Effects of Calmodulin-dependent Protein Kinase Ⅱ Inhibitor,KN-93,on Electrophysiological Features of Rabbit Hypertrophic Cardiac Myocytes

Cardiac hypertrophy is an independent risk factor for sudden cardiac death in clinical settings and the incidence of sudden cardiac death and ventricular arrhythmias are closely related.The aim of this study was to determine the effects of the calmodulin-dependent protein kinase(CaMK) Ⅱ inhibitor,KN-93,on L-type calcium current(I Ca,L) and early after-depolarizations(EADs) in hypertrophic cardiomyocytes.A rabbit model of myocardial hypertrophy was constructed through abdominal aortic coarctation(LVH group).The control group(sham group) received a sham operation,in which the abdominal aortic was dissected but not coarcted.Eight weeks later,the degree of left ventricular hypertrophy(LVH) was evaluated using echocardiography.Individual cardiomyocyte was isolated through collagenase digestion.Action potentials(APs) and I Ca,L were recorded using the perforated patch clamp technique.APs were recorded under current clamp conditions and I Ca,L was recorded under voltage clamp conditions.The incidence of EADs and I ca,L in the hypertrophic cardiomyocytes were observed under the conditions of low potassium(2 mmol/L),low magnesium(0.25 mmol/L) Tyrode’s solution perfusion,and slow frequency(0.25-0.5 Hz) electrical stimulation.The incidence of EADs and I ca,L in the hypertrophic cardiomyocytes were also evaluated after treatment with different concentrations of KN-92(KN-92 group) and KN-93(KN-93 group).Eight weeks later,the model was successfully established.Under the conditions of low potassium,low magnesium Tyrode’s solution perfusion,and slow frequency electrical stimulation,the incidence of EADs was 0/12,11/12,10/12,and 5/12 in sham group,LVH group,KN-92 group(0.5 μmol/L),and KN-93 group(0.5 μmol/L),respectively.When the drug concentration was increased to 1 μmol/L in KN-92 group and KN-93 group,the incidence of EADs was 10/12 and 2/12,respectively.At 0 mV,the current density was 6.7±1.0 and 6.3±0.7 PA·PF-1 in LVH group and sham group,respectively(P>0.05,n=12).When the drug concentration was 0.5 μmol/L in KN-92 and KN-93 groups,the peak I Ca,L at 0 mV was decreased by(9.4±2.8)% and(10.5±3.0)% in the hypertrophic cardiomyocytes of the two groups,respectively(P>0.05,n=12).When the drug concentration was increased to 1 μmol/L,the peak I Ca,L values were lowered by(13.4±3.7)% and(40±4.9)%,respectively(P<0.01,n=12).KN-93,a specific inhibitor of CaMKII,can effectively inhibit the occurrence of EADs in hypertrophic cardiomyocytes partially by suppressing I Ca,L,which may be the main action mechanism of KN-93 antagonizing the occurrence of ventricular arrhythmias in hypertrophic myocardium.

MicroRNA-219 alleviates glutamate-induced neurotoxicity in cultured hippocampal neurons by targeting calmodulin-dependent protein kinase Ⅱ gamma

