IP3R2及RYR2介导Ca^(2+)信号在急性一氧化碳中毒迟发性脑病小鼠模型中的表达

背景:研究发现星形胶质细胞中Ca^(2+)的表达与认知功能密切相关,目前由1,4,5-三磷酸肌醇受体(Inositol 1,4,5-trisphosphate receptors,IP3Rs)2、兰尼碱受体(ryanodine receptors,RYRs)2受体及其调控的Ca^(2+)信号通路已经成为认知障碍相关疾病研究的热点。目的:研究急性一氧化碳中毒迟发性脑病动物模型中,海马组织内星形胶质细胞和IP3R2、RYR2介导的Ca^(2+)信号的表达情况,探索急性一氧化碳中毒迟发性脑病可能的发病机制。方法:Morris水迷宫实验筛选认知功能合格的C57BL小鼠随机分为对照组、实验组,实验组小鼠采用静态吸入一氧化碳建立急性一氧化碳中毒迟发性脑病模型,对照组小鼠吸入等量空气。造模后第21天,利用Morris水迷宫、苏木精-伊红染色、Western blot、免疫荧光双标法、Ca^(2+)荧光探针检测中毒小鼠行为学及神经元改变、星形胶质细胞特异性标记物胶质纤维酸性蛋白及IP3R2、RYR2受体、星形胶质细胞内Ca^(2+)浓度变化。结果与结论:①Morris水迷宫实验发现与对照组相比,实验组小鼠逃避潜伏期明显延长(P<0.05);②苏木精-伊红染色表明实验组小鼠海马锥体细胞数减少、细胞结构紊乱、细胞核碎裂伴溶解;③免疫荧光检测表明海马区IP3R2、RYR2分别和胶质纤维酸性蛋白存在共表达,且实验组海马区IP3R2、RYR2和胶质纤维酸性蛋白表达均上调(P<0.05);④Western blot检测显示实验组海马区IP3R2、RYR2及胶质纤维酸性蛋白的蛋白表达均增多(P<0.05);⑤Ca^(2+)荧光探针法检测表明实验组小鼠海马区星形胶质细胞内Ca^(2+)浓度明显升高(P<0.05);⑥结果说明,星形胶质细胞可能通过介导IP3R2、RYR2受体影响Ca^(2+)信号,进而使一氧化碳中毒的小鼠认知功能受损,最终导致急性一氧化碳中毒迟发性脑病发生。

IP3R1基因沉默对鸭子宫上皮细胞Ca^(2+)转运的调控效应研究

本研究旨在探究IP3R1基因沉默后对鸭子宫上皮细胞增殖、胞内Ca^(2+)浓度和离子转运相关基因的影响。构建IP3R1基因shRNA干扰载体,利用Fluo-3/AM钙离子荧光标记法检测鸭子宫上皮细胞内Ca^(2+)浓度,CCK-8法检测鸭子宫上皮细胞的增殖情况,利用RT-qPCR法检测10个离子转运相关基因和4个细胞增殖相关基因的表达量。结果显示:IP3R1基因沉默后,细胞内Ca^(2+)浓度极显著升高,10个离子转运相关基因的表达发生变化,细胞也呈现增殖状态,进而影响了细胞增殖相关基因的表达。本研究结果揭示鸭子宫上皮细胞内IP3R1基因表达下调会影响细胞内Ca^(2+)稳态,改变钙转运相关基因mRNA的表达水平,并促进细胞增殖。

IP3R2基因敲除小鼠的繁育及基因型鉴定

目的:繁殖并鉴定IP3R2基因敲除小鼠,为后续实验提供样本支持,同时验证PCR法对基因鉴定的适用性。方法:购买IP3R2杂合子小鼠15只,以1雄2雌的合笼方式进行繁殖。繁殖出的子代小鼠生长至6周时,剪子代鼠尾做基因提取及PCR扩增,琼脂糖凝胶电泳结果判定。取鉴定结果为IP3R2基因敲除纯合子小鼠和野生型小鼠脑组织进行Western印迹及免疫荧光双标法,验证脑组织中IP3R2蛋白的表达情况。结果:可成功繁育IP3R2基因敲除小鼠,子代小鼠中,IP3R2纯合率为23.3%。PCR扩增可成功鉴定子代小鼠的基因型。与野生小鼠比较,IP3R2基因敲除小鼠脑组织中IP3R2表达量显著降低,差异有统计学意义(P<0.05)。结论:该实验可成功繁殖并鉴定出IP3R2基因敲除小鼠,为后续实验提供大量样本,PCR技术可快速、准确地鉴定IP3R2基因型,为后续实验提供技术支持。

