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Tetrameric interaction of the ectoenzyme CD38 on the cell surface enables its catalytic and raft-association activities
Authors:Miki Hara-Yokoyama  Mutsuko Kukimoto-Niino  Kazue Terasawa  Satoru Harumiya  Katarzyna A Podyma-Inoue  Nobumasa Hino  Kensaku Sakamoto  Satsuki Itoh  Noritaka Hashii  Yoko Hiruta  Nana Kawasaki  Chiemi Mishima-Tsumagari  Yoko Kaitsu  Tomoko Matsumoto  Motoaki Wakiyama  Mikako Shirouzu  Takeshi Kasama  Hiroshi Takayanagi  Naoko Utsunomiya-Tate  Kiyoshi Takatsu  Toshiaki Katada  Yoshio Hirabayashi  Shigeyuki Yokoyama  Masaki Yanagishita
Institution:Section of Biochemistry, Tokyo Medical and Dental University, Tokyo 113-8549, Japan; The Global Center of Excellence (GCOE) Program, International Research Center for Molecular Sciences in Tooth and Bone Diseases, Tokyo Medical and Dental University, Tokyo 113-8549, Japan.
Abstract:The leukocyte cell-surface antigen CD38 is the major nicotinamide adenide dinucleotide glycohydrolase in mammals, and its ectoenzyme activity is involved in calcium mobilization. CD38 is also a raft-dependent signaling molecule. CD38 forms a tetramer on the cell surface, but the structural basis and the functional significance of tetramerization have remained unexplored. We identified the interfaces contributing to the homophilic interaction of mouse CD38 by site-specific crosslinking on the cell surface with an expanded genetic code, based on a crystallographic analysis. A combination of the three interfaces enables CD38 to tetramerize: one interface involving the juxtamembrane α-helix is responsible for the formation of the core dimer, which is further dimerized via the other two interfaces. This dimerization of dimers is required for the catalytic activity and the localization of CD38 in membrane rafts. The glycosylation prevents further self-association of the tetramer. Accordingly, the tetrameric interaction underlies the multifaceted actions of CD38.
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