Effects of Tiaomaiyin and Its Disassembled Prescription on Expression of L-type Calcium Channel β2 Subunit in Rat Model of Tachyarrhythmia

[Objectives] To study the effects of Tiaomaiyin and its disassembled prescription on expression of L-type calcium channel β2 subunit in rat model of tachyarrhythmia. [Methods] Sixty Wistar rats were randomly divided into model group,Tiaomaiyin prescription group( whole prescription group),main efficacy group of removing heat to cool blood( blood cooling group),and auxiliary drug efficacy group of benefiting qi and nourishing heart( qi benefiting group),auxiliary efficacy group of promoting flow of qi and blood circulation( qi flow promoting group),and amiodarone group( western medicine group). Aconitine was given 7 d after the intragastric administration of the corresponding drugs,and the time of occurrence of arrhythmia in each group was observed. The left ventricular myocardium was subjected to reverse transcription-polymerase chain reaction and Western blotting. [Results] The ventricular premature beats( VPB) time in the whole prescription group and western medicine group was significantly longer than that in the model group. Ventricular tachycardia( VT),ventricular fibrillation( VF),and cardiac arrest( CA) were longer in the whole prescription group,blood cooling group,and western medicine group. The mRNA and protein expression of L-type calcium channel β2 subunit in the whole prescription group,blood cooling group and western medicine group were significantly decreased. [Conclusions] Tiaomaiyin whole prescription group and blood cooling group can reduce the occurrence time of tachyarrhythmia and reduce the expression of LTCC β2 in myocardium.

Antiepileptic Drug-Induced Apoptosis Was Prevented by L-Type Calcium Channel Activator in Cultured Rat Cortical Cells

Experimental data have shown that antiepileptic drugs cause neurodegeneration in developing rats. Valproate (VPA) is the drug of choice in primary generalized epilepsies, and carbamazepine (CBZ) is one of the most prescribed drugs in partial seizures. These drugs block sodium channels, thereby reducing sustained repetitive neuronal firing. The intracellular mechanisms whereby AEDs induce neuronal cell death are unclear. We examined whether AEDs induce apoptotic cell death in cultured cortical cells and whether calcium ions are involved in the AED-induced cell death. VPA and CBZ increased apoptotic cell death and induced morphological changes that were characterized by cell shrinkage and nuclear condensation or fragmentation. Incubation of cortical cultures with VPA or CBZ decreased phospho-Akt levels. CBZ decreased the intracellular calcium levels. On the other hand, FPL64176, an L-type calcium channel activator, increased the intracellular calcium levels and prevented the AED-induced apoptosis. Glycogen synthase kinase-3 inhibitors, such as alsterpaullone and azakenpaullone, prevented the AED-induced apoptosis. These results suggest that intracellular calcium level changes are associated with AEDs and apoptosis and that the activation of glycogen synthase kinase-3 is involved in the death of rat cortical neurons.

Hydrogen sulfide-induced enhancement of gastric fundus smooth muscle tone is mediated by voltagedependent potassium and calcium channels in mice

AIM:To investigate the effect of hydrogen sulfide(H2S)on smooth muscle motility in the gastric fundus.METHODS:The expression of cystathionineβ-synthase(CBS)and cystathionineγ-lyase(CSE)in cultured smooth muscle cells from the gastric fundus was examined by the immunocytochemistry technique.The tension of the gastric fundus smooth muscle was recorded by an isometric force transducer under the condition of isometric contraction with each end of the smooth muscle strip tied with a silk thread.Intracellular recording was used to identify whether hydrogen sulfide affects the resting membrane potential of the gastric fundus in vitro.Cells were freshly separated from the gastric fundus of mice using a variety of enzyme digestion methods and whole-cell patch-clamp technique was used to find the effects of hydrogen sulfide on voltage-dependent potassium channel and calcium channel.Calcium imaging with fura-3AM loading was used to investigate the mechanism by which hydrogen sulfide regulates gastric fundus motility in cultured smooth muscle cells.RESULTS:We found that both CBS and CSE were expressed in the cul tured smooth muscle cel ls from the gastric fundus and that H2S increased the smooth muscle tension of the gastric fundus in mice at low concentrations.In addition,nicardipine and aminooxyacetic acid(AOAA),a CBS inhibitor,reduced the tension,whereas Nω-nitro-L-arginine methyl ester,a nonspecific nitric oxide synthase,increased the tension.The AOAA-induced relaxation was significantly recovered by H2S,and the Na HS-induced increase in tonic contraction was blocked by 5 mmol/L4-aminopyridine and 1μmol/L nicardipine.Na HS significantly depolarized the membrane potential and inhibited the voltage-dependent potassium currents.Moreover,Na HS increased L-type Ca2+currents and caused an elevation in intracellular calcium([Ca2+]i).CONCLUSION:These findings suggest that H2S may be an excitatory modulator in the gastric fundus in mice.The excitatory effect is mediated by voltagedependent potassium and L-type calcium channels.

