Effects ofβ_2-Adrenergic Antagonist on Cytosolic Ca^(2+) in Ventricular Myocytes from Infarcted Rat Heart

Objectives To investigate the effects of β2-adrenergic antagonist on cytosolic Ca^2 ＋ （[Ca^2＋ ]i） in ventricular myocytes from infarcted rat heart. Methods A ligature was placed around left anterior descending coronary artery of rat hearts. Rats in the control group were sham-operated. Cardiomyocytes were dissociated at two, four, eight weeks after myocardial infarction （MI） and [Ca^2＋]i was measured via fura-2 fluorescence. The response of cardiomyocytes to isoproterenol in presence or absence of betal-adrenergic antagonist atenolol, beta2-adrenergic antagonist ICI118, 551 or non-selective β1, 2- adrenergic antagonists propranolol was examined. Results The followings were found that ICI 118, 551 had no significant effects on the rise of [Ca^2＋]i induced by isoproterenol in normal ventricular myocytes （P 〉 0.05）, ICI118, 551 only significantly attenuated the rise of [Ca^2＋]i induced by isoproterenol at four weeks and eight weeks after MI （24.5%±5.7% vs 57.8% ± 13.2%, P〈 0.01; 12.2%±7.9% vs 44.6%±11.3%, P〈 0.01）. Atenolol had suppressive effects only in the control group and the post-MI group of two weeks （P 〈 0.05）, and propranolol had suppressive effects in the control and all the three post-MI groups （P 〈 0.01）. Conclusions Beta2-adrenergic antagonist ICI118, 551 may exert negative effects on Ca^2＋ overload initiated by sympathetic stimulation after MI.

Relationship of Intracellular Free Ca^(2+) Concentration and Calcium-activated Chloride Channels of Pulmonary Artery Smooth Muscle Cells in Rats under Hypoxic Conditions

To investigate the relationship between intracellular free Ca^2＋ concentration （[Ca^2＋ ]i ） and calcium-activated chloride （Clca） channels of pulmonary artery smooth muscle cells （PASMCs） in rats under acute and chronic hypoxic conditions, acute hypoxia-induced contraction was observed in rat pulmonary artery by using routine blood vascular perfusion in vitro. The fluorescence Ca^2＋ indicator Fura-2/AM was used to observe [Ca^2＋ ]i of rat PASMCs under normal and chronic hypoxic condition. The effect of Clca channels on PASMCs proliferation was assessed by MTT assay. The Clca channel blockers niflumic acid （NFA） and indaryloxyacetic acid （IAA-94） exerted inhibitory effects on acute hypoxia-evoked contractions in the pulmonary artery. Under chronic hypoxic condition, [Ca^2＋ ]i was increased. Under normoxic condition, [Ca^2＋ If was （123.634-18.98） nmol/ L, and in hypoxic condition, [Ca^2＋]i wag （281. 754-16.48） nmol/L （P〈0. 01）. Under normoxic condition, [Ca^2＋ ]i showed no significant change and no effect on Clca channels was observed （P〉 0. 05）. Chronic hypoxia increased [Ca^2＋ ]i which opened Clca channels. The NFA and IAA-94 blocked the channels and decreased [Ca^2＋ ]i from （281.75± 16.48） nmot/L to （117.66 ±15.36） nmol/L （P〈0.01）. MTT assay showed that under chronic hypoxic condition NFA and IAA-94 decreased the value of absorbency （A value） from 0. 459±0. 058 to 0. 224±0. 025 （P〈0. 01）. Hypoxia increased [Ca^2＋ ]i which opened Cl~ channels and had a positive-feedback in [Ca^2＋ ]i. This may play an important role in hypoxic pulmonary hypertension. Under chronic hypoxic condition, Clca channel may play a part in the regulation of proliferation of PASMCs.

牛磺酸和茵陈素对顺铂引起的原代培养肾小管上皮细胞内游离Ca^(2+)浓度变化的影响

目的 研究牛磺酸、茵陈素对顺铂引起的原代培养肾小管上皮细胞 (PTC)内游离Ca2 +浓度变化的影响。方法 在体外培养PTC、顺铂与PTC共同保温 2 4h ,牛磺酸、茵陈素分别提前与PTC作用 2 4h ,然后再加入顺铂 ( 2 6 μmol·L- 1 )共同保温 2 4h。采用Fura 2 AM测细胞内游离Ca2 +浓度。结果 顺铂 ( 13,2 6 ,5 2 μmol·L- 1 )升高PTC细胞内游离Ca2 +浓度 ,牛磺酸 ( 1,10g·L- 1 )和茵陈素 ( 4 ,8mg·L- 1 ) ,可拮抗顺铂导致的PTC细胞内游离Ca2 +浓度超载。结论 顺铂可引起原代培养肾小管上皮细胞内Ca2 +超载 ,牛磺酸、茵陈素能拮抗顺铂导致的细胞内Ca2 +超载 ,起到细胞保护作用。