Knockdown of RCN1 contributes to the apoptosis of colorectal cancer via regulating IP3R1

Background:The incidence of colorectal cancer(CRC)has been increasing in recent years.Thus,the discovery of factors that can assist in alleviating CRC is urgently warranted.Methods:To identify a potential factor involved in the development of CRC,we screened the upregulated genes in tumor tissues through four datasets from an online database.The expression of reticulocalbin 1(RCN1),a Ca2+-binding protein,was upregulated in the four datasets.Based on loss-offunction experiments,the effect of RCN1 on cell viability was assessed by Cell Counting Kit-8(CCK-8)assay.The regulatory effect of RCN1 on apoptosis was evaluated through Annexin V-fluorescein 5-isothiocyanate(FITC)/propidium iodide(PI)staining assay and terminal deoxynucleotidyl transferase-mediated dUTP nick-end labeling(TUNEL)assay in RKO and SW480 cells.Activation of endoplasmic reticulum(ER)stress signaling pathways was confirmed by estimating the phosphorylation and expression of PRKR-like ER kinase(PERK),inositol-requiring kinase-1(IRE1),transcription factor 6(ACT6),and CCAAT/enhancer-binding protein-homologous protein(CHOP).The intracellular Ca2+homeostasis regulated by RCN1 was determined through the detection of Ca2+concentration and mitochondrial membrane potential(MMP)measurement.Moreover,whether inositol 1,4,5-trisphosphate receptor type 1(IP3R1)was involved in the regulation of RCN1 in CRC was verified through the depletion of IP3R1 in RKO cells.Results:Knockdown of RCN1 reduced cell viability and facilitated apoptosis in RKO and SW480 cells.Phosphorylation of PERK and IRE1,activation of ATF6,and upregulation of CHOP were induced by the absence of RCN1,suggesting that the unfolded protein response(UPR)was activated in CRC cells.The concentration of Ca2+in mitochondria was increased after RCN1 depletion,followed by reduction in the MMP and release of cytochrome c from mitochondria to the cytoplasm in RKO and SW480 cells.Moreover,it was demonstrated that IP3R1 mediates the effect of RCN1 on apoptosis induced by ER stress in CRC cells.The downregulation of IP3R1 restored the RCN1 loss-induced apoptosis and the increased Ca2+concentration.Conclusion:Taken together,our results confirmed that silencing of RCN1 disrupted intracellular Ca2+homeostasis and promoted cell apoptosis caused by TG-induced ER stress by regulating IP3R1 and activating the UPR signaling pathways.

腹部推拿对UC模型大鼠背根神经节PLC/IP3R/Ca2+信号通路及AKT、p-AKT蛋白表达的影响

目的:观察腹部推拿干预溃疡性结肠炎(UC)模型大鼠后,对大鼠背根神经节PLC/IP3R/Ca^(2+)信号通路及AKT、p-AKT蛋白表达的影响,从而探讨腹部推拿对溃疡性结肠炎内脏高敏感的作用机制。方法:将36只SPF级大鼠分成空白组、模型组、推拿组、美沙拉嗪组4组,除空白组自由饮用蒸馏水外,其余各组采用自由饮5%葡聚糖硫酸钠溶液(DSS)的方法制备大鼠UC模型。造模第2日起推拿组采用腹部推拿进行干预,美沙拉嗪组进行美沙拉嗪溶液进行灌胃,空白组、模型组仅俯卧位束缚固定于固定器中。干预15日后,采用邻-甲酚酞络合铜比色法检测背根神经节(DRG)细胞钙离子浓度;ELISA法检测DRG组织中磷脂酶C(PLC)、肌醇1,4,5-三磷酸(IP3)、肌醇1,4,5-三磷酸受体(IP3R)的表达,WesternBlot检测DRG组织中蛋白激酶B(AKT)、磷酸化蛋白激酶B(p-AKT)蛋白表达。结果:与模型组比较,推拿组大鼠DRG细胞Ca^(2+)浓度和DRG组织中IP3、IP3R含量呈降低趋势,其中DRG细胞Ca^(2+)浓度有显著差异(P<0.01),其他指标的组间差异无统计学意义(P>0.05);推拿组DRG组织中PLC含量及AKT、p-AKT蛋白表达呈增加趋势,但差异无统计学意义(P>0.05)。结论:腹部推拿抑制UC内脏高敏感性,其作用机制可能与抑制PLC-IP3R-Ca^(2+)信号通路和促进UC大鼠背根神经节AKT激活有关。