微小RNA-26b-5p对缺血性心律失常大鼠心房肌细胞L型钙通道的影响

目的探讨微小RNA(miR)-26b-5p对磷脂酰肌醇3-激酶(PI3K)/磷脂酰肌醇3,4,5-三磷酸(PIP3)信号通路的调控作用以及对缺血性心律失常大鼠心房肌细胞L型钙通道的影响。方法选择SD大鼠72只,按照随机数表法分为假手术组、模型组、LY294002组、阴性对照组、过表达组、联合组,每组12只。各组给予相应干预24h,除假手术组外的其余各组大鼠建立缺血性心律失常模型,假手术组大鼠仅开胸不结扎。建模过程中检测各组大鼠心律失常指标,采用Curtis-Walker评分法进行心律失常评分;荧光定量PCR法检测心房肌细胞中miR-26b-5p表达;全细胞膜片钳技术记录心房肌细胞L型钙通道电流(ICa-L);蛋白印迹法检测L型钙通道α1C亚基(CACNA1C)、钙调蛋白及PI3K/PIP3通路相关蛋白表达。结果与模型组比较,LY294002组大鼠左心室室性期前收缩次数、室性心动过速持续时间、心室颤动持续时间、心律失常评分、心房肌细胞ICa-L峰值密度绝对值、CACNA1C、钙调蛋白表达显著升高,磷酸化PI3K、PIP3、磷酸化蛋白激酶B(Akt)表达显著降低,过表达组大鼠左心室室性期前收缩次数、室性心动过速持续时间、心室颤动持续时间、心律失常评分、心房肌细胞ICa-L峰值密度绝对值、CACNA1C、钙调蛋白表达显著降低,miR-26b-5p、磷酸化PI3K、PIP3、磷酸化Akt表达显著升高(P<0.05)。与过表达组比较,联合组大鼠左心室室性期前收缩次数、室性心动过速持续时间、心室颤动持续时间、心律失常评分、心房肌细胞ICa-L峰值密度绝对值、CACNA1C、钙调蛋白表达显著升高,磷酸化PI3K、PIP3、磷酸化Akt表达显著降低(0.82±0.08vs1.09±0.11,0.91±0.09vs1.17±0.11,0.94±0.09vs1.20±0.12,P<0.05)。结论miR-26b-5p过表达可能通过激活PI3K/PIP3相关信号通路,阻滞缺血性心律失常大鼠心房肌细胞L型钙通道,改善心律失常表现。

Effect of gingerol on colonic motility via inhibition of calcium channel currents in rats