MN9202对血栓形成大鼠红细胞Ca^(2+)浓度、脂质过氧化的影响及其与增强红细胞变形性关系的探讨

目的 探讨二氢吡啶类钙拮抗剂 2 ,6 二甲基 4 (3 硝基苯基 ) 1,4 二氢 3,5 吡啶二羧酸 3 甲酯 5 正戊酯(MN92 0 2 )增强红细胞 (RBC)变形性的可能机制。方法 角叉菜胶复制大鼠血栓模型 ;荧光染料Fura 2负载 ,荧光分光度法测定RBC内游离Ca2 +浓度 ;紫外分光光度法测定脂质过氧化产物丙二醛 (MDA)以及膜蛋白交联形成的共轭双烯的含量 ;孔雀绿法测定Ca MgATPase活力。 结果 MN92 0 2在本实验剂量范围内 ,剂量依赖地降低RBCMDA含量 (r =0 998) ,抑制膜共轭双烯的形成。MN92 0 2 0 1、1μmol·kg-1能增强全血SOD活力 ;有效抑制角叉菜胶引起的RBC内Ca2 +浓度的升高 ,但对RBCCa MgATPase活性无影响。结论 MN92 0 2阻断Ca2 +内流、抑制脂质过氧化是其改善RBC变形性的主要机制。

凝血酶对荧光标记的人单个血小板游离［Ca^（2＋）］和膜电位的动态影响

本文将ｆｌｕｏ－３和ｄ_ｉ－ＢＡ－Ｃ４（３）荧光标记的血小板固定于纤维蛋白原表面，以５７０型粘附式细胞仪（ＡＣＡＳ５７０）动态观察了凝血酶激活的人单个血小板细胞内游离［Ｃａ^（２＋）］（钙离子浓度）和膜电位的变化。静息状态时细胞游离［Ｃａ^（２＋）］和膜电位荧光较低，波动不明显。当加入０．１Ｕ／ｍｌ凝血酶激活时，［Ｃａ^（２＋）］（细胞内游离钙离子浓度）与膜电位迅速升高，随后［Ｃａ^（２＋）］出现反复振荡，幅度达约５００荧光单位，而膜电位基本上保持峰值水平。［Ｃａ^（２＋）］_ｉ升高与膜电位变化在时间和程度上不一致。本文结果提示，凝血酶引起血小板［Ｃａ^（２＋）］振荡和膜去极化，后者不是Ｃａ^（２＋）内流引起的。

1-(2,6-二甲基苯氧基)-2-(3,4-二甲氧基苯乙氨基)丙烷盐酸盐对培养的乳鼠心肌细胞[Ca^(2+)]_i的影响

采用 Fura- 2 / AM显微荧光测钙技术 ,检测培养新生大鼠单个心肌细胞内游离钙的浓度 ,并观察 1- (2 ,6 -二甲基苯氧基 ) - 2 - (3,4-二甲氧基苯乙氨基 )丙烷盐酸盐 (DDPH)对不同刺激〔去氧肾上腺素 ,高 K+ ,血管紧张素 (Ang II)〕所致心肌细胞钙超载的影响。结果表明 :1在含钙、无钙标准台氏液 ,DDPH 10 - 4 m ol· L- 1 对去氧肾上腺素(Phe) 10 - 4 mol· L- 1 所致钙增高有显著抑制作用。 2 DDPH 10 - 4 m ol· L- 1 对高 K+ 5 0 m mol· L- 1 引起的 [Ca2 + ]i增高有一定抑制作用 ,对 Ang 10 - 4 mol· L- 1 引起的 [Ca2 + ]i增高有部分拮抗作用。提示 :DDPH可拮抗 α1 受体调控的 Ca2 +通道 ,对钙库钙释放也有抑制作用 。

外源性神经节苷脂GM_3对Ca^（2＋）－ATP酶及红细胞胞浆Ca^（2＋）－浓度的影响

研究神经节苷脂ＧＭ３（简称ＧＭ３）对部分纯化的人红细胞膜Ｃａ２＋－ＡＴＰ酶的作用和对完整兔红细胞浆［Ｃａ２＋］的影响。结果表明：外源性ＧＭ３对Ｃａ２＋－ＡＴＰ酶的作用呈浓度依赖性双相调节即浓度为１～６．５μｍｏｌ／Ｌ时抑制酶活性，浓度大于６．５μｍｏｌ／Ｌ时激活酶活性；ＧＭ３不影响钙调素（ＣａＭ）对酶的激活；ＣＭ３对兔红细胞浆［Ｃａ２＋］也呈浓度依赖性双相调节即在ＧＭ３浓度低于６９μｍｏｌ／Ｌ时［Ｃａ２＋］有不同程度升高，浓度大于６０μｍｏｌ／Ｌ时则降低［Ｃａ２＋］。