Pik3ip1通过抑制PI3K/AKT/mTOR信号通路促进牛MDSCs分化

PI3K相互作用蛋白1(Pik3ip1)为PI3K/AKT/mTOR信号通路负调控因子,其对牛MDSCs(Muscle derived satellite cells,MDSCs)分化研究较少。采用Western blot及免疫荧光,在牛MDSCs分化过程中检测Pik3ip1表达。构建Pik3ip1基因过表达及抑制载体,研究Pik3ip1对牛MDSCs分化及PI3K/AKT/mTOR信号通路活性的影响。结果表明,在牛MDSCs分化中Pik3ip1表达量逐渐升高;激活Pik3ip1表达后,细胞分化程度升高;抑制Pik3ip1表达则出现相反现象。Co-IP结果表明,在牛MDSCs分化过程中Pik3ip1与p110α相互作用。激活Pik3ip1抑制PI3K/AKT/mTOR信号通路活性。相反在抑制Pik3ip1表达后,PI3K/AKT/mTOR信号通路活性增强。综上所述,Pik3ip1通过抑制PI3K/AKT/mTOR信号通路促进牛MDSCs分化。

芪苈强心胶囊对心肌梗死大鼠心脏IP3Rs/GRP75/VDAC1基因调控的机制研究

目的:探讨芪苈强心胶囊对心肌梗死大鼠线粒体Ca^(2+)转运相关基因的调控作用。方法:采用冠状动脉左前降支结扎术建立心肌梗死大鼠模型。术后随机将动物分到模型组、芪苈强心组和卡托普利组;同时设有假手术组作为对照。治疗四周后,通过心脏大体结构观察大鼠心脏梗死范围,HE染色观察大鼠心肌组织病理形态变化;实时荧光(Real⁃Time)PCR检测大鼠心脏梗死边缘区线粒体Ca^(2+)转运相关基因三磷酸肌醇受体2(IP3R2),葡萄糖调节蛋白75(GRP75),电压依赖性阴离子通道1(VDAC1),线粒体融合蛋白2(Mfn2),以及线粒体凋亡相关基因B淋巴细胞瘤⁃2(Bcl⁃2),Bcl⁃2相关X蛋白(Bax)mRNA表达变化;Western blot检测心肌组织Bcl⁃2,Bax蛋白表达变化;TUNEL染色检测心肌组织细胞凋亡率。结果:与假手术组相比,模型组大鼠心脏左室前壁呈现大面积梗死区域,心肌组织结构紊乱;线粒体Ca^(2+)转运相关基因IP3R2,GRP75,VDAC1,Mfn2 mRNA表达显著升高(P<0.05,P<0.01);线粒体凋亡相关分子Bcl⁃2 mRNA和蛋白表达均明显下降(P<0.01),Bax mRNA和蛋白表达均显著升高(P<0.01),心肌细胞凋亡率显著增加(P<0.01)。与模型组相比,芪苈强心组和卡托普利组心脏大体标本的梗死范围缩小,心肌纤维排列相对规整;线粒体Ca^(2+)转运相关基因IP3R2,GRP75,VDAC1,Mfn2 mRNA表达显著降低(P<0.01);线粒体凋亡相关分子Bcl⁃2 mRNA和蛋白表达有所提高(P<0.05,P<0.01),Bax mRNA和蛋白表达显著降低(P<0.05,P<0.01),心肌细胞凋亡率明显下降(P<0.01)。结论:芪苈强心胶囊能够改善心肌梗死大鼠心脏形态结构,其作用机制与调节线粒体Ca^(2+)转运复合体IP3R2/GRP75/VDAC1基因表达,进而抑制细胞凋亡有关。

五加丹方对绝经综合征模型大鼠下丘脑PLC-β/IP3/CaM通路作用的研究

目的:探讨中药方剂五加丹方对去卵巢雌性大鼠下丘脑组织匀浆中PLC-β1、IP3、IP3R、CaM及PLC-β1、IP3R1、GnRHmRNA和GnRH、CaM蛋白的影响,试图阐释五加丹方对PLC-β/IP3/CaM通路及绝经综合征的影响。方法:取雌性SD大鼠64只,随机分为空白组(NG)、模型组(MG)、中药对照组(TMC)、西药对照组(WMC)各10只,五加丹方高(WH)、中(WM)、低剂量组(WL)各8只。除NG组外,其余6组均手术摘除大鼠双侧卵巢复制去势模型。模型复制成功后,各组采用灌胃给药1次/日,TMC组及WMC组分别给予相应剂量更年安片混悬液及补佳乐混悬液灌胃,NG组、MG组予等剂量生理盐水灌胃。4周后,处死大鼠,检测脑组织中PLC-β1、IP3、IP3R、CaM的含量;PCR法检测PLC-β、IP3R1、GnRH mRNA表达;Western Blot法检测各组脑组织CaM和GnRH蛋白的表达。结果:与NG组比较,大鼠去势后下丘脑组织PLC-β1、IP3、IP3R、CaM含量明显升高(P<0.01),PLC-β1、IP3R1、GnRHmRNA的表达显著升高(P<0.01),GnRH、CaM蛋白表达较空白组均升高(P<0.01),五加丹方可降低去势模型大鼠下丘脑组织中PLC-β1、IP3、IP3R、CaM水平,并下调PLC-β1、IP3R1、GnRHmRNA的表达。结论:五加丹方下调GnRH的表达,可能是通过作用于GnRH上游调节因子PLC-β1、IP3、IP3R、CaM等而产生,从而起到协调生殖轴功能,改善绝经综合征患者生殖内分泌水平。