AIM: To investigate the effect of gingerol on colonic motility and the action of L-type calcium channel currents in this process.METHODS: The distal colon was cut along the mesenteric border and cleaned with Ca^(2+)-free physiological saline solution. Muscle strips were removed and placed in Ca^(2+)-free physiological saline solution, which was oxygenated continuously. Longitudinal smooth muscle samples were prepared by cutting along the muscle strips and were then placed in a chamber. Mechanical contractile activities of isolated colonic segments in rats were recorded by a 4-channel physiograph. Colon smooth muscle cells were dissociated by enzymatic digestion. L-type calcium currents were recorded using the conventional whole-cell patch-clamp technique.RESULTS: Gingerol inhibited the spontaneous contraction of colonic longitudinal smooth muscle in a dose-dependent manner with inhibition percentages of 13.3% ± 4.1%, 43.4% ± 3.9%, 78.2% ± 3.6% and 80.5% ± 4.5% at 25 μmol/L, 50 μmol/L, 75 μmol/L and 100 μmol/L, respectively(P < 0.01). Nifedipine, an L-type calcium channel blocker, diminished the inhibition of colonic motility by gingerol. Gingerol inhibited L-type calcium channel currents in colonic longitudinal myocytes of rats. At a 75 μmol/L concentration of gingerol, the percentage of gingerolinduced inhibition was diminished by nifedipine from 77.1% ± 4.2% to 42.6% ± 3.6%(P < 0.01). Gingerol suppressed IBa in a dose-dependent manner, and the inhibition rates were 22.7% ± 2.38%, 35.77% ± 3.14%, 49.78% ± 3.48% and 53.78% ± 4.16% of control at 0 m V, respectively, at concentrations of 25 μmol/L, 50 μmol/L, 75 μmol/L and 100 μmol/L(P < 0.01). The steady-state activation curve was shifted to the right by treatment with gingerol. The value of half activation was-14.23 ± 1.12 m V in the control group and-10.56 ± 1.04 m V in the 75 μmol/L group(P < 0.05) with slope factors, Ks, of 7.16 ± 0.84 and 7.02 ± 0.93(P < 0.05) in the control and 75 μmol/L groups, respectively. However, the steady-state inactivation curve was not changed, with a half-inactivation voltage, 0.5 V, of-27.43 ± 1.26 m V in the control group and-26.56 ± 1.53 m V in the 75 μmol/L gingerol group(P > 0.05), and a slope factor, K, of 13.24 ± 1.62 in the control group and 13.45 ± 1.68(P > 0.05) in the 75 μmol/L gingerol group.CONCLUSION: Gingerol inhibits colonic motility by preventing Ca^(2+) influx through L-type calcium channels.

Comparative identification of Ca～(2+) channel expression in INS-1 and rat pancreatic β cells

AIM:To identify and compare the profile of Ca2+ channel subunit expression in INS-1 and rat pancreatic β cells. METHODS:The rat insulin-secreting INS-1 cell line was cultured in RPMI-1640 with Wistar rats employed as islet donors.Ca2+ channel subunit expression in INS-1 and isolated rat β cells were examined by reverse transcription polymerase chain reaction (RT-PCR).Absolute real-time quantitative PCR was performed in a Bio-Rad iQ5 Gradient Real Time PCR system and the data analyzed using an iQ5 system to identify the expression level of the Ca 2+ channel subunits. RESULTS:In INS-1 cells,the L-type Ca 2+ channel 1C subunit had the highest expression level and the TPRM2 subunit had the second highest expression. In rat β cells,the TPRC4 β subunit expression was dominant and the expression of the L-type 1C subunit exceeded the 1D subunit expression about two-fold. This result agreed with other studies,confirming the important role of the L-type 1C subunit in insulinsecreting cells,and suggested that non-voltageoperated Ca 2+ channels may have an important role in biphasic insulin secretion. CONCLUSION:Twelve major Ca 2+ channel subunit types were identified in INS-1 and rat β cells and significant differences were observed in the expression of certain subunits between these cells.

