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The Journal of Neuroscience, January 1, 2002, 22(1):82-92

Identification and Characterization of Novel Human Cav2.2 (alpha 1B) Calcium Channel Variants Lacking the Synaptic Protein Interaction Site

Shuji Kaneko1, Conan B. Cooper4, Naoto Nishioka1, Hironobu Yamasaki1, Atsushi Suzuki1, Scott E. Jarvis4, Akinori Akaike2, Masamichi Satoh3, and Gerald W. Zamponi4

Departments of 1 Neuropharmacology, 2 Pharmacology, and 3 Molecular Pharmacology, Graduate School of Pharmaceutical Sciences, Kyoto University, Sakyo-ku, Kyoto 606-8501, Japan, and 4 Department of Physiology and Biophysics, University of Calgary, Calgary, T2N 4N1 Canada

The physical interaction between the presynaptic vesicle release complex and the large cytoplasmic region linking domains II and III of N-type (Cav2.2) calcium channel alpha 1B subunits is considered to be of fundamental importance for efficient neurotransmission. By PCR analysis of human brain cDNA libraries and IMR32 cell mRNA, we have isolated novel N-type channel variants, termed Cav2.2-Delta 1 and Delta 2, which lack large parts of the domain II-III linker region, including the synaptic protein interaction site. They appear to be widely expressed across the human CNS as indicated by RNase protection assays. When expressed in tsA-201 cells, both novel variants formed barium-permeable channels with voltage dependences and kinetics for activation that were similar to those observed with the full-length channel. All three channel types exhibited the hallmarks of prepulse facilitation, which interestingly occurred independently of G-protein beta gamma subunits. By contrast, the voltage dependence of steady-state inactivation seen with both Delta 1 and Delta 2 channels was shifted toward more depolarized potentials, and recovery from inactivation of Delta 1 and Delta 2 channels occurred more rapidly than that of the full-length channel. Moreover, the Delta 1 channel was dramatically less sensitive to both omega -conotoxin MVIIA and GVIA than either the Delta 2 variant or the full-length construct. Finally, the domain II-III linker region of neither variant was able to effectively bind syntaxin in vitro. These results suggest that the structure of the II-III linker region is an important determinant of N-type channel function and pharmacology. The lack of syntaxin binding hints at a unique physiological function of these channels.

Key words: human brain; class B calcium channel; alternative splicing; synprint site; omega -conotoxins; syntaxin; Gbeta gamma

Copyright © 2002 Society for Neuroscience  0270-6474/02/22182-11$05.00/0


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