Distinct protein kinase C isozymes mediates inhibitory effects of different G-protein coupled receptors on cardiac rapidly activating delayed rectifier K ~ current

Aim Evidence has shown that stimulation of alA-adrenorecetors receptor （alA-AR） or angiotensin II type 1 receptor （AT1R） acutely down-regulates the rapid component of the delayed rectifier K ＋ current （IKr） via protein kinase C （PKC）. This study was designed to investigate which PKC isozymes mediate down-regulations of IKr by alA-AR and AT1R. Method The whole-cell patch-clamp technique was used to record IKr in native cardio- myocytes and in human embryonic kidney （HEK） 293 cells co-transfected with human ether-a-go-go related gene （hERG） encoding α-subunit of IKr and human alA-AR or AT1R gene. Result In isolated guinea-pig ventricular cardiomyocytes the inhibitory action of Ang II on IKr was little affected by Go6976 （selectively inhibiting PKCα, β and γ） and Go6983 （selectively inhibiting PKCα, β, γ , δ, and ζ）, but was significantly antagonized by an inter- nal dialysis with PKCe-selective inhibitory peptide εV1 -2. In contrast, the inhibitory action of alA-AR agonist A61603 on IKr was remarkably attenuated by Go6976 or Go6983, but not affected by peptide εV1 -2. Moreover, specific PKC-selective inhibitory peptide antagonized the effect of A61603. The results suggested that PKCe and PKCα isoform respectively mediated the inhibitory effect of AT1R and a1A-AR. In heterologous expression system, both PKCα and e-selective activator peptides down regulated hERG current with different manner. PKCα activator peptide shifted the activation curve of the channel to the right, but PKCe-selective activator peptide did not. Simi- larly, A61603 shifted the activation curve to the right, whereas Ang Ⅱ had no effect. In addition, both A61603 and PKCα activator peptide showed inhibitory action on bERG A PKC current （an bERG mutant in which 17 of the 18 ROSITE-predicted PKC acceptor serines/threonines were changed to alanine） with a similar potency to wild type bERG current. But, both Ang Ⅱ and PKCe-selective activator peptide exhibited no effects on bERG △ PKC cur- rent. The results indicated that PKCα and PKCe isoforms down-regulated bERG current through different mecha- nism. Conclusion PKCα and PKCe isoform respectively mediates the inhibition on IKr by stimulation of AT1R and alA-AR via different molecular mechanism.

Effect of Interleukin-1β on I_A and I_K Currents in Cultured Murine Trigeminal Ganglion Neurons

To investigate the effect of intedeukin-1β （IL-1β） on IA and IK currents in cultured murine trigeminal ganglion （TG） neurons, whole-cell patch clamp technique was used to record the IA and IK currents before and after 20 ng/mL IL-1β perfusion. Our results showed that 20 ng/mL IL-1β inhibited IA currents （18.3±10.7）% （n=6, P〈0.05）. IL-1β at 20 ng/mL had no effect on G-V curve of IA but moved the H-infinity curve V0.5 from -36.6±6. 1 mV to-42.4±5.2 mV （n=5, P〈0.01）. However, 20 ng/mL IL-1β had effect on neither the amplitude nor the G-V curve of IK. IL-1β was found to selectively inhibit IA current in TG neurons and the effect may contribute to hyperalgesia under various inflammatory conditions.

苦参碱对缺血性心室肌细胞快速延迟整流钾电流的作用

目的观察苦参碱对病理条件下(缺血、酸中毒)单个心室肌细胞快速延迟整流钾电流(rapid component of delayed rectifier potassium current,IKr)的作用,初步探讨苦参碱治疗缺血性心律失常的作用机制。方法冠状动脉左前降支结扎建立家兔心肌梗死模型,应用全细胞膜片钳技术记录酶解法分离的心肌梗死模型家兔苦参碱灌胃1mon后右心室心肌细胞IKr的变化。在pH=7·4和pH=6·5的条件下,应用全细胞膜片钳技术记录苦参碱对酶解法分离的豚鼠心室肌细胞IKr的作用。结果在正常细胞外液(pH=7·4)的条件下苦参碱(50μmol·L-1)降低IKr,在刺激电压为+60mV时,IKr电流密度由(12·15±0·70)pA/pF降低至(9·22±0·65)pA/pF(n=8,P<0·05)。在细胞外液酸化(pH=6·5)的条件下苦参碱(50μmol·L-1)仍表现抑制IKr电流的作用,在刺激电压为+60mV时,IKr电流密度由(7·05±0·41)pA/pF降低至(5·76±0·28)pA/pF(n=8,P<0·05)。家兔冠状动脉结扎1mon后,在刺激电压为+60mV时,心肌梗死组家兔心室肌细胞IKr电流密度为(1·17±0·12)pA/pF较正常组(1·70±0·11)pA/pF降低(n=12,P<0·05)。苦参碱组(8mg·kg-1·d-1)家兔心室肌细胞IKr电流密度为(0·86±0·25)pA/pF较心梗组降低(n=12,P<0·05)。结论苦参碱阻断心室肌细胞IKr,可能是其延长有效不应期,降低异位节律的发生率,治疗心律失常的机制之一。苦参碱对酸化条件及长期心肌缺血后心室肌细胞IKr仍表现出明显的抑制作用,表明其对心肌梗死后心律失常有效。