不同频率摩腹法对脾虚型功能性消化不良家兔胃肠平滑肌IP3浓度及Ca^(2+)强度的影响

【目的】探讨不同频率摩腹法对脾虚型功能性消化不良(FD)家兔的治疗作用及机制。【方法】将76只家兔随机分为正常组、模型组、摩法低频组(机械臂摩腹101~150次/min)、摩法高频组(机械臂摩腹201~250次/min)、摩法低频+抑制剂组[机械臂摩腹101~150次/min+腹腔注射肌球蛋白轻链激酶(MLCK)抑制剂ML-92.0 mg·kg^(-1)]、摩法高频+抑制剂组(机械臂摩腹201~250次/min+腹腔注射ML-92.0 mg·kg^(-1))。除正常组外,其余各组采用苦寒泻下法联合饥饱失常法构建FD模型。干预过程中,记录家兔一般情况。干预结束后,采用酶联免疫吸附分析(ELISA)测定胃体、小肠平滑肌组织中三磷酸肌醇(IP3)浓度,采用流式细胞术测定家兔胃体平滑肌细胞中Ca^(2+)强度。【结果】经摩腹法干预后,高、低频组家兔一般情况有不同程度改善。摩法低频组、摩法高频组小肠平滑肌细胞IP3浓度较模型组升高(P<0.05或P<0.01),摩法低频+抑制剂组、摩法高频+抑制剂组IP3浓度较模型组降低(P<0.05)。摩法低频组、摩法高频组、摩法低频+抑制剂组胃体平滑肌细胞Ca^(2+)强度较模型组升高,其中摩法低频组、摩法高频组与模型组间的差异有统计学意义(P<0.01),摩法高频+抑制剂组Ca^(2+)强度较模型组降低(P<0.05);摩法低频组Ca^(2+)强度较摩法高频组升高,摩法低频+抑制剂组Ca^(2+)强度较摩法高频+抑制剂组升高(均P<0.01)。【结论】高、低频率摩腹法干预均可以改善脾虚型FD家兔症状,提高胃肠道平滑肌细胞中IP3浓度与Ca^(2+)强度,低频摩腹法的改善作用优于高频摩腹法。

The effect of Wujiadan Recipe on the role of PLC-β/IP3/CaM signaling pathway of hypothalamus in ovariectomized rats

Objective:To investigate the effect of Wujiadan Recipe on PLC-β1,IP3,IP3R,Cam,PLC-β1,IP3R1 mRNA and GnRH,Cam protein from hypothalamus tissue of ovariectomized female rats,and to further clarify whether Wujiadan Recipe plays a role through PLC-β/IP3/CaM signal pathway.Methods:We randomly divided 64 SD adult female rats into NG group(normal group),MG group(the model group),TMC group(the control group with traditional Chinese medicine),WMC group(the control group with western medicine)with 10 rats in each,and Wujiadan Recipe high(WH),Wujiadan Recipe medium(WM)and Wujiadan Recipe low dose group(WL)with 8 rats in each.Except the NG group,we removed the ovarian tissues of other six groups to establish the ovariectomized model.When the model is successfully replicated,we give the medicine to the rats in each group once a day.The TMC and WMC group were given the corresponding dose of Gengnian'an tablet suspension and Bujiale suspension by gavage respectively.The NG and MG group were given equal measure of normal saline.After 4 weeks,the rats were killed.We use ELISA to detecte the levels of PLC-β1,IP3,IP3R and Cam;and we use PCR to detecte the mRNA expression levels of PLC-βand IP3R1;and use WesternBlot to detecte the protein expression levels of Cam and GnRH in rat hypothalamus tissue.Results:The test results of PLC-β1,IP3,IP3R and Cam in the hypothalamus homogenate of the model group were significantly increased than the NG group(P<0.01).The results of PLC-β1 and IP3R1 and GnRHmRNA were significantly increased(P<0.01),and the expressions of GnRH and Cam protein were higher than NG(P<0.01).Wujiadan Recipe could reduce the results of PLC-β1,IP3,IP3R and Cam in hypothalamus of ovariectomized rats,and reduce the expression of PLC-β1 and IP3R1 and GnRH mRNA.Conclusion:Wujiadan Recipe down-regulates GnRH expression,which may be caused by acting on PLC-β1,IP3,IP3R,CaM in hypothalamus of ovariectomized rats,so as to coordinate the function of reproductive axis and improve the reproductive endocrine level of patients with menopausal syndrome.

