| Type of Document |
Dissertation |
| Author |
Adebamiro, Adedotun
|
| Author's Email Address |
adast15@pitt.edu |
| URN |
etd-07272006-132858 |
| Title |
SERINE PROTEASE REGULATION OF THE EPITHELIAL SODIUM CHANNEL |
| Degree |
Doctor of Philosophy |
| Program |
Cell Biology and Molecular Physiology |
| School |
School of Medicine |
| Advisory Committee |
| Advisor Name |
Title |
| Daniel C. Devor |
Committee Chair |
| John P. Horn |
Committee Member |
| John P. Johnson |
Committee Member |
| Peter F. Drain |
Committee Member |
| Robert J. Bridges |
Committee Member |
|
| Keywords |
- serine protease
- aprotinin
- noise analysis
- epithelial sodium channel
- short-circuit current
- sodium transport
|
| Date of Defense |
2006-07-13 |
| Availability |
unrestricted |
Abstract
Na+ transport through epithelial cells mediated by the epithelial Na+ channel (ENaC) is important for maintaining body fluid Na+ homeostasis, alveolar fluid clearance and normal airway mucocilliary function. A large body of evidence shows significant correlation between serine protease activity, channel fragmentation and transepithelial movement of Na+. The extracellular protease dependent regulation may play an important role in epithelial cells where the channel activity is intended more for the control of the extracellular environment, such as in airway cells, than in the control of the internal fluid status of the organism. Presented here is evidence supporting the hypothesis that Na+ channels are inserted into the apical membrane as inactive precursors whereupon they are acted upon by membrane resident serine proteases resulting in active channels. The effects of the serine protease inhibitor, aprotinin, on ENaC single channel properties were studied using transepithelial fluctuation analysis in the A6 amphibian kidney epithelium. Aprotinin causes a potent specific time-dependent inhibition of Na+ transport. Analysis of blocker induced fluctuations in Na+ current (INa) showed linear rate-concentration plots with the same blocker on- and off-rates in control and aprotinin inhibited conditions. Verification of open-block kinetics allowed for the use of a pulse protocol method to study the same cells under different conditions as well as the reversibility of the aprotinin effect on single channel properties. It was shown that protease regulation of INa is mediated by increasing the number of active channels in the apical membrane. To test the hypothesis that residues on ENaC mediate protease dependent channel activation ENaC was subjected to site-directed mutagenesis and heterologously expressed in Fisher rat thyroid (FRT) model epithelial cells. Activation by exogenous proteases depended on the presence of substrate specific residues in ENaC which dictated the rates of activation and the steady-state current levels.
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| Filename |
Size |
Approximate Download Time
(Hours:Minutes:Seconds)
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56K Modem |
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adebamiroa_etd2006.pdf |
4.33 Mb |
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