Characterization of Subcellular Dynamics of Sterol Methyltransferases Clarifies Defective Cell Division in smt2 smt3, a C-24 Ethyl Sterol-Deficient Mutant of Arabidopsis

Author:

Ohta Daisaku12ORCID,Fuwa Ayaka2,Yamaroku Yuka2,Isobe Kazuki12,Nakamoto Masatoshi2,Okazawa Atsushi12ORCID,Ogawa Takumi12ORCID,Ebine Kazuo34ORCID,Ueda Takashi34ORCID,Mercier Pierre5,Schaller Hubert5ORCID

Affiliation:

1. Graduate School of Agriculture, Osaka Metropolitan University, 1-1 Gakuen-cho, Sakai 599-8531, Japan

2. Graduate School of Life and Environmental Sciences, Osaka Prefecture University, 1-1 Gakuen-cho, Sakai 599-8531, Japan

3. National Institute for Basic Biology, Nishigonaka 38, Myodaiji, Okazaki 444-8585, Japan

4. The Graduate Institute for Advanced Studies, SOKENDAI, Nishigonaka 38, Myodaiji, Okazaki 444-8585, Japan

5. Institute de Biologie Moléculaire des Plantes, CNRS, 12, Rue du Général Zimmer, F-67084 Strasbourg, France

Abstract

An Arabidopsis sterol mutant, smt2 smt3, defective in sterolmethyltransferase2 (SMT2), exhibits severe growth abnormalities. The loss of C-24 ethyl sterols, maintaining the biosynthesis of C-24 methyl sterols and brassinosteroids, suggests specific roles of C-24 ethyl sterols. We characterized the subcellular localizations of fluorescent protein-fused sterol biosynthetic enzymes, such as SMT2-GFP, and found these enzymes in the endoplasmic reticulum during interphase and identified their movement to the division plane during cytokinesis. The mobilization of endoplasmic reticulum-localized SMT2-GFP was independent of the polarized transport of cytokinetic vesicles to the division plane. In smt2 smt3, SMT2-GFP moved to the abnormal division plane, and unclear cell plate ends were surrounded by hazy structures from SMT2-GFP fluorescent signals and unincorporated cellulose debris. Unusual cortical microtubule organization and impaired cytoskeletal function accompanied the failure to determine the cortical division site and division plane formation. These results indicated that both endoplasmic reticulum membrane remodeling and cytokinetic vesicle transport during cytokinesis were impaired, resulting in the defects of cell wall generation. The cell wall integrity was compromised in the daughter cells, preventing the correct determination of the subsequent cell division site. We discuss the possible roles of C-24 ethyl sterols in the interaction between the cytoskeletal network and the plasma membrane.

Funder

JSPS (the Japan Society for the Promotion of Science) KAKENHI Grant-in-Aid for Scientific Research

JSPS Bilateral Joint Research Projects

Basic Research Program of Osaka Prefecture University

University of Strasbourg (EXPLOratory Research Project INOPHYT

CNRS

National Institute of Basic Research Japan

Publisher

MDPI AG

Reference72 articles.

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3. Phytosterols and their derivatives: Structural diversity, distribution, metabolism, analysis, and health-promoting uses;Moreau;Prog. Lipid Res.,2018

4. Darnet, S., and Schaller, H. (2019). Metabolism and biological activities of 4-methyl-sterols. Molecules, 24.

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