lncRNA KCNQ1OT1调控miR-384/CACNA1C轴对心肌细胞增殖、凋亡的影响

目的探讨长链非编码RNA钾电压门控通道亚家族Q成员1反向转录物1(lncRNA KCNQ1OT1)调控miR-384/L型钙离子通道α1C亚基基因(CACNA1C)轴对心肌细胞增殖、凋亡的影响。方法实时荧光定量PCR(qRT-PCR)、Western blot分别检测正常培养的大鼠心肌H9c2、CP-R073细胞及缺氧/复氧(H/R)诱导的H9c2、CP-R073细胞中的KCNQ1OT1、miR-384、CACNA1C蛋白表达。将H9c2细胞分为Ct组、Model组、si-NC组、si-KCNQ1OT1组、mimic NC组、miR-384 mimic组、si-KCNQ1OT1+inhibitor NC组、si-KCNQ1OT1+miR-384 inhibitor组。除Ct组外,其他组H9c2细胞均需转染对应物质后构建H/R损伤模型。qRT-PCR检测细胞中KCNQ1OT1、miR-384表达;CCK-8法、EdU染色检测细胞增殖;流式细胞术检测细胞凋亡;ELISA法检测细胞中肌红蛋白(Mb)、肌钙蛋白-Ⅰ(cTnⅠ)水平;Western blot检测CACNA1C、增殖细胞核抗原(PCNA)、半胱氨酰天冬氨酸特异性蛋白酶-3(Caspase-3)、Bcl-2相关X蛋白(Bax)蛋白表达;双荧光素酶报告基因实验验证KCNQ1OT1与miR-384、miR-384与CACNA1C的关系。结果H/R诱导的H9c2、CP-R073细胞中KCNQ1OT1、CACNA1C蛋白表达升高,miR-384表达降低,且H/R诱导的H9c2细胞中KCNQ1OT1、CACNA1C蛋白表达最高,miR-384表达最低,因此,后续选择H9c2细胞为研究对象。与Ct组比较,Model组细胞中KCNQ1OT1、细胞凋亡率、Mb、cTnⅠ水平、CACNA1C、Caspase-3、Bax蛋白表达升高,miR-384表达、D 450值、EdU阳性率、PCNA蛋白表达降低(P<0.05);沉默KCNQ1OT1或过表达miR-384可促进H/R诱导的H9c2细胞增殖,抑制细胞凋亡;miR-384 inhibitor减弱了沉默KCNQ1OT1对H/R诱导的H9c2细胞增殖的促进作用,以及对细胞凋亡的抑制作用;KCNQ1OT1靶向调控miR-384/CACNA1C轴。结论沉默KCNQ1OT1可能通过上调miR-384来抑制CACNA1C表达,进而促进H/R诱导的H9c2细胞增殖,抑制细胞凋亡。

大果木姜子油调控miR-328基因抗心律失常H9c2细胞的机制研究

目的:探讨大果木姜子油通过调控miR-328基因抗心律失常H9c2细胞的可能机制。方法:慢病毒转染构建miR-328过表达H9c2细胞株,再运用生物机能实验系统构建H9c2细胞和miR-328过表达H9c2细胞心律失常模型。将H9c2细胞分为正常对照组、模型组、大果木姜子油组、miR-328过表达组和miR-328过表达+大果木姜子油组。根据分组条件培养结束后,qPCR检测H9c2细胞中miR-328相对表达量;ELISA检测炎性因子IL-1β、IL-6、TGF-β含量;比色法检测SOD活性和MDA浓度;DCFH荧光探针检测ROS水平;流式细胞术检测细胞凋亡率;Western Blot检测H9c2细胞L型钙通道相关蛋白表达。结果:成功构建H9c2细胞和miR-328过表达H9c2细胞心律失常模型。与正常对照组比较,模型组和miR-328过表达组细胞TGF-β、SOD活性及CaM、CaMKⅡ、p-CaMKⅡ蛋白表达显著降低,细胞凋亡率、miR-328及CaV1.2蛋白表达和IL-1β、IL-6、MDA、ROS水平显著升高(P<0.01)。经大果木姜子油干预后,心律失常模型细胞形态改善,上述指标均被显著逆转(P<0.01)。结论:大果木姜子油可改善心律失常H9c2细胞,其作用机制可能与调控miR-328基因降低炎症因子水平、调节氧化应激、抑制细胞凋亡及调节L型钙通道相关蛋白表达有关。