苄基四氢巴马汀对豚鼠心室肌细胞快激活延迟整流钾电流的作用(英文)

目的 研究苄基四氢巴马汀 (BTHP)对心室肌细胞快激活 (Ikr)延迟整流钾电流的作用。方法用全细胞膜片钳技术记录豚鼠心室肌细胞钾离子通道电流。结果 BTHP在 1～ 10 0 μmol·L-1以浓度依赖性方式阻滞Ikr,其IC50 为 13 5 μmol·L-1(95 %可信范围 :11 2～ 15 8μmol·L-1)。 30 μmol·L-1BTHP可使Ikr及Ikr,tail分别降低 (31± 4 ) %和 (36± 5 ) % (n =6 ,P <0 0 1)。与多数III类抗心律失常药物不同 ,BTHP可频率依赖性地抑制Ikr。该药主要改变Ikr的失活过程 ,可使Ikr的失活时间常数 (τ)从 (2 38± 16 )ms降至 (196± 14 )ms ,而对Ikr的激活动力学影响不大。结论 BTHP对Ikr有明显的抑制作用 。

桂枝甘草汤对豚鼠心室肌细胞IKs及HEK293细胞IKr的影响

目的探讨桂枝甘草汤治疗心律失常的可能作用机制及配伍意义。方法30只SD大鼠随机分为桂枝组(桂枝单煎液120 mg/ml)、甘草组(甘草单煎液60 mg/ml)、桂枝甘草单煎液混合组(桂枝单煎液+甘草单煎液混合180 mg/ml)、桂枝甘草汤同煎液组(桂枝和甘草同煎液180 mg/ml)、对照组(生理盐水),每组6只。各组每天灌胃相应药物1 ml/100 g,3天后腔静脉取血制备含药血清。分离豚鼠心室肌细胞,设桂枝血清组、甘草血清组、桂枝甘草单煎液混合血清组、桂枝甘草汤同煎液血清组、对照血清组,每组5个复孔;各组以体积比分别加入10%和15%浓度含药血清,培养24 h后分别检测各组在0、20、30、40、50 mV条件下慢激活延迟整流钾电流(IKs)电流密度。HEK293细胞分组及干预方法同心室肌细胞,培养24 h后分别检测各组在0、20、30、40、50 mV条件下快激活延迟整流钾电流(IKr)尾电流密度及IKr尾电流动力学参数(包括激活半电压、斜率因子)。结果在10%浓度药物干预下,0、20、30、40、50 mV时各组IKs电流密度比较差异均无统计学意义(P>0.05),20、30、40、50 mV时各组IKr尾电流密度比较差异均无统计学意义(P>0.05)。在15%浓度药物干预下,与对照血清组比较,甘草血清组和桂枝甘草单煎液混合血清组各电压IKs电流密度均降低,桂枝血清组30、40、50 mV时IKs电流密度降低,桂枝甘草汤同煎液血清组50 mV时IKs电流密度降低(P<0.05);桂枝甘草汤同煎液血清组各电压IKr尾电流密度均降低,桂枝甘草单煎液混合血清组50 mV时IKr尾电流密度降低,甘草血清组0 mV时IKr尾电流密度升高(P<0.05)。在15%浓度药物干预下,与甘草血清组比较,桂枝甘草汤同煎液血清组30 mV时IKs电流密度升高,各电压IKr尾电流密度均降低(P<0.05);与桂枝血清组比较,桂枝甘草汤同煎液血清组30、40、50 mV时IKr尾电流密度降低(P<0.05)。与对照血清组比较,在10%药物浓度干预下,各组IKr尾电流激活半电压均减小(P<0.05);在15%药物浓度干预下,各组IKr尾电流激活半电压均减小(P<0.05),甘草血清组、桂枝血清组斜率因子减小(P<0.05)。结论桂枝甘草汤可在一定程度上抑制心室肌细胞IKs及HEK293细胞IKr,这可能是其治疗心律失常的作用机制之一,且方中桂枝和甘草配伍具有协同增效的作用。