Mechanism of Qiliqiangxin capsule on the regulation of IP3Rs/GRP75/VDAC1 gene in myocardial infarction rat heart

Objective:To investigate the regulatory effect of Qiliqiangxin Capsule on mitochondrial Ca^(2+)related genes in rats with myocardial infarction(MI).Methods:The rat model of MI was established by ligation of the left anterior descending coronary artery.After operation,the rats were randomly assigned to the model group,the Qiliqiangxin group and the captopril group;a sham-operated group was also available as a control.After four weeks of treatment,the extent of infarction in rats was observed by gross cardiac structure and the morphological changes of myocardial histopathology were observed by HE staining.Detection of mitochondrial Ca^(2+)transport-related genes such as inositol-1,4,5-trisphosphate receptor 2(IP3R2),glucose regulated protein 75(GRP75),voltage-dependent anion channel 1(VDAC1),and mitofusion 2(Mfn2)and mitochondrial apoptosis-related genes such as B-cell lymphoma-2(Bcl-2)and Bcl-2 related X protein(Bax)mRNA expression changes was measured by RT-PCR in the infarct margins of the heart;Western blot was used to detect changes in Bcl-2,Bax protein expression in myocardial tissue.The rate of apoptosis in cardiac myocardial tissue was detected by TUNEL staining.Results:Compared with the sham group,the anterior left ventricular wall of the model group showed a large area of infarction,and the structure of myocardial tissue was disordered.The mRNA expression level of mitochondrial Ca^(2+)transport-related genes such as IP3R2,GRP75,VDAC1,and Mfn2 were significantly increased(P<0.05,P<0.01);The mRNA and protein expression of Bcl-2,a molecule related to mitochondrial apoptosis,were significantly decreased(P<0.01),while the mRNA and protein expression of Bax were significantly increased(P<0.01);and apoptosis rate was significantly increased(P<0.01).Compared with the model group,the infarct size of cardiac gross specimens in the Qiliqiangxin group and the captopril group was reduced and myocardial fibers were relatively well ordered;The mRNA expression of mitochondrial Ca^(2+)transport-related genes such as IP3R2,GRP75,VDAC1,and Mfn2 were significantly reduced(P<0.01);the mRNA and protein expression of Bcl-2,a molecule related to mitochondrial apoptosis,were increased(P<0.05,P<0.01),and the mRNA and protein expression of Bax were significantly decreased(P<0.05,P<0.01).and apoptosis rate was significantly decreased(P<0.01).Conclusion:Qiliqiangxin Capsule can improve the morphological structure of the heart of rats with MI,and its mechanism is related to regulation of the gene expression of mitochondrial Ca^(2+)transport complex IP3R2/GRP75/VDAC1,thereby inhibiting apoptosis.