Septic encephalopathy is a frequent complication of sepsis,but there are few studies examining the role of micro RNAs（mi Rs） in its pathogenesis.In this study,a mi R-219 mimic was transfected into rat hippocampal neurons to model mi R-219 overexpression.A protective effect of mi R-219 was observed for glutamate-induced neurotoxicity of rat hippocampal neurons,and an underlying mechanism involving calmodulin-dependent protein kinase II γ（Ca MKIIγ） was demonstrated.mi R-219 and Ca MKIIγ m RNA expression induced by glutamate in hippocampal neurons was determined by quantitative real-time reverse transcription-polymerase chain reaction（q RT-PCR）.After neurons were transfected with mi R-219 mimic,effects on cell viability and apoptosis were measured by 3-（4,5-dimethylthiazolyl-2）-2,5-diphenyltetrazolium bromide（MTT） assay and flow cytometry.In addition,a luciferase reporter gene system was used to confirm Ca MKIIγ as a target gene of mi R-219.Western blot assay and rescue experiments were also utilized to detect Ca MKIIγ expression and further verify that mi R-219 in hippocampal neurons exerted its effect through regulation of Ca MKIIγ.MTT assay and q RT-PCR results revealed obvious decreases in cell viability and mi R-219 expression after glutamate stimulation,while Ca MKIIγ m RNA expression was increased.MTT,flow cytometry,and caspase-3 activity assays showed that mi R-219 overexpression could elevate glutamate-induced cell viability,and reduce cell apoptosis and caspase-3 activity.Moreover,luciferase Ca MKIIγ-reporter activity was remarkably decreased by co-transfection with mi R-219 mimic,and the results of a rescue experiment showed that Ca MKIIγ overexpression could reverse the biological effects of mi R-219.Collectively,these findings verify that mi R-219 expression was decreased in glutamate-induced neurons,Ca MKIIγ was a target gene of mi R-219,and mi R-219 alleviated glutamate-induced neuronal excitotoxicity by negatively controlling Ca MKIIγ expression.

Amelioration of mitochondrial dysfunction in heart failure through S-sulfhydration of Ca^2＋/calmodulin-dependent protein kinase Ⅱ

OBJECTIVE To determine the functional role of hydrogen sulfide(H_2S) in protecting against mitochondrial dysfunction in heart failure through the inhibition of Ca^(2+)/calmodulin-dependent protein kinaseⅡ(Ca MKⅡ) using wild type and CSE knockout mouse models.METHODS Continuous subcutaneous injection isoprenaline(7.5 mg·kg^(-1) per day),once a day for 4 weeks to induce heart failure in male C57BL/6(6-8 weeks old) mice and CSE-/-mice.150 μmol·L^(-1) H_2O_2 was used to induce oxidative stress in H9c2 cells.Echocardiograph was used to detect cardiac parameters.H&E stain and Masson stain was to observation histopathological changes.Western blot was used to detect protein expression and activity.The si RNA was used to silence protein expression.HPLC was used to detect H_2S level.Biotin assay was used to detect the level of S-sulfhydration protein.RESULTS Treatment with S-propyl-L-cysteine(SPRC) or sodium hydrosulfide(Na HS),modulators of blood H_2S levels,attenuated the development of heart failure in animals,reduced lipid peroxidation,and preserved mitochondrial function.The inhibition Ca MKⅡ phosphorylation by SPRC and Na HS as demonstrated using both in vivo and in vitro models corresponded with the cardioprotective effects of these compounds.Interestingly,Ca MKⅡ activity was found to be elevated in CSE-/-mice as compared to wild type animals and the phosphorylation status of Ca MK Ⅱ appeared to relate to the severity of heart failure.Importantly,in wild type mice SPRC was found to promote S-sulfhydration of Ca MKⅡ leading to reduced activity of this protein however,in CSE-/-mice S-sulfhydration was abolished following SPRC treatment.CONCLUSION A novel mechanism depicting a role of S-sulfhydration in the regulation of Ca MKⅡ is presented.SPRC mediated S-sulfhydration of Ca MKⅡ was found to inhibit Ca MKⅡ activity and to preserve cardiovascular homeostasis.

