CALCIUM REGULATION IN SINGLE AIRWAY SMOOTH MUSCLE CELLS
Project Number5R01HL054143-06
Contact PI/Project LeaderMADISON, JOHN MARK
Awardee OrganizationUNIV OF MASSACHUSETTS MED SCH WORCESTER
Description
Abstract Text
DESCRIPTION: (adapted from abstract) Contraction of airway smooth muscle
cause airway obstruction, and relaxation of this muscle is the principal
action of B-adrenergic agonists used to treat asthma. Calcium, both
extracellular and that released from intracellular stores, is an important
second messenger that contributes to the determination of tension in smooth
muscle. However, a paradox underscores our limited understanding of how
cytosolic calcium concentrations ([Ca2+])i are regulated in airway smooth
muscle cells. First, studies have shown that B-adrenergic agonists and
muscarinic agonists both stimulated calcium influx and caused large
increases in basal [Ca2+]i, yet paradoxically, had different effects on
tension. To explain this, it is hypothesized that the cytosol is not
homogeneous with respect to calcium concentrations. Independent of
regulating the net flux of calcium that determines tension, muscarinic and
B-adrenergic agonists stimulate calcium influx pathways that are either
functionally or anatomically segregated at the periphery of the cell. These
segregated influx pathways maintain peripheral sarcoplasmic reticulum (SR)
calcium stores but are not major determinants of tension. Progress supports
this general hypothesis and, further, it appears that SR refilling may have
unique features in airway smooth muscle. Since SR calcium stores are
important for understanding smooth muscle responses to multiple stimulations
by contractile agonists as probably occurs in asthma, th aims of continuing
this study are to better understand SR refilling. The aims are: (1) in the
absence of agonist, determine how the sarcoplasmic reticulum (SR) refills
after being depleted of calcium; (2) determine whether protein tyrosine
kinases and the cytoskeleton support SR refilling: (3) characterize S
refilling during sustained muscarinic stimulation; (4) characterize SR
refilling in the presence of B-adrenergic agonists. To address these aims,
the principal method is radiometric imaging of [Ca2+]i in single, bovine
airway smooth muscle cells loaded with the calcium dye, fura-2.
No Sub Projects information available for 5R01HL054143-06
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