蝙蝠葛苏林碱对PC12细胞内游离钙浓度的影响

目的进一步探讨蝙蝠葛苏林碱（Dau）的抗脑缺血／缺氧损伤与其钙拮抗作用间的关系。方法：培养的PC12细胞用Fura－2／AM负载，用AR－CM－MIC阳离子测定系统观测Dau对单细胞内游离钙（[Ca(2+)]_i）升高的影响。结果：Dau（0．1～100μmol·L(－1)）可浓度依赖性抑制高钾和caffeine引起的[Ca(2+)］_i增加，对肌浆网钙泵抑制剂cy－clopiszonicacid引起的[Ca(2+)]_i升高也有抑制作用。结论：Dau不仅抑制电压依赖性钙通道开放引起的细胞外钙内流和caffeine引起的内钙释放．而且对钙泵也可能有影响，这可能是其抗脑缺血／缺氧损伤的重要机制。

芥子碱对PC12细胞内游离钙升高的影响

目的:考察芥子碱对高钾除极和谷氨酸引起细胞外钙内流以及咖啡因和环匹阿尼酸(cyclopia-zonic acid,CPA)引起细胞内钙释放所导致的PC12细胞内游离钙升高的影响。方法:PC12细胞用终浓度为5μmo.lL-1的钙离子荧光指示剂Fluo-3/AM于37℃避光负载孵育。细胞内游离钙([Ca2+]i)用VictorⅡ1420多功能标记分析仪检测,以荧光强度(FI)表示。结果:当有外钙存在时,PC12细胞静息[Ca2+]i的FI值为(1 188±163),75 mmol.L-1KCl和10 mmol.L-1谷氨酸引起细胞外钙内流,使[Ca2+]i增高,FI峰值分别增至(4 270±982)和(3 096±402)。芥子碱(0.01,0.1,1.0,10,100μmol.L-1)对静息[Ca2+]i没有明显的影响,但浓度相关性地抑制高钾和谷氨酸诱发的[Ca2+]i增高,抑制率分别为10.2%,39.5%,53.7%,71.8%,88.4%和30.3%,55.7%,68.5%,79.2%,94.1%。当无外钙存在时,PC12细胞静息[Ca2+]i的FI值为(813±112)。咖啡因(40 mmol.L-1)和CPA(30μmol.L-1)分别引起Caffeine-ryanodine和三磷酸肌醇(InsP3)敏感型-钙池释放而使[Ca2+]i升高,FI值分别增至(2 944±371)和(1 844±332)。芥子碱(0.1,1.0,10,100μmol.L-1)浓度相关性地抑制咖啡因和CPA诱发的[Ca2+]i增高,抑制率分别为23.7%,61.9%,77.5%,88.2%和10.9%,23.8%,44.6%,68.3%。结论:芥子碱能显著抑制电压依赖性和受体依赖性钙通道开放所引起的外钙内流,且对受体依赖性钙通道的抑制作用更强。此外,芥子碱对Caffeine-ryan-odine受体和InsP3敏感型钙池的内钙释放也有明显抑制作用,且对Caffeine-ryanodine受体敏感型钙池的抑制作用更强。这提示芥子碱有望成为很有研发前景的新型钙阻滞剂。

2型糖尿病患者细胞内钙离子浓度变化的研究

目的:探讨型糖尿病患者血中单个核细胞内2Ca2+浓度变化及其与胰岛素受体活性变化的关系。TPK方法:荧光分光分析法测定例型糖尿病及例正常对照单个核细胞内40220Ca2+浓度,并用酶联免疫法测定单个核细胞胰岛素受体酪氨酸激酶()活性。TPK结果:型糖尿病患者单个核细胞内2Ca2+浓度显著高于正常对照组,胰岛素受体活性显著低于正常对照TPK组。相关分析显示型糖尿病患者单个核细胞内2Ca2+浓度与、显著正相关,与受体活性显著负相关。FBGFINSTPK结论:细胞内Ca2+浓度升高可能通过影响胰岛素受体活性参与胰岛素抵抗的发生。