慢性铝暴露对大鼠海马神经元PKC、CaMKⅡ、Ng的影响

通过研究慢性铝暴露对大鼠学习记忆和海马长时程增强(long-term potentiation,LTP)的影响,并检测海马神经元蛋白激酶C(protein kinasec,PKC)活性及Ca2+-钙调蛋白激酶Ⅱ(Ca2+-calmodulin dependent protein kinaseⅡ,CaMKⅡ)和神经颗粒素(neurogranin,Ng)蛋白表达的变化,探讨铝暴露损害学习记忆的作用机制.选用断乳后Wistar大鼠,以含有不同浓度AlCl3的蒸馏水进行饲养.3个月后,测定铝暴露组大鼠脑内和血中的铝含量;测量记录大鼠海马群体峰电位(population spike,PS)LTP;用改良Takai法测定海马神经元PKC活性变化;Western印迹法检测CaMKⅡ和Ng的蛋白表达.结果显示,与对照组相比,铝暴露组的PKC活性降低,差异有统计学意义(P<0·01);与对照组相比,铝暴露组的CaMⅡ蛋白表达降低,差异有统计学意义(P<0·05);与对照组相比,铝暴露组的Ng蛋白表达降低,且差异有统计学意义(P<0·05).实验结果说明:慢性铝暴露可以降低大鼠海马神经元PKC的活性及Ng和CaMKⅡ的蛋白表达,可能影响Ng磷酸化水平,从而影响CaM与Ng之间的亲和性,也影响Ca2+-CaM对CaMKⅡ的调节,抑制LTP的形成,损害学习记忆的功能.

鞘内注射硫酸镁和吗啡对切口痛大鼠脊髓背角p-αCaMK Ⅱ表达的影响

目的观察鞘内注射(it)硫酸镁(MgSO4)和吗啡对切口痛大鼠脊髓背角磷酸化钙—钙调蛋白依赖性蛋白激酶Ⅱα(p-αCaMKⅡ)表达的影响。方法所有大鼠术前8d鞘内置管,用机械缩足反射阈值、热缩足潜伏期和累计疼痛评分来评价大鼠疼痛行为学变化;用免疫组织化学和Western blot法来测定吗啡和硫酸镁对大鼠脊髓背角p-αCaMKⅡ表达的影响。结果术前或术后30minit吗啡5μg或MgSO4188μg和吗啡2.5μg使术后2h的机械性缩爪阈值(MWT)和热刺激缩爪阈值(TWL)明显延长(P<0.01),累积疼痛评分明显降低(P<0.01);术前30minitMgSO4375μg或吗啡5μg或MgSO4188μg和吗啡2.5μg使大鼠术后2h脊髓背角p-αCaMKⅡ表达明显减少(P<0.05)。结论在大鼠切口痛模型中,it吗啡5μg或MgSO4188μg和吗啡2.5μg具有确切的抗伤害作用,其抗伤害作用可能与抑制脊髓背角p-αCaMKⅡ表达有关。

脊髓背角长时程增强中CaMKⅡ磷酸化水平的变化

目的探讨长时程增强诱导和维持过程中脊髓背角钙/钙调蛋白依赖性蛋白激酶Ⅱ(CaMKⅡ)磷酸化水平的变化。方法(1)细胞外记录脊髓腰膨大部背角浅层神经元C-纤维诱发电位;(2)免疫组化技术观察脊髓背角CaMKⅡ磷酸化水平的变化。结果(1)LTP30min、LTP3h脊髓背角CaMKⅡThr286的磷酸化水平明显高于对照组;(2)强直刺激前30min脊髓局部给予KN-93(CaMKⅡ选择性抑制剂,100μmol/L),LTP的诱导被完全阻断,CaMKⅡ磷酸化水平与对照组无明显差别;(3)强直刺激后30min给予KN-93,明显抑制LTP,CaMKⅡ的磷酸化水平也显著降低;(4)LTP3h后给予KN-93,LTP幅度和CaMKⅡ磷酸化水平与用药前相比,差异没有统计学意义。结论CaMKⅡ磷酸化可能在脊髓背角C-纤维诱发电位长时程增强诱导和早期维持中发挥重要作用。

Decorin Induces Cardiac Hypertrophy by Regulating the CaMKⅡ/MEF-2 Signaling Pathway In Vivo