老年胃癌患者幽门螺旋杆菌感染与血清BEX2、APOC1、PIK3IP1表达的相关性

目的探讨老年胃癌患者幽门螺旋杆菌(Hp)感染与血清脑表达的X连锁基因2(BEX2)、载脂蛋白C1(APOC1)、磷脂酰肌醇3激酶相互作用蛋白1(PIK3IP1)表达的相关性。方法前瞻性选取2022年3月至2023年1月复旦大学附属中山医院青浦分院收治的老年胃癌患者86例,作为胃癌组,另选取同期在同院行胃镜检查的非胃癌者80例作为对照组。对比胃癌和非胃癌患者血清中BEX2、APOC1和PIK3IP1的mRNA水平及Hp感染U值,Hp不同感染程患者与未感染患者血清BEX2、APOC1、PIK3IP1的mRNA表达水平,不同临床病理特征患者血清BEX2、APOC1、PIK3IP1的mRNA表达水平,应用Pearson相关性分析BEX2、APOC1和PIK3IP1 mRNA水平与Hp感染U值的相关性,采用受试者工作特征(ROC)曲线分析血清中BEX2、APOC1和PIK3IP1 mRNA表达水平对老年胃癌患者Hp感染诊断价值。结果胃癌患者血清中BEX2、APOC1 mRNA水平及Hp感染U值均明显高于对照组,胃癌患者血清中PIK3IP1 mRNA水平明显低于对照组,差异均有统计学意义(P<0.05)。HpⅠ级、HpⅡ级、HpⅢ级感染患者中BEX2、APOC1 mRNA水平均明显高于Hp未感染的患者,HpⅠ级、HpⅡ级、HpⅢ级感染患者中PIK3IP1 mRNA水平明显低于Hp未感染的患者,差异均有统计学意义(P<0.05)。老年胃癌患者血清中BEX2、APOC1和PIK3IP1 mRNA水平与TNM分期、分化程度、淋巴结转移有关(P<0.05),与性别、年龄、肿瘤直径无关(P>0.05);老年胃癌患者血清中BEX2、APOC1 mRNA水平与Hp感染U值呈正相关(r=0.425、0.347,P<0.05),PIK3IP1 mRNA水平与Hp感染U值呈负相关(r=-0.323,P=0.002);3者联合检测诊断老年胃癌患者Hp感染的ROC曲线下面积AUC值明显优于BEX2、APOC1和PIK3IP1 mRNA 3者单独检测(P<0.05)。结论老年胃癌患者血清中BEX2和APOC1 mRNA表达升高,PIK3IP1 mRNA表达降低,与胃癌的TNM分期、分化程度、淋巴结转移及Hp的感染程度相关,3者联合检测BEX2、APOC1和PIK3IP1 mRNA对老年胃癌患者Hp感染具有一定的诊断效能。

预先电针三阴交 血海 合谷对痛经大鼠模型子宫IP_3的影响

目的:观察预先电针同经不同类及不同经脉腧穴对痛经大鼠模型子宫IP3的影响。方法:50只雌性SD大鼠,随机分为盐水组、模型组、电针三阴交组、血海组、合谷组,每组10只。除盐水组外,其余各组大鼠均连续10天给予大鼠皮下注射苯甲酸雌二醇注射液,末次给药后1h,腹腔注射缩宫素2U/只,制造痛经大鼠模型,盐水组每日给予同等剂量的生理盐水。于第8日针刺各组给予电针20min,盐水组及模型组束缚20min,每日1次,共3次,于末次针刺后观察扭体反应,并采用酶联免疫法检测子宫IP3。结果:①每分钟扭体分数:与盐水组比较,模型组、血海组及合谷组均明显升高(P均<0.01);三阴交组无显著性差异(P>0.05)。与模型组比较,三阴交组显著性降低(P<0.05);血海组、合谷组均无显著性差异(P均>0.05)。各电针组之间比较,血海组较三阴交组明显升高(P<0.01)。②子宫IP3水平:与盐水组比较,模型组、血海组、合谷组均显著降低(P<0.01,P<0.05);三阴交无显著性差异(P>0.05)。与模型组比较,三阴交组明显升高(P<0.01);血海组、合谷组均无统计学差异(P均>0.05)。各电针组之间比较,三阴交组明显高于血海组、合谷组(P均<0.01)。结论:三阴交组明显抑制了大鼠扭体反应,其机制是通过对IP3信号转导途径的生理性调节,而产生抑制子宫平滑肌收缩的作用。血海组及合谷组对扭体反应及IP3均未产生明显调节作用,表明同经不同类及不同经脉穴位之间的效应存在差异。

苏云金芽孢杆菌营养期杀虫蛋白基因vip3A的研究

根据已知vip3A基因序列设计一对特异性引物VIP3／VIP5，对218株Bt菌株进行PCR鉴定，有51株含有vip3A类基因，其中12株为不同亚种的标准菌株，有4株标准菌株不含有该基因。从Bt C9菌株中分离克隆了vip—C9基因，并插入表达载体pET—21b，转化大肠杆菌BL21，诱导表达出分子量88．6kDa的可溶性蛋白，表达产物对甜菜夜蛾和棉铃虫具有较高的杀虫活性，LC50分别为0．42ng／mg和25．95ng／mg，对小菜蛾活性较低。构建了缺失蛋白Vip—C9—N(N端去除39个氨基酸组成的信号肽序列)，杀虫活性测定结果表明其对甜菜夜蛾的活性显著降低，说明N端39个氨基酸对甜菜夜蛾的活性是必需的。

