Cholesterol activates BK channels by increasing KCNMB1 protein levels in the plasmalemma.

J Biol Chem

Department of Pharmacology, Addiction Science, and Toxicology, College of Medicine, The University of Tennessee Health Science Center, Memphis, Tennessee, USA. Electronic address:

Published: August 2021

AI Article Synopsis

  • Calcium-/voltage-gated, large-conductance potassium channels (BKs) play a vital role in physiological functions like smooth muscle contraction, with high membrane cholesterol inhibiting their activity.
  • Research on rat cerebral artery myocytes revealed that while enriching membrane cholesterol (CLR) can initially activate BK channels, this effect requires a longer cellular process and is dependent on the presence of accessory KCNMB1 (β) subunits.
  • Blocking intracellular protein trafficking inhibited BK activation in the presence of elevated CLR, highlighting that the regulation of BK channels switches from inhibition to activation through a process that increases membrane KCNMB1 levels.

Article Abstract

Calcium-/voltage-gated, large-conductance potassium channels (BKs) control critical physiological processes, including smooth muscle contraction. Numerous observations concur that elevated membrane cholesterol (CLR) inhibits the activity of homomeric BKs consisting of channel-forming alpha subunits. In mammalian smooth muscle, however, native BKs include accessory KCNMB1 (β) subunits, which enable BK activation at physiological intracellular calcium. Here, we studied the effect of CLR enrichment on BK currents from rat cerebral artery myocytes. Using inside-out patches from middle cerebral artery (MCA) myocytes at [Ca]=30 μM, we detected BK activation in response to in vivo and in vitro CLR enrichment of myocytes. While a significant increase in myocyte CLR was achieved within 5 min of CLR in vitro loading, this brief CLR enrichment of membrane patches decreased BK currents, indicating that BK activation by CLR requires a protracted cellular process. Indeed, blocking intracellular protein trafficking with brefeldin A (BFA) not only prevented BK activation but led to channel inhibition upon CLR enrichment. Surface protein biotinylation followed by Western blotting showed that BFA blocked the increase in plasmalemmal KCNMB1 levels achieved via CLR enrichment. Moreover, CLR enrichment of arteries with naturally high KCNMB1 levels, such as basilar and coronary arteries, failed to activate BK currents. Finally, CLR enrichment failed to activate BK channels in MCA myocytes from KCNMB1 mouse while activation was detected in their wild-type (C57BL/6) counterparts. In conclusion, the switch in CLR regulation of BK from inhibition to activation is determined by a trafficking-dependent increase in membrane levels of KCNMB1 subunits.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7950327PMC
http://dx.doi.org/10.1016/j.jbc.2021.100381DOI Listing

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