Objective:Cardiac hypertrophy is an adaptive reaction of the heart against cardiac overloading,but continuous cardiac hypertrophy can lead to cardiac remodeling and heart failure.Cardiac hypertrophy is mostly considered reversible,and recent studies have indicated that decorin not only prevents cardiac fibrosis associated with hypertension,but also achieves therapeutic effects by blocking fibrosis-related signaling pathways.However,the mechanism of action of decorin remains unknown and unconfirmed.Methods:We determined the degree of myocardial hypertrophy by measuring the ratios of the heart weight/body weight and left ventricular weight/body weight,histological analysis and immunohistochemistry.Western blotting was performed to detect the expression levels of CaMKⅡ,p-CaMKⅡ and MEF-2 in the heart.Results:Our results confirmed that decorin can regulate the CaMKⅡ/MEF-2 signaling pathway,with inhibition thereof being similar to that of decorin in reducing cardiac hypertrophy.Conclusion:Taken together,the results of the present study showed that decorin induced cardiac hypertrophy by regulating the CaMKⅡ/MEF-2 signaling pathway in vivo,revealing a new therapeutic approach for the prevention of cardiac hypertrophy.

Ginsenoside Rb1 Pretreatment Attenuates Myocardial Ischemia by Reducing Calcium/Calmodulin-Dependent Protein Kinase Ⅱ-Medicated Calcium Release

Objective:The aim of this study was to investigate the protective effects of ginsenoside Rb1 and assess whether these protective effects are related to calcium/calmodulin-dependent protein kinaseⅡ(Ca MKⅡ).Methods:A myocardial ischemia(IS)rat.model and a myocardial H9 C2 cell hypoxia model were established.MI was induced by occluding the left anterior descending artery for 120 min.Ginsenoside Rb1(10 mg/kg)was administered 30 min before ischemia induction,and the treatment continued for 7 days.Results:In the rat IS injury model,ginsenoside Rb1 reduced myocardial infarct size,mean left ventricular diastolic pressure,incidence of arrhythmia,and levels of serum creatine kinase,lactate dehydrogenase,and malondialdehyde.However,the mean left ventricular systolic pressure,and maximal rising and falling rates of ventricular pressure(±dp/dtmax)increased.In the myocardial H9 C2 cell hypoxia model,ginsenoside Rb1 reduced intracellular calcium concentrations([Ca2+]i)during hypoxia,and markedly reversed the hypoxia-induced decrease in cell survival.Ginsenoside Rb1 was involved in the downregulation of CaMKⅡand the ryanodine receptor,as well as hypoxia-induced H9 C2 cell survival.Conclusion:The findings of the present study suggest that ginsenoside Rb1 attenuates MI injury in rats,partially through the downregulation of CaMKⅡexpression.

钙调蛋白依赖性蛋白激酶Ⅱ在小鼠卵母细胞减数分裂恢复中的作用

目的:探究钙调蛋白依赖性蛋白激酶Ⅱ(CaMK-Ⅱ)在小鼠卵母细胞减数分裂恢复中的作用。方法:构建卵丘卵母细胞复合物(COCs)体外培养模型,研究CaMK-Ⅱ特异抑制剂KN-93及AIP对EGF诱导的减数分裂恢复及卵丘扩展的影响,利用酶联免疫法检测胞内cGMP水平变化。结果:CaMK-Ⅱ抑制剂KN-93及AIP能够有效抑制EGF诱导的减数分裂恢复(P<0.05);KN-93能够抑制EGF诱导的卵丘扩展;KN-93及AIP降低COCs内cGMP的含量(P<0.05)。结论:EGF通过CaMK-Ⅱ诱导小鼠卵母细胞恢复减数分裂。

