The effects of calmodulin kinase Ⅱ inhibitor on hypertrophic cardiac myocytes
10.3760/cma.j.issn.1671-0282.2012.02.011
- VernacularTitle:钙调蛋白激酶Ⅱ抑制剂对肥厚心肌细胞的影响
- Author:
Jun KE
;
Feng CHEN
;
Xin XIAO
;
Musen DAI
;
Xiaoping WANG
;
Bin CHEN
;
Min CHEN
;
Cuntai ZHANG
- Publication Type:Journal Article
- Keywords:
Calmodulin kinase Ⅱ;
KN-93;
Cardiac hypertrophy;
Cardiac myocytes;
Electrophysiology;
L-type calcium current;
Intracellular calcium concentration([Ca2+]i);
Perforated patch recording techniques
- From:
Chinese Journal of Emergency Medicine
2012;21(2):151-155
- CountryChina
- Language:Chinese
-
Abstract:
Objective To investigate the effect of the calmodulin kinase Ⅱ Inhibitor KN-93 on L-typecalcium current(ICa,L)and intracellular calcium concentration([Ca2+]i)in hypertrophic cardiac myocytes.Methods Forty-eight female New Zealand white rabbits were randomized(random number)into four groups(12 animals in each group):the sham operation group(sham group),the left ventricular hypertrophy group(LVH group),the myocardial hypertrophy + KN-93 group(KN-93 group),and the myocardial hypertrophy + KN-92 group(KN-92 group).Myocardial hypertrophy in the rabbits was established by coarctation of the abdominal aorta.In the sham group,the abdominal aorta was dissociated without coarctation.Eight weeks after coarctation,single ventricular myocytes were isolated by enzymaticdissociation,and ICa,L was recorded using perforated-patch recording(PPR)techniques.[Ca2+]i was measured using single-cell calcium imaging with the fluorescence calcium indicator dye fura-2/AM.Results Cardiac hypertrophy was successfully established after 8 weeks of coarctation of the abdominal aorta.The peak ICa,L in the LVH group and the sham group was(1.38 ± 0.3)nA and(0.87 ± 0.1)nA at 0 mV,respectively(P <0.01,n =12).There was no significant difference in Ica,L density between the LVH group and the sham group[(6.7 ±1.0)pA/pF vs.(6.3±0.7)pA/pF; P≥0.05,n=12].The addition of either KN-92(0.5 μmol/L)or KN-93(0.5 μmol/L)to the perfusing solution caused a modest steady-state inhibition of peak ICaL(9.4% ±2.8%,KN-92; 10.5% ±3%,KN-93)(P≥0.05,n =12)at 0 mV.However,at a higher concentration(1 μmol/L),KN-93 more potently inhibited peak ICa,L(40%±4.9%)compared to KN-92(13.4% ± 3.7% ; P < 0.01,n =12).Resting[Ca2+]i levels in fura-2-loaded myocytes isolated from the sham,LVH,KN-92,and KN-93 groups were(98 ± 12.3)nmol/L,(154 ± 26.2)nmol/L,(147 ± 29.6)nmol/L,and(108 ± 21.2)nmol/L,respectively.Conclusions The CaMK Ⅱ specific inhibitor,KN-93,can effectively block ICa,L and reduce intracellular calcium overload in hypertrophic cardiac myocytes.This action may account for the antiarrhythmic effect of KN-93 in hypertrophic ventricular myocardium.
