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Calcium-supported calpain degradation rates for cardiac myofibrils in diabetes
Authors:Angelo N Belcastro  James S Gilchrist  Jennifer A Scrubb  Gavin Arthur
Institution:(1) Laboratory of Cell Physiology and Exercise, Division of Human Kinetics, University of British Columbia, 6081 University Blvd., V6T 1Z1 Vancouver, British Columbia, Canada
Abstract:Objective The purpose was to investigate the calcium required for calpain-mediated degradation of selected cardiac myofibril proteins modified by diabetes, sulfhydryl (SH) and hydrophobic reagents.Methods: After 20 weeks of streptozotocin-induced (55 mg·kg–1) diabetes, calcium sensitive calpain (1.5 U·ml–1) degradation rates of purified cardiac myofibrillar proteins (1 mg·ml–1) were measured,in vitro, and compared to degradation rates for N-ethylmaleimide (NEM) and 2-ptoluidinylnapthalene-6-sulfonate (TNS) treated samples.Results: Diabetes (blood glucose of 550±32 mg·dl–1) reduced the yield of purified myofibrillar protein with minimal change in fibril protein composition. Total SH group reactivities (nmol·mg–130min) were 220±21, 163±17 and 156±24 for control, diabetic and NEM-treated (0.5mM) myofibrils (ple0.05). Calpain degradation rates were faster for all diabetic and SH modified myofibrillar proteins (ple0.05), with a 45 and 35% reduction in the pCa50 for a 37 kDa protein of diabetic and NEM-treated fibril complexes. For control myofibrils, both 100 and 200 uM TNS, reduced calpain degradation rates to a similar extent for all substrate proteins. In contrast, diabetic and NEM-treated samples showed a further reduction in calpain degradation rates with increasing TNS from 100 to 200 divi.Conclusion Our results support the hypothesis that in diabetes the calcium requirements for calpain degradation rates are reduced and dependent upon sulfhydryl group status and Ca2+-induced hydrophobic interactions, implicating a 37 kDa myofbillar-complexed protein.
Keywords:diabetic cardiomyopathy  proteolysis  calcium binding proteins  myofibrillar complexes  troponin
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