Calcium channels and iron uptake into the heart

Iron overload can lead to iron deposits in many tissues,particularly in the heart.It has also been shown to be associated with elevated oxidative stress in tissues.Elevated cardiac iron deposits can lead to iron overload cardiomyopathy,a condition which provokes mortality due to heart failure in iron-overloaded patients.Currently,the mechanism of iron uptake into cardiomyocytes is still not clearly understood.Growing evidence suggests L-type Ca2+channels(LTCCs)as a possible pathway for ferrous iron(Fe2+)uptake into cardiomyocytes under iron overload conditions.Nevertheless,controversy still exists since some findings on pharmacological interventions and those using different cell types do not support LTCC’s role as a portal for iron uptake in cardiac cells.Recently,T-type Ca2+channels (TTCC)have been shown to play an important role in the diseased heart.Although TTCC and iron uptake in cardiomyocytes has not been investigated greatly,a recent finding indicated that TTCC could be an important portal in thalassemic hearts.In this review,comprehensive findings collected from previous studies as well as a discussion of the controversy regarding iron uptake mechanisms into cardiomyocytes via calcium channels are presented with the hope that understanding the cellular iron uptake mechanism in cardiomyocytes will lead to improved treatment and prevention strategies,particularly in iron-overloaded patients.

人参皂苷单体Rb_1对缺血心室肌细胞动作电位及L-型钙离子通道的影响

目的:观察人参皂苷单体Rb1对豚鼠缺血心室肌细胞动作电位(AP)和L-型钙离子通道的影响。方法:Langendorff离体心脏逆向灌流法分离豚鼠心室肌细胞,随机选取心室肌细胞分为正常对照组、缺血组及Rb1100、200和400μmol.L-13个剂量组。应用全细胞电流钳模式记录心室肌细胞动作电位,应用电压钳模式记录L-型钙离子通道电流(Ica-L)。结果:Rb1100、200和400μmol.L-1组缺血心室肌细胞动作电位复极50%(APD50)和动作电位复极90%(APD90)明显低于给药前(P<0.05或P<0.001),缺血后的心室肌细胞L-型钙离子通道峰值电流明显低于给药前(P<0.05或P<0.01)。Rb1抑制缺血心室肌细胞钙离子通道的开放,随浓度增加钙电流显著降低,具有浓度依赖性。结论:Rb1缩短缺血心肌细胞AP时程和抑制钙通道的作用,可能是其抗心肌缺血的机制之一。

17β-雌二醇对豚鼠心室肌细胞L型钙电流的抑制作用

目的观察17β-雌二醇对豚鼠心室肌细胞L型钙电流的影响及其与雌激素受体(estrogen receptor,ER)的关系。方法酶机械法分离豚鼠单个心室肌细胞;膜片钳全细胞模式观察17β-雌二醇对单个心室肌细胞L型钙电流(ICa-L)的影响,并通过加入雌激素受体阻断剂tamoxifen(TAM)研究该作用与雌激素受体的关系。结果 17β-雌二醇(10-9～10-7mol.L-1)使ICa-L峰电流密度值从(-3.5±0.6)pA.pF-1分别减少至(-2.4±0.3)pA.pF-1、(-1.9±0.3)pA.pF-1和(-1.1±0.3)pA.pF-1(与对照组比较,均为P<0.01,n=5)。TAM(10-7 mol.L-1)预处理后,17β-雌二醇(10-7mol.L-1)使ICa-L峰电流密度值从(-3.5±0.6)pA.pF-1减少到(-1.0±0.2)pA.pF-1(与对照组比较,P<0.01,n=5),与未应用TAM(10-7 mol.L-1)预处理时比较,ICa-L峰电流密度值无变化(P>0.05,n=5)。结论 17β-雌二醇抑制豚鼠心室肌细胞ICa-L的作用呈浓度依赖性,雌激素受体阻断剂TAM不能阻断17β-雌二醇对豚鼠心室肌细胞ICa-L的抑制作用,提示17β-雌二醇对ICa-L的抑制作用可能与ER作用无关。

