Data-independent acquisition-based global phosphoproteomics reveal the diverse roles of casein kinase 1 in plant development

Li Qu; Moyang Liu; Lingli Zheng; Xu Wang; Hongwei Xue

doi:10.1016/j.scib.2023.08.017

Data-independent acquisition-based global phosphoproteomics reveal the diverse roles of casein kinase 1 in plant development

Sci Bull (Beijing). 2023 Sep 30;68(18):2077-2093. doi: 10.1016/j.scib.2023.08.017. Epub 2023 Aug 9.

Authors

Li Qu¹, Moyang Liu¹, Lingli Zheng¹, Xu Wang¹, Hongwei Xue²

Affiliations

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 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. Electronic address: hwxue@sjtu.edu.cn.

PMID: 37599176
DOI: 10.1016/j.scib.2023.08.017

Abstract

Casein kinase 1 (CK1) is serine/threonine protein kinase highly conserved among eukaryotes, and regulates multiple developmental and signaling events through phosphorylation of target proteins. Arabidopsis early flowering 1 (EL1)-like (AELs) are plant-specific CK1s with varied functions, but identification and validation of their substrates is a major bottleneck in elucidating their physiological roles. Here, we conducted a quantitative phosphoproteomic analysis in data-independent acquisition mode to systematically identify CK1 substrates. We extracted proteins from seedlings overexpressing individual AEL genes (AEL1/2/3/4-OE) or lacking AEL function (all ael single mutants and two triple mutants) to identify the high-confidence phosphopeptides with significantly altered abundance compared to wild-type Col-0. Among these, we selected 3985 phosphopeptides with higher abundance in AEL-OE lines or lower abundance in ael mutants compared with Col-0 as AEL-upregulated phosphopeptides, and defined 1032 phosphoproteins. Eight CK1s substrate motifs were enriched among AEL-upregulated phosphopeptides and verified, which allowed us to predict additional candidate substrates and functions of CK1s. We functionally characterized a newly identified substrate C3H17, a CCCH-type zinc finger transcription factor, through biochemical and genetic analyses, revealing a role for AEL-promoted C3H17 protein stability and transactivation activity in regulating embryogenesis. As CK1s are highly conserved across eukaryotes, we searched the rice, mouse, and human protein databases using newly identified CK1 substrate motifs, yielding many more candidate substrates than currently known, largely expanding our understanding of the common and distinct functions exerted by CK1s in Arabidopsis and humans, facilitating future mechanistic studies of CK1-mediated phosphorylation in different species.

Keywords: Arabidopsis EL1-like (AEL); C3H17; Casein kinase 1 (CK1); Data-independent acquisition (DIA); Embryo development; Phosphoproteomics.

MeSH terms

Animals
Arabidopsis Proteins* / genetics
Arabidopsis* / genetics
Casein Kinase I / genetics
Humans
Mice
Phosphopeptides / chemistry
Plant Development / genetics

Substances

Arabidopsis Proteins
Casein Kinase I
Phosphopeptides