黄芩苷对扩张型心肌病大鼠心室重构、心室肌细胞凋亡及β1-AR/PKA/CaMKⅡ信号通路的影响

目的：探讨黄芩苷对阿霉素（ADR）诱导扩张型心肌病大鼠心室重构、心室肌细胞凋亡及β_1肾上腺素受体（β_1-AR）/蛋白激酶A（PKA）/钙调素依赖蛋白激酶Ⅱ（CaMKⅡ）信号通路的影响。方法：雄性Wistar大鼠60只,随机分为正常组、模型组、黄芩苷低、中、高剂量组及卡维地洛组;模型组给予ADR 2 mg·kg^（-1）腹腔注射,黄芩苷组及卡维地洛组在模型组基础上分别给予黄芩苷（25,50,100 mg·kg^（-1）·d^（-1））,卡维地洛10 mg·kg^（-1）·d^（-1）灌胃,正常组给予等体积0.9%NaCl腹腔注射,1次/周,共3次;7周末各组大鼠行心脏超声检测心室变化及心功能指标;酶联免疫吸附法（ELISA）检测各组大鼠血清氨基末端脑钠肽前体（N-terminal pro-brain natriuretic peptide,NT-pro BNP）,人基裂解素（human stromelysin-2,ST2）含量;采用原位末端转移酶标记法（TUNEL）染色观察各组大鼠心室肌细胞凋亡情况;蛋白免疫印迹法（Western blot）检测各组大鼠心室肌组织中β_1-AR,PKA及CaMKⅡ表达。结果：与正常组比较,模型组大鼠出现心室重构明显及心功能减弱（P〈0.05）,血清NT-proBNP,ST2含量增多（P〈0.05）,心室肌细胞凋亡数量增加（P〈0.05）,心室肌组织中β_1-AR,PKA及CaMKⅡ表达增多;与模型组比较,黄芩苷及卡维地洛组大鼠心室重构及心功能改善（P〈0.05）,血清NT-pro BNP,ST2含量降低（P〈0.05）,心室肌凋亡数量减少（P〈0.05）,心室肌组织中β_1-AR,PKA及CaMKⅡ表达减少（P〈0.05）。结论：黄芩苷可有效改善ADR诱导的扩张型心肌病大鼠心室重构,减少心肌细胞凋亡,其机制可能与抑制心室肌细胞β-AR/PKA/CaMKⅡ信号通路表达有关。

鞘内注射吗啡对切口痛大鼠脊髓背角p-αCaMK Ⅱ表达的影响

目的 研究鞘内注射（IT）吗啡对切口痛大鼠脊髓背角磷酸化钙-钙调蛋白依赖性蛋白激酶Ⅱ（p-αCaMKⅡ）表达的影响.方法 雄性SD大鼠32只,随机分为4组（n=8）,分别为假手术组（S组）、切口痛组（IP组）、术前吗啡组和术后吗啡组.按Yaksh法鞘内置管,按Brennan法制备大鼠足底切口痛模型,以von Frey细丝法和热辐射法测定机械缩足反射阈值（MWT）和热刺激缩足反射潜伏期（TWL）,观察大鼠术后2 h时的疼痛行为学变化,应用免疫组织化学和Western blot法观察脊髓背角p-αCaMK Ⅱ表达的变化.结果 与S组比较,IP组大鼠MWT明显降低（P＜0.01）,TWL明显缩短（P＜0.01）.脊髓背角p-αCaMKⅡ阳性神经元数量和蛋白表达明显增加（P＜0.01） 与IP组比较,术前吗啡组和术后吗啡组大鼠的MWT明显升高（P＜0.01）,TWL明显延长（P＜0.01）,术前吗啡组大鼠脊髓背角p-aCaMK Ⅱ阳性神经元数量和蛋白表达明显减少（P＜0.05或P＜0.01）.结论 在大鼠切口痛模型中,术前IT吗啡的抗伤害作用可能与抑制切口痛引起的脊髓背角P-aCaMK Ⅱ表达增加有关.