盐酸关附甲素对大鼠心室肌细胞膜L型钙通道(J_(Ca-L))的影响

目的:研究盐酸关附甲素对正常大鼠心室肌细胞L型钙离子通道(I_(Ca-L))的影响。方法:应用膜片钳全细胞记录法,记录关附甲素对I_(Ca-L)的作用并对通道动力学进行初步评价。结果:关附甲素呈浓度依赖性阻滞I_(Ca-L),在25,125,250和1000μmol·L^(-1)时I_(Ca-L)峰值电流密度(去极化至0mV时)分别减少为用药前的81．76%, 77．54%,76．46%和64．77%(P＜0．05)。关附甲素使I_(Ca-L)的I-V曲线上移,但不改变其激活电位、峰值电位。关附甲素呈轻度使用依赖性阻滞I_(Ca-L),对I_(Ca-L)静息态有阻滞作用。关附甲素对I_(Ca-L)激活曲线无明显影响,但使I_(Ca-L)失活后再激活的恢复时间常数(τ)延长,有作用于I_(Ca-L)的失活态的可能。结论:因为关附甲素产生明显I_(Ca-L)阻滞的浓度远大于临床浓度,其对I_(Ca-L)的阻滞作用可能不是抗心律失常的主要作用机制。关附甲素呈浓度依赖性阻滞I_(Ca-L),其作用于L型钙通道的静息态,也有可能作用于失活态。

MicroRNA-1在心肌肥大中对L-型钙通道β_2亚基的负性调控作用

目的:研究微小RNA-1(microRNA-1,miR-1)在心肌细胞肥大中对L-型钙通道β2亚基(Cavβ2)的负性调控作用及机制。方法:应用异丙肾上腺素(ISO)诱导心肌细胞肥大;采用HJ2000通用图像分析系统测定心肌细胞表面积;应用数据库microCosm预测miR-1的靶基因;构建含Cavβ23’UTR报告基因质粒和miR-1瞬时共转染HEK293细胞,验证Cavβ2为miR-1靶基因;应用qRT-PCR或Western blot方法检测心房钠尿肽(ANP)、β-肌球蛋白重链(β-MHC)、miR-1和Cavβ2mRNA和蛋白表达水平;转染miR-1模拟物上调miR-1或应用Cavβ2RNAi干扰Cavβ2蛋白的表达,观察对心肌细胞肥大的影响。结果:①在ISO诱导的心肌细胞肥大中,miR-1表达显著下降;应用miR-1 mimic转染心肌细胞使miR-1表达上调,心肌细胞表面积、ANP和β-MHC mRNA表达均显著低于ISO组(P<0.05)。②网络数据库预测显示Cavβ2为miR-1的潜在靶点;将miR-1和含Cavβ23’UTR报告基因质粒共转染HEK293细胞,其萤光值显著降低(P<0.01)。转染miR-1 mimic使心肌细胞miR-1表达上调,可以明显抑制Cavβ2蛋白的表达。③在ISO诱导心肌细胞肥大中Cavβ2表达较对照组显著增加;应用RNAi技术下调Cavβ2表达可明显抑制心肌细胞表面积、ANP和β-MHC mRNA表达的增加。结论:预测并验证L-型钙通道β2亚基为miR-1的靶基因。miR-1可能通过抑制其靶基因Cavβ2蛋白的表达,降低细胞内钙离子浓度,抑制心肌细胞肥大。

血管紧张素Ⅱ对模拟缺血心室肌细胞L-型钙通道的影响

实验研究了血管紧张素Ⅱ (AngⅡ )对模拟缺血心室肌细胞L 型钙离子通道的作用。用胶原酶酶解法急性分离豚鼠心室肌细胞 ,以全细胞膜片钳方法记录心室肌细胞的L 型钙电流 (ICa L)。采用低氧、无糖、高乳酸和酸中毒综合方式模拟缺血液灌流 ,造成心室肌细胞的模拟缺血 ,并在缺血的基础上继续用含 10 0nmol/LAngⅡ灌流细胞 ,观察AngⅡ对模拟缺血心室肌细胞钙离子通道的影响。实验结果显示 :模拟缺血时ICa L峰值电流明显减小 ,最大激活电压为 0mV ;AngⅡ能抵抗模拟缺血对ICa L的抑制效应 ,使ICa L峰值电流增大 ,并使最大激活电压左移至 - 10mV。

三羟异黄酮对豚鼠心室肌细胞L-型钙通道电流的影响(英文)

