Sites of proteolytic processing and noncovalent association of the distal C-terminal domain of CaV 1.1 channels in skeletal muscle

Joanne T. Hulme, Keiichi Konoki, Teddy W.C. Lin, Marina A. Gritsenko, David G. Camp, Diana J. Bigelow, William A. Catterall

研究成果: Article査読

83 被引用数 (Scopus)

抄録

In skeletal muscle cells, voltage-dependent potentiation of Ca2+ channel activity requires phosphorylation by cAMP-dependent protein kinase (PKA) anchored via an A-kinase anchoring protein (AKAP15), and the most rapid sites of phosphorylation are located in the C-terminal domain. Surprisingly, the site of interaction of the complex of PKA and AKAP15 with the α1-subunit of CaV1.1 channels lies in the distal C terminus, which is cleaved from the remainder of the channel by in vivo proteolytic processing. Here we report that the distal C terminus is noncovalently associated with the remainder of the channel via an interaction with a site in the proximal C-terminal domain when expressed as a separate protein in mammalian nonmuscle cells. Deletion mapping of the C terminus of the α1-subunit using the yeast two-hybrid assay revealed that a distal C-terminal peptide containing amino acids 1802-1841 specifically interacts with a region in the proximal C terminus containing amino acid residues 1556-1612. Analysis of the purified α1-subunit of CaV1-1 channels from skeletal muscle by saturation sequencing of the intracellular peptides by tandem mass spectrometry identified the site of proteolytic processing as alanine 1664. Our results support the conclusion that a noncovalently associated complex of the α1-subunit truncated at A1664 with the proteolytically cleaved distal C-terminal domain, AKAP15, and PKA is the primary physiological form of CaV1-1 channels in skeletal muscle cells.

本文言語English
ページ(範囲)5274-5279
ページ数6
ジャーナルProceedings of the National Academy of Sciences of the United States of America
102
14
DOI
出版ステータスPublished - 2005 4月 5
外部発表はい

ASJC Scopus subject areas

  • 一般

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