心力衰竭大鼠心肌β_3肾上腺素受体表达及其对钙离子相关调节蛋白的作用

目的研究心力衰竭(HF)大鼠心肌β3肾上腺素受体(beta3-adrenergic receptors,β3-AR)表达情况及对钙离子相关调节蛋白的作用。方法以正常大鼠作对照组,皮下注射生理盐水;实验组大鼠皮下注射异丙肾上腺素(Isoproterenol,ISO),常规饲养8w。造模成功后实验组随机分为3组,激动剂组给予尾静脉注射β3-AR激动剂BRL37344,抑制剂组给予尾静脉注射β3-AR抑制剂SR59230A,HF组给予生理盐水。用药8w后行心脏彩超、RT-PCR法检测心肌组织钙调蛋白(CaM)、钙调蛋白激酶Ⅱ(CaMKⅡ)、肌内质网Ca2+-ATP酶异构体2a(SERCA2a)的mRNA表达。结果①HF组较对照组β3-ARmRNA表达水平增高,CaM、CaMKⅡ、SERCA2amRNA表达水平减低(均P<0.05)。②与HF组相比较,激动剂组β3-ARmRNA水平表达增加,CaM、CaMKⅡ、SERCA2a表达进一步减少(均P<0.05)。③抑制剂组β3-ARmRNA表达水平较对照组减少,CaM、CaMKⅡ、SERCA2a较对照组减低,但较HF组增加(均P<0.05)。结论β3-AR激动剂减低衰竭心肌CaM、CaMKⅡ、SERCA2a的mRNA表达,导致心功恶化,β3-AR抑制剂则相反,可延缓HF进展,预示β3-AR抑制剂在药物治疗HF中的应用前景。

缺锌对大鼠脑肌醇磷脂信号转导系统的影响

目的 探讨缺锌对大鼠脑肌醇磷脂信号转导系统的影响。方法 2 4只 Wistar大鼠 ,雌雄各半 ,按体重随机分为 A(缺锌组 ) ,B(自由进食组 ) ,C(配对饲养组 )三组 ,每组 8只 ,实验期 40天 ,测定脑锌和血锌含量 ,并观察缺锌对大鼠脑组织内磷脂酶 C(PLC)活性 ,蛋白激酶 C(PKC)活性 ,钙调蛋白 (Ca M)含量 ,及钙依赖性蛋白激酶 (Ca MK )活性的影响。结果 A组大鼠血清和脑锌含量明显降低 ,同时 A组大鼠大脑皮层和海马中 PLC,PKC,Ca MK 活性亦明显低于 B组和 C组。A组大鼠脑组织 Ca M含量明显低于 B组 ,与 C组无显著性差异。

鞘内注射KN93对小鼠神经病理性疼痛的镇痛效应

目的探讨钙离子/钙调蛋白依赖蛋白激酶Ⅱ(CaMKⅡ)在神经病理性疼痛发病机制中的作用。方法雄性ICR小鼠32只,随机均分为四组:神经病理性疼痛(SNL)组,制作L5/6脊神经结扎(SNL)模型;SNL/KN92组,制作SNL模型,鞘内注射无药理活性的KN93的结构类似物KN9245nmol;SNL/KN93组,制作SNL模型,鞘内注射KN9345nmol;假手术(Sham)组,仅显露脊神经而不结扎。分别于SNL术前及术后2～5d每天测定小鼠的机械痛阈和热痛阈,SNL/KN92组与SNL/KN93组于术后5d痛阈测定前30min行鞘内给药。于最后一次痛阈测定毕处死小鼠,取腰段脊髓组织用Western blot检测pCaMKⅡα的表达水平。结果SNL可导致机械痛阈和热痛阈降低(P<0.05),脊髓组织pCaMKⅡα的表达增加(P<0.05);鞘内注射KN93可翻转SNL所致的上述改变(P<0.05),但KN92无此效应。结论CaMKⅡ参与了SNL诱导的神经病理性疼痛的维持,靶向于CaMKⅡ信号途径的治疗可为慢性疼痛治疗提供新的策略。