本实验用全细胞膜片钳技术观察三羟异黄酮(genistein,GST)对豚鼠心室肌细胞L-钙通道电流(ICa、L)的影响。结果如下:(1)GST(10、50、100 μmol/L)可浓度依赖性地降低ICa,L(n=6,P<0.01)。GST的非活性结构类似物daidzein(100μmol/L),在同一浓度范围对ICa,L没有影响(n=5,P>0.05)。(2)GST使I-V曲线上移,但对ICa,L的电压依赖特征和最大激活电压无明显影响。(3)GST对ICa,L的激活动力学特性也无影响,但可使钙电流稳态失活曲线左移。V0.5从对照的-28.6±0.6 mV变为-32.8±1.1mV,κ值从对照的5.8±0.5 mV升至6.5±0.9 mV(n=6,P<0.05)。(4)GST明显使复活曲线右移,从而使ICa,L从失活状态下恢复明显减慢(n=7,P<0.01)。(5)酪氨酸磷酸酶抑制剂正钒酸钠(1 mmol/L)显著对抗GST引起的ICa,L抑制效应(n=6,P<0.01)。根据以上结果得出的结论是:GST抑制ICa,L加速钙通道失活和钙通道在失活状态下恢复减慢;GST对ICa,L的这种抑制作用与蛋白酪氨酸激酶(PTK)抑制有关。

肾上腺髓质素对豚鼠心室肌细胞L-型钙通道的调制(英文)

应用全细胞膜片钳技术研究了肾上腺髓质素 (ADM )对豚鼠心室肌细胞L 型钙电流 (ICa ,L)的影响及其信号传导机制。结果发现 :ADM ( 1～ 10 0nmol/L)浓度依赖性抑制ICa,L(P <0 0 5 ) ,并可被ADM特异受体阻断剂ADM2 2 52 ( 10 0nmol/L)完全阻断。用蛋白激酶A特异拮抗剂H 89( 10 μmol/L)预处理 ,对ADM抑制ICa ,L的作用无影响。但用蛋白激酶C (PKC)特异性拮抗剂PKC19 36 预处理 ,可完全阻断ADM的抑制效应 ;而PKC特异性激动剂PMA则可以模仿ADM的抑制效应 (P <0 0 5 )。上述结果提示 :ADM作用于特异性ADM受体可浓度依赖性地抑制豚鼠心室肌细胞ICa ,L,而此作用可能是PKC介导的。

丹酚酸B和延胡索乙素对大鼠心室肌细胞L-型钙通道的影响

目的观察单独及联合使用丹酚酸B和延胡索乙素对大鼠心室肌细胞L-型钙通道的影响。方法采用急性酶解分离法获得大鼠的单个心肌细胞,使用全细胞膜片钳技术记录钙通道电流。观察给药前后钙通道电流峰值(钙电流活化后峰值点与完全失活后电流轨迹的垂直距离)的变化。结果单独使用丹酚酸B(1,10,100μmol/L)对钙电流峰值的抑制率分别为:(25.3±16.4)%(n=4),(44.6±24.0)%(n=6),(86.0±20.4)%(n=4)。单独使用延胡索乙素(10,30,100μmol/L)对钙电流峰值的抑制率分别为:(22.2±6.4)%(n=5),(27.4±1.6)%(n=3),(51.0±23.0)%(n=9);联合使用丹酚酸B(1μmol/L)和延胡索乙素(10μmol/L)对钙通道电流峰值的抑制作用强于单独使用丹酚酸B(1μmol/L)或延胡索乙素(10μmol/L),差异有统计学意义(P<0.05);盐酸阿托品(14mmol/L)能够逆转延胡索乙素对L-型钙通道的抑制作用,而加强丹酚酸B的抑制作用。结论丹酚酸B和延胡索乙素对大鼠心室肌细胞L-型钙通道均有抑制作用,两者之间能够产生协同效应,并且这两种有效成分调控L-型钙通道的作用机制不同。