白香丹含药血清对大鼠海马神经元中5-羟色胺2C受体的表达及其下游信号通路中IP_3的影响

目的观察白香丹胶囊含药血清对原代海马神经元中5-羟色胺2C受体(5-HTR2C)蛋白表达水平及下游信号通路中IP3含量的影响,探讨其可能的中枢作用机制。方法采用情志刺激为主多因素造模法制备经前期综合征(PMS)肝气逆证大鼠模型,给予白香丹干预,制备大鼠含药血清,结合中药血清药理学,对体外培养的新生大鼠原代海马神经元进行不同血清干预,运用Western blot方法检测海马神经元中5-HTR2C蛋白表达水平,运用ELISA法检测各组海马神经细胞内IP3的含量。结果与正常血清组相比,PMS肝气逆模型血清组海马神经元的5-HTR2C蛋白表达水平和下游信号通路中IP3含量均明显升高(P<0.01,P<0.01),白香丹含药血清能够明显降低5-HTR2C蛋白表达水平和IP3的含量(P<0.01,P<0.01)。结论 PMS肝气逆证模型大鼠血清使海马神经元中5-HTR2C蛋白表达异常升高,同时,可引起第二信使IP3含量升高;白香丹胶囊可能通过降低5-HTR2C蛋白表达水平,改变其下游信号通路中IP3的含量而发挥疗效。

磷脂酶C对ADP诱导的兔血小板IP_3水平的影响

目的测定磷酯酶C（PLC）对ADP诱导的兔血小板三磷酸肌醇（IP3）的影响，从而进一步阐明PLC抗血小板聚集作用的机制。方法取家兔血除去红细胞制备血小板，血小板计数后分为8个组。第1组用生理盐水处理，第2组用ADP处理，第3组用ASP处理以ADP诱导激活，第4～8组分别用不同剂量的PLC处理并以ADP诱导激活。采用三氯醋酸法制备血小板IR，再用放射免疫分析法分别测定IR含量。结果家兔血小板经生理盐水处理后的IP3含量为0．29pmol／10。血小板，而经ADP处理后IR含量为0．39pmol/10^8血小板。经ASP668μmol·L^-1、5、10、15、20和25U PLC·ml^-1各组处理，并以ADP激活的血小板，测得的IP3含量分别为0．19、0．08、0．15、0．25、0．04和0．18μmol／10^8血小板）。ADP组比生理盐水组IP3有明显的提高，而ASP组、不同的PLC组比ADP组IR有明显的降低（P〈0.05）。结论PLC使得ADP激活后的兔血小板IP3水平下降，且无剂量依赖性，表明PLC具有降低血小板中IP3水平的作用，这可能是PLC抗血小板聚集作用的重要原因之一。

钙信号通过IP3通路对肥胖小鼠脂肪合成代谢的影响

【目的】探讨IP3信号通路是否会影响肥胖小鼠细胞内的钙离子浓度以及钙信号对肥胖小鼠脂肪代谢的作用机制,进一步了解胞内钙离子浓度变化对脂肪代谢的作用机理。【方法】用高脂日粮饲喂小鼠30d以建立肥胖模型,将肥胖小鼠分为对照组、去甲肾上腺素(NE)组、肝素组、钙组、钙+NE组和钙+肝素组,除对照组和钙组外的各药物组小鼠分别给予相应的药物处理,腹腔注射质量浓度0.1mg/mL的NE或1.5mg/mL的肝素0.2mL/(只.d);对照组和钙组同法给予等体积的生理盐水。对照组、NE组和肝素组小鼠饲喂普通日粮,钙组、钙+NE组和钙+肝素组小鼠饲喂加钙饲粮(钙含量12g/kg),小鼠共饲喂16d,期间每3d测1次体质量,17d时禁食12h,摘眼球取血后脱颈椎处死,分离血清检测其中甘油三酯(TG)、总胆固醇(TC)和高密度脂蛋白(HDL-C)的浓度,并取脂肪组织,测定附睾脂肪和肾周脂肪组织质量,分析附睾脂肪、肾周脂肪和肝脏的钙含量。通过RT-PCR法分析与脂肪生成密切相关的转录因子PPARγ、C/EBPα和脂解基因HSL及生脂基因FAS mRNA的表达水平,检测IP3受体IP3R1的mRNA表达水平。【结果】肝素和膳食钙处理对肥胖小鼠有极显著的减肥效果(P<0.01),可极显著减少体脂质量(P<0.01),降低血清中TG和TC浓度(P<0.01),而HDL-C浓度极显著升高(P<0.01),肝素和膳食钙处理肥胖小鼠的PPARγ、FAS和IP3R1的mRNA水平均极显著降低(P<0.01),HSL mRNA水平极显著升高(P<0.01),C/EBPα的mRNA水平无明显变化;NE处理对肥胖小鼠的作用效果与肝素相反,其可明显削弱减肥作用(P<0.01)。膳食钙有显著的减肥效果(P<0.01),但钙+NE组的减肥效果弱于钙组(P<0.01),钙+肝素组的减肥效果强于膳食钙的处理效果(P<0.01)。【结论】IP3通路激活可引起胞内钙离子浓度升高,脂肪蓄积增加;反之,脂肪蓄积减少。通过IP3通路,膳食钙可抑制胞内钙离子增加。

