Large conductance Ca2+-activated K+ channels (BKCa, channels), provide feedback control for a number Ca2+-dependent physiological processes. In some tissues these channels may be composed simply of four a subunits surrounding a central pore. In smooth muscle, however, the BKCa channel's Ca2+ sensitivity is greatly enhanced and its kinetic behavior is altered by an auxiliary subunit known as beta1. These effects are essential for the channel to function properly in smooth muscle. Despite the BKCa channel's physiological importance and the powerful modulatory effects of beta1, until recently very little was known about the mechanism by which beta1 alters channel behavior. By performing experiments proposed in the original submission of this application, however, we have gone some distance addressing this issue. Specifically, we have found that despite beta1's large effects on Ca2+ sensitivity, beta1 appears to alter Ca2+ binding very little. Instead, other aspects of gating are altered by beta1, aspects that indirectly influence Ca2+ sensitivity through altering the voltage-dependent mechanism of channel gating. Having come to this understanding, under Specific Aim 1 of the present application we propose to examine quantitatively how beta1 alters BKCa voltage-dependent gating so as to gain further insight into the biophysical mechanism behind beta1's ability to enhance Ca2+ sensitivity.
In Specific Aim 2 we then turn our attention to beta1's molecular mechanism, addressing the question: what regions of beta1 make functionally important interactions with the BKCa a subunit? We view these experiments as an important step toward elucidating the molecular interactions involved in B-mediated BKCa channel regulation. We also propose in Specific Aim 3 experiments to determine whether different types of BKCa beta subunits (four beta subunits have now been identified beta1, beta2, beta3, beta4) can associate with a single channel and, as well, to examine the properties of BKCa channels coupled to differing numbers of beta1 subunits. This will allow us to test the hypothesis that variation in subunit stoichiometry contributes to the functional heterogeneity of BKCa channels in native tissues. Information for the proposed experiments will advance our understanding of the relationship between BKCa channel structure and function and as well the regulation of these channels in vivo. It may also form the basis for the development of therapeutic agents that modulate BKCa channel gating.

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL064831-03
Application #
6607295
Study Section
Special Emphasis Panel (ZRG1-MDCN-3 (01))
Program Officer
Wang, Lan-Hsiang
Project Start
2001-09-01
Project End
2005-06-30
Budget Start
2003-07-01
Budget End
2004-06-30
Support Year
3
Fiscal Year
2003
Total Cost
$237,000
Indirect Cost
Name
Tufts University
Department
Type
DUNS #
079532263
City
Boston
State
MA
Country
United States
Zip Code
02111
Kim, Hyun-Ju; Lim, Hyun-Ho; Rho, Seong-Hwan et al. (2008) Modulation of the conductance-voltage relationship of the BK Ca channel by mutations at the putative flexible interface between two RCK domains. Biophys J 94:446-56
Isacson, Christina Kaldany; Lu, Qing; Karas, Richard H et al. (2007) RACK1 is a BKCa channel binding protein. Am J Physiol Cell Physiol 292:C1459-66
Bao, Lin; Cox, Daniel H (2005) Gating and ionic currents reveal how the BKCa channel's Ca2+ sensitivity is enhanced by its beta1 subunit. J Gen Physiol 126:393-412
Bao, Lin; Kaldany, Christina; Holmstrand, Ericka C et al. (2004) Mapping the BKCa channel's ""Ca2+ bowl"": side-chains essential for Ca2+ sensing. J Gen Physiol 123:475-89
Dwir, Oren; Solomon, Ariel; Mangan, Shmuel et al. (2003) Avidity enhancement of L-selectin bonds by flow: shear-promoted rotation of leukocytes turn labile bonds into functional tethers. J Cell Biol 163:649-59
Bao, Lin; Rapin, Anne M; Holmstrand, Ericka C et al. (2002) Elimination of the BK(Ca) channel's high-affinity Ca(2+) sensitivity. J Gen Physiol 120:173-89