过氧化氢对大鼠心室肌细胞L-型钙通道电流的影响

目的:研究过氧化氢(H2O2)对单个大鼠心室肌细胞L-型钙通道电流(Ica,L)的影响。方法:用急性酶解法获得单个大鼠心室肌细胞;用标准的全细胞膜片钳技术记录钙通道电流,观察5mmol·L-1H2O2引起单个大鼠心室肌细胞Ica,L改变。结果:在5mmol·L-1H2O2作用下,大鼠心室肌细胞Ica,L峰值电流密度从4.89±0.52pA/pF增加至9.80±0.65pA/pF(P<0.05,n=10),电流-电压曲线下移,但激活电位、峰电位和翻转电位无明显改变;H2O2对Ica,L激活时间常数-电压曲线无明显影响,但可使其灭活时间常数-电压曲线明显向上移;H2O2对Ica,L稳态激活曲线无明显改变,但可使其稳态失活曲线明显左移,V0.5从(-26.85±5.3)mV左移至(-37.20±4.5)mV(P<0.05,n=5)。结论:H2O2可以增加大鼠心肌细胞Ica,L,且使其失活明显减慢。

应激对大鼠心室肌细胞L-型钙离子通道的影响

目的 :研究应激对心室肌细胞L 型钙离子通道电流及激活、失活门控动力学特性的影响。方法 :制备离体心室肌细胞并用去甲肾上腺素 (NE)诱导建立应激心肌细胞模型 ,应用流式细胞术 (FCM )和Fura 2荧光分光光度法测定应激心室肌细胞的凋亡率和心肌细胞内游离钙浓度变化。利用膜片钳全细胞钳制记录法记录应激心室肌细胞L 型钙离子通道电流I V曲线图及稳态激活、失活曲线图。结果 :FCM检测发现 1 0 - 4mol/L的NE模拟应激可导致心室肌细胞凋亡率明显上升 ,对照组 :0 .36 % ,应激组 :2 .1 7% (P <0 .0 1 )。 1 0 - 4mol/L的NE干预使Ica L峰电流幅值显著性上升 ,激活曲线分析发现应激后曲线明显左移 ,半数最大激活膜电位 (V1 /2 )为 (- 1 4 .59± 0 .2 4 )mV ,较之于对照组 :(- 0 .69± 0 .36)mV ,差异显著 ,而稳态失活曲线特性未发生有意义的改变。实验组心肌细胞内游离钙浓度较对照组升高 1 6 .7%。结论 :应激可导致L 型钙离子通道电流增加 ,通道更易于激活 ,通道的这种异常活动可能导致钙超载 ,从而引起心肌细胞凋亡 。

大鼠骨髓间充质干细胞L-型钙通道的表达及电流检测

目的 探讨L-型钙通道基因和蛋白在骨髓间充质干细胞（MSCs）中的表达及离子电流，以进一步研究其在MSCs增殖和分化中的作用。方法 分离、培养和纯化大鼠骨髓间充质干细胞，细胞免疫荧光化学方法检测表面分子CD14、CD29、CD34，CD44、CD45、CD106的阳性率和L-型钙通道蛋白的表达；采用RT-PCR技术观察MSCs细胞中钙离子通道不同亚基α1C、α1D、α1G、α1H、α1S mRNA的表达；全细胞膜片钳技术记录单个细胞离子电流。结果 细胞免疫荧光化学方法检测CD29、CD44、CD106阳性率在93％左右，CD14、CD34、CD45表达阴性。RT-PCR结果显示，可见L-型钙通道α1C亚基的mRNA高表达；但未见L-型钙通道α1D、α1S亚基和T-型钙通道的α1G、α1H亚基mRNA的表达。L-型钙通道蛋白（α1C）呈阳性表达。在36例细胞中16例细胞记录到电压依赖性内向电流。此电流激活电位-30mV，最大激活电位为0-10mV，可被nifedipine（10μmol／L）阻断，细胞外液中以10mmol／L Ba^2＋作为负载离子，记录的电流强度明显大于2mmol／L Ca^2＋时，证实为L-型钙电流。结论 MSCs不仅有L-型钙通道的基因和蛋白的表达，并且具有功能电流。