补脾方药对脾虚大鼠壁细胞内三磷酸肌醇(IP_3)含量的影响

目的:观察脾虚大鼠模型壁细胞内IP3含量的变化及补脾方药党参、白术、补中益气汤对其的影响。方法:大鼠壁细胞采用EDTA-Pronase酶消化法,采用竞争蛋白结合法测定大鼠壁细胞内IP3含量。结果:大黄脾虚模型大鼠壁细胞内IP3含量显著低于正常组,经党参、白术、补中益气汤治疗后,IP3含量有不同程度的升高,尤以党参组明显。结论:脾虚证可能与壁细胞内IP含量生成量减少相关,补脾方药对其有一定的调节作用。

PLC及IP_3R拮抗剂对弥漫性轴索损伤后继发性脑损伤的治疗作用

目的研究弥漫性轴索损伤(diffuse axonal injury,DAI)后PLC及IP3R抑制剂对DAI引发的脑水肿及神经元变性、损伤程度的影响,阐明PLC及IP3R抑制剂对DAI后继发性损伤的治疗作用。方法采用头颅冠状面瞬间加速旋转装置,制作大鼠颅脑DAI模型,并使用侧脑室穿刺给药的方法注射PLC抑制剂U73122及IP3R抑制剂光溜海绵素C(Xestospongin,XeC)。采用干湿重法测量脑组织含水量,ELISA测量脑脊液及动脉血中血清白蛋白(Alb)浓度并计算比值(QAlb),免疫组化法测量β-淀粉样前体蛋白(β-APP)的阳性面积及Western blot方法测量PLC的磷酸化程度。结果 DAI后6h大鼠脑组织含水量已明显增加,24h到达顶点,之后逐步下降,在5d时恢复到损伤前水平,XeC及U73122干预明显降低了损伤后24h脑组织含水量。ELISA结果显示DAI后6h及24h脑脊液中Alb浓度及QAlb明显升高,之后下降至损伤前水平,XeC及U73122干预对DAI引起的脑脊液中Alb浓度及QAlb升高无明显影响。免疫组化结果显示DAI后24h的β-APP的阳性面积较损伤前明显升高,XeC及U73122干预显著降低了DAI后24h的β-APP阳性面积。结论 DAI后脑水肿的形成是由细胞毒性水肿及血管源性水肿共同构成的;PLC及IP3R抑制剂降低了DAI后的细胞毒性水肿及神经元变性、损伤程度,对DAI后的继发性脑损伤具有治疗作用。

复心汤对大鼠原代心肌细胞IP3-Ca^(2+)/CaM-CaN通路的影响

目的研究用复心汤含药血清培养的大鼠原代心肌细胞中IP3-Ca^(2+)/CaM-CaN通路的表达情况,并与缬沙坦干预后的心肌细胞模型进行比较,观察复心汤对心肌细胞的干预效果,进一步探讨复心汤抗心衰的作用靶点及机制,为临床及科研提供一条新思路。方法健康成年的雄性Wistar大鼠50只,随机分为空白对照组、复心汤低剂量组、复心汤中剂量、复心汤高剂量组、西药(缬沙坦)组,分别给予生理盐水,低、中、高剂量复心汤及缬沙坦每天1次灌胃1周,末次灌胃后腹主动脉采血并分离血清,血清经灭活、滤菌。含药血清干预原代心肌细胞后分别采用Elisa、激光共聚焦成像技术、Western blot法检测心肌中IP3、Ca^(2+)、CaM及CaN的表达情况及或定量分析。结果复心汤高剂量组及西药组IP3表达量较空白组明显降低,有显著统计学意义(P<0.01);复心汤中、高剂量及西药组CaM、CaN表达量明显降低,差异有统计学意义(P<0.01或P<0.05);与西药组相比,复心汤高剂量组IP3、CaM、CaN表达量差异无显著统计学意义(P>0.05);Ca^(2+)荧光探针荧光强度由高到低依次是空白组,复心汤低、中、高剂量组,西药组。表明高剂量复心汤治疗心衰的效果与缬沙坦相当。结论复心汤治疗心衰可能与IP3-Ca^(2+)/CaM-CaN通路有关。