Changes of learning, memory and levels of CaMKII, CaM mRNA, CREB mRNA in the hippocampus of chronic multiple-stressed rats

Background The effect of chronic stress on cognitive functions has been one of the hot topic in neuroscience. But there has been much controversy over its mechanism. Such single stressor applied in the past could not simulate complicated living circumstances that people confronted with. The aim of this study was to investigate the effects of chronic multiple-stress on learning and memory as well as on the levels of calcium/calmodulin-dependent protein kinase Ⅱ（CaMKⅡ）, calmodulin （CAM） mRNA, and cAMP-response element binding protein （CREB） mRNA in the hippocampus of rats. Methods The rats were divided randomly into stressed and control groups. The stressed group was given chronic multiple-stress for 6 weeks to set up a chronic multiple-stressed model. The rats＇ performance of spatial learning and memory was tested using Morris Water Maze （MWM） and Y-maze. Meanwhile, the expressions of CAMKII, CAM mRNA and CREB mRNA of rats＇ hippocampus were detected by immunohistochemistry, Western blot and reverse transcription-polymerase chain reaction （RT-PCR）, respectively. In addition, the width of synaptic cleft and the thickness of post-synaptic densities （PSD） were observed in the hippocampal CA3 region of rats by electron microscopy. Results After exposure to chronic multiple-stress for 6 weeks, the ability of learning and memory of the stressed group was higher than that of the control group （P〈0.05, P〈0.01）. The width of synaptic cleft was smaller and the thickness of PSD was larger in the hippocampal CA3 region of the stressed group than in that of the control group （P〈0.01）. The CAMKII immunostaining of the stressed group was stronger than that of the control group in the stratum radiatum and oriens of the hippocampal CA1 and CA3, especially in the stratum oriens. Quantitative analysis indicated that the expression of CAMKII, CAM mRNA, and CREB mRNA in the hippocampus of the stressed group was higher than that of the control group （P〈0.05, P〈0.01）. Conclusions The capacity of learning and memory can be enhanced after chronic multiple-stress. The increased levels of CAMKⅡ, CAM mRNA, and CREB mRNA may contribute to the enhancing effect of chronic multiple-stress on learning and memory.

1,25二羟维生素D_3通过ERK5通路调节破骨细胞分化

[目的]探讨体外1,25二羟维生素D_3(1,25-(OH)_2-VitD_3)通过细胞外信号调节激酶5(extracellularregulated kinase 5,ERK5)信号通路在诱导破骨细胞分化中的作用。[方法]对骨髓来源巨噬细胞(bone marrow macrophages,BMMs)进行不同浓度(0,10^(-9),10^(-8),10^(-7)mol/L)1,25-(OH)_2-VitD_3孵育,明确1,25-(OH)_2-VitD_3能否激活ERK5信号通路,并筛选出合适浓度的1,25-(OH)_2-VitD_3激活ERK5。调配不同工作液,分为正常细胞对照组、XMD8-92组、1,25-(OH)_2-VitD_3组及1,25-(OH)_2-VitD_3+XMD8-92组,分别孵育BMMs细胞6 d。采用TRAP染色检测4组破骨细胞的分化水平;Western Blot分别检测p-ERK5、ERK5等蛋白水平变化;RT-PCR检测NFATc1、CAMKⅡmRNA相对表达量。[结果]10^(-8)mol/L的1,25-(OH)_2-VitD_3可显著激活ERK5磷酸化(P<0.05)并通过ERK5通路促进破骨细胞分化(P<0.01),但此效应可被ERK5高选择性抑制剂XMD8-92抑制(P<0.05)。ERK5激活可显著上调破骨细胞CAMKⅡ、NFATc1 mRNA的表达(P<0.01);而XMD8-92可显著抑制CAMKⅡm RNA的表达(P<0.01),但对NFATc1 mRNA无显著影响(P>0.05)。[结论]体外低浓度(10^(-8)mol/L)的1,25-(OH)_2-VitD_3通过激活ERK5信号通路促进破骨细胞分化,CAMKⅡ是破骨细胞中ERK5信号下游通路的重要靶点。

