bidirectional regulation hypothesis of “Khib modifications” and “Khib erasing” in stem development, and reveal a novel epigenetic regulatory network in which the CaMYB61‐CaAFR1 molecular module participating in the regulation of Khib levels and biosynthesis of cellulose and hemicellulose for the first time.

Funder

National Natural Science Foundation of China

Hunan Provincial Innovation Foundation for Postgraduate

Natural Science Foundation of Hunan Province

Publisher

Wiley

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