ENDOTHELIN INCREASES MYOFILAMENT CA2+ SENSITIVITY IN ALPHA-TOXIN PERMEABILIZED RABBIT MESENTERIC-ARTERY

被引:102
作者
NISHIMURA, J
MORELAND, S
AHN, HY
KAWASE, T
MORELAND, RS
VANBREEMEN, C
机构
[1] GRAD HOSP PHILADELPHIA, BOCKUS RES INST, 415 S 19TH ST, PHILADELPHIA, PA 19146 USA
[2] UNIV MIAMI, SCH MED, DEPT MOLEC & CELLULAR PHARMACOL, MIAMI, FL 33152 USA
[3] BRISTOL MYERS SQUIBB PHARMACEUT RES INST, PRINCETON, NJ USA
关键词
MYOSIN LIGHT CHAIN PHOSPHORYLATION; CROSSBRIDGE CYCLING; MYOFILAMENT CA2+ SENSITIVITY; PROTEIN KINASE-C; ENDOTHELIN; VASCULAR SMOOTH MUSCLE;
D O I
10.1161/01.RES.71.4.951
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
This study was designed to investigate the mechanism of endothelin-1 (ET-1) contractions in Staphylococcus alpha-toxin-permeabilized vascular smooth muscle. Rabbit small mesenteric arteries permeabilized with alpha-toxin were mounted for isometric or isotonic force recording or were processed for determination of myosin light chain (MLC) phosphorylation levels. Addition of 100 nM ET-1 plus 10-mu-M GTP significantly enhanced myofilament Ca2+ sensitivity as compared with the addition of Ca2+ alone (EC50, 0.47-mu-M Ca2+ for Ca2+ alone and 0.13-mu-M Ca2+ for ET-1 plus GTP). This enhanced sensitivity was reversed by GDP-beta-S. ET-1-induced contractions were relaxed at a constant [Ca2+] by the addition of 30-mu-M cAMP or cGMP, demonstrating a direct effect of the cyclic nucleotides on contractile regulation. Inhibition of protein kinase C activity by 100 nM staurosporine relaxed ET-1 plus GTP-induced contractions, and pretreatment with 40-mu-M chelerythrine inhibited the ET-1 plus GTP increase in force. At 0.32-mu-M Ca2+, steady-state levels of shortening velocity were not increased by ET-1 plus GTP, although steady-state levels of MLC phosphorylation were significantly enhanced. The ET-1-induced increase in MLC phosphorylation was not altered by changes in [Ca2+], whereas the shortening velocity was Ca2+ dependent, suggesting that the increase MLC phosphorylation level may be the result of protein kinase C, rather than MLC kinase, activation. These results are consistent with the hypothesis that ET-1 increases myofilament Ca2+ sensitivity by a G protein-dependent pathway and subsequent activation of protein kinase C. We propose that protein kinase C increases myofilament Ca2+ sensitivity during ET-1 stimulation either by phosphorylation of a thin-filament regulatory protein or by downregulation of the MLC phosphatase.
引用
收藏
页码:951 / 959
页数:9
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