铅暴露大鼠海马区神经颗粒素表达与学习记忆关系研究

【目的】探讨铅接触大鼠脑组织海马区神经颗粒素表达及在学习记忆障碍中的作用。【方法】32只Wistar大鼠随机分为4组,每组8只,3个染铅组分别在饮用的蒸馏水中添加0.02%、0.10%、0.20%醋酸铅为低、中、高剂量染铅组,空白对照组饮用蒸馏水,连续45 d复制慢性铅中毒模型,对各组进行Morris水迷宫试验,麻醉后分别检测各组动物血铅、脑铅含量;RT-PCR检测海马区组织Ng mRNA、CaMKⅡmRNA表达;免疫组化方法检测P-CaMKⅡ表达,Western Blotting法检测Ng蛋白表达。【结果】1)与空白对照组比较,染铅各组血铅、脑铅含量均显著增高(P<0.01),高剂量组动物体重显著降低(P<0.05);2)Morris水迷宫结果显示,随染铅浓度增高,潜伏期显著延长(P<0.05);通过强化训练,各组动物均获得了一定的定位能力,但各染铅组动物潜伏期显著高于空白对照组(P<0.05);3)与空白对照组比较,各浓度染铅组Ng mRNA及CaMKⅡmRNA表达均显著降低(P<0.05);4)Ng的Western Blotting结果显示,与空白对照组比较,中、高剂量染铅组Ng蛋白表达均显著降低(P<0.01),低剂量组表达也下降,但没有显著差异;P-CaMKⅡ的免疫组化结果显示,与空白对照组比较,低、中、高剂量染铅组表达均显著降低(P<0.05或<0.01)。【结论】Ng作为突触后CaM结合蛋白和PKC的作用底物,参与介导了铅导致的的学习记忆障碍。

化瘀祛痰方对血管性痴呆的保护作用机制探讨

目的:研究化瘀祛痰方对血管性痴呆(VD)沙鼠的保护作用,并初步探讨其作用机制是否与钙离子-钙调素依赖性蛋白激酶Ⅱ(Ca MKⅡ)/环磷腺苷效应元件结合蛋白(CREB)/脑源性神经营养因子(BDNF)信号通路相关。方法:将健康沙鼠40只,随机分为假手术组,模型组,化瘀祛痰方低、中、高(5.35,10.7,21.4 g·kg^-1)剂量组,每组8只,模型组及化瘀祛痰三组参考Levine法对全部沙鼠进行侧颈总动脉结扎再灌注法造VD模型;假手术组则不封闭颈部动脉,其他操作同手术组。术后沙鼠给予相应药物灌胃2次/日,21 d后进行水迷宫实验考察沙鼠的空间学习记忆能力。蛋白免疫印迹法(Western blot)及免疫组化分别测定沙鼠脑组织海马体的磷酸化(p)-Ca MKⅡ/Ca MKⅡ,p-CREB/CREB,BDNF蛋白的表达。结果:与假手术组比较,模型组沙鼠的上台潜伏期和平台穿梭次数明显降低,p-CaMKⅡ/Ca MKⅡ,p-CREB/CREB,BDNF蛋白表达均明显降低(P<0.01);与模型组比较,化瘀祛痰方组沙鼠的上台潜伏期和平台穿梭次数明显升高,其中化瘀祛痰方中以高剂量组效果最为明显(P<0.01),化瘀祛痰方可以有效的保护CA1区锥体细胞,明显上调p-CaMKⅡ/Ca MKⅡ,p-CREB/CREB,BDNF蛋白的表达(P<0.01)。结论:化瘀祛痰方改善了血管性痴呆沙鼠的学习和记忆能力,作用机制可能与Ca MKⅡ/CREB/BDNF信号通路的激活相关。