N-terminal Inactivation Domains of {beta} Subunits Are Protected from Trypsin Digestion by Binding within the Antechamber of BK Channels

doi:10.1085/jgp.200810079

Scientifica: Experts in Electrophysiology

Published online
doi:10.1085/jgp.200810079
The Journal of General Physiology, Vol. 133, No. 3, 263-282
The Rockefeller University Press, 0022-1295 $30.00
© Zhang et al.

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ARTICLE

N-terminal Inactivation Domains of β Subunits Are Protected from Trypsin Digestion by Binding within the Antechamber of BK Channels

Zhe Zhang, Xu-Hui Zeng, Xiao-Ming Xia, and Christopher J. Lingle

Department of Anesthesiology, Washington University School of Medicine, St. Louis, MO 63110

Correspondence to Christopher J. Lingle: clingle{at}morpheus.wustl.edu

N termini of auxiliary β subunits that produce inactivationof large-conductance Ca²⁺-activated K⁺ (BK) channels reach theirpore-blocking position by first passing through side portalsinto an antechamber separating the BK pore module and the largeC-terminal cytosolic domain. Previous work indicated that theβ2 subunit inactivation domain is protected from digestionby trypsin when bound in the inactivated conformation. Otherresults suggest that, even when channels are closed, an inactivationdomain can also be protected from digestion by trypsin whenbound within the antechamber. Here, we provide additional testsof this model and examine its applicability to other βsubunit N termini. First, we show that specific mutations inthe β2 inactivation segment can speed up digestion by trypsinunder closed-channel conditions, supporting the idea that theβ2 N terminus is protected by binding within the antechamber.Second, we show that cytosolic channel blockers distinguishbetween protection mediated by inactivation and protection underclosed-channel conditions, implicating two distinct sites ofprotection. Together, these results confirm the idea that β2N termini can occupy the BK channel antechamber by interactionat some site distinct from the BK central cavity. In contrast,the β3a N terminus is digested over 10-fold more quicklythan the β2 N terminus. Analysis of factors that contributeto differences in digestion rates suggests that binding of anN terminus within the antechamber constrains the trypsin accessibilityof digestible basic residues, even when such residues are positionedoutside the antechamber. Our analysis indicates that up to twoN termini may simultaneously be protected from digestion. Theseresults indicate that inactivation domains have sites of bindingin addition to those directly involved in inactivation.

Abbreviations used in this paper: bbTBA, N-(4-[benzoyl]benzyl)-N,N,N-tributylammoniumbromide; BK, large-conductance Ca²⁺-activated K⁺; TBA, tetrabutylammonium;TM1, transmembrane segment 1.

© 2009 Zhang et al.
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