用Fura-2测定人外周血中性粒细胞内游离钙浓度

本文用 2 - [6-双乙酸基 - 5 - ( 2 -双乙酸基 ) - 5 -甲苯氧乙氧基 ]- 2 -苯骈呋喃基 - 5 -恶唑羧酸五钾盐 ( Fura- 2 )建立了测定人外周血中性粒细胞内游离钙浓度的方法 ,并对一些测试条件进行了探讨。测定标本内中性粒细胞数以大约 10 6个 /m L为宜 ,在离心分离出中性粒细胞悬液时 ,标本制备好需静置 0 .5 h后才能上机测试 ,否则振荡形成的剪切应力将增大细胞内游离钙的浓度 ,p H偏离 7.4和受损细胞会极大增加细胞内游离钙的浓度。结果表明 ,正常人外周血中性粒细胞游离钙浓度为 3.95± 0 .76μg/L。对中性粒细胞内游离钙的测定有助于了解其功能状态。

应用Frua-2测定人腹腔巨噬细胞胞浆游离钙浓度

为了解子宫内膜异位症患者腹腔巨噬细胞活性变化，建立了应用Ｆｒｕａ－２测定人腹腔巨噬细胞胞浆游离钙浓度（［Ｃａ２＋］ｉ）的方法。结果显示，正常盆腔患者腹腔巨噬细胞［Ｃａ２＋］ｉ为（１００．３２±５．６９）ｎｍｏｌ／Ｌ，而子宫内膜异位症患者腹腔巨噬细胞较正常盆腔者显著升高。

离体灌流鼠心胞浆游离钙—fura—2测定

本实验建立了一种浮动基点式 fura—2测定离体灌流心脏细胞内游离钙浓度的新模型。本模型中浮动基点式测定法克服了目前 fura—2技术中受细胞内某些物质产生的自身荧光变化干扰的缺点,实现了自动消除细胞自身荧光变化对实验结果的影响,并在此基础上将广泛用于测定游离状态的细胞内游离钙的 fura—2技术推广到了离体灌流心脏,实现了在更接近心肌生理状态的条件下测定其胞浆游离钙。

GM_3、GD_3作用下SMMC－7721肝癌细胞内磷脂酰肌醇（1，4，5）三

外源性ＧＭ３（１０ｎｍｏｌ／ｍＬ）、ＧＤ３（１ｎｍｏｌ／ｍＬ）可使ＳＭＭＣ－７７２１人肝癌培养细胞内钙浓度呈快速的短暂升高，其到达峰值时间为４５秒，一次作用后，内钙水平于２－３ｍｉｎ内恢复至对照水平。在一定时间间隔中连续几次加入ＧＭ３或ＧＤ３后内钙水平的变化表明，ＧＭ３所引起的［Ｃａ２＋］ｉ的增加依赖于内质网钙贮的释放和细胞外钙的流入；而ＧＤ３增加［Ｃａ２＋］ｉ与此二系统无关。进一步研究表明，在细胞内钙达峰值时，１０ｎｍｏｌ／ｍＬＧＭ３可使ＩＰ３（１，４，５）浓度增加９．３倍，ｃＡＭＰ浓度增加８２％；１ｎｍｏｌ／ｍＬＧＤ３反使Ｉｐ３浓度增加１．２倍，提示ＧＭ３、ＧＤ３升高内钙的不同机制。

EFFECTS OF ACUPUNCTURE ON INTRACELLULAR FREE CALCIUM AND MAGNESIUM CONCENTRATIONS IN CARDIAC MYOCYTES OF HEMORRHAGIC HYPOTENSION RABBITS

The effects of electroacupuncture on hypotension and the concentrations of intracellular free calcium([Ca2+]i) and free magnesium([ Mg2+]i) in cardiac myocyte of rabbit were studied. The hemorrhapic hypotension was induced by losing blood from femoral artery of rabbit. [Ca2+]i and [Mg2+]i were determined by use of AN-CM-COM cation measurment system and the Fura-2-AM and Furaptra-AM ionic probes. [Ca2+]i was significantly decreased, while [Mg2+]i was increased, and the ratio of [Ca2+]i / [ Mg2+]i was decreased as the blood pressure went down with losing blood. The blood pressure and [ Ca2+ ] i of treatment group rabbits were significantly raised by electroacupuncturing the points of "Renzhong "and "Chengjiang", and the ratio of [ Ca2+] i / [ Mg2+]i was increased. The [Ca2+]i and [ Mg2+]i in cardiac myocyte of normal rabbits had no clear changes by electroacupuncture. It suggested that intracellular free calcium and magnesium ion in cardiac myocyte may play an important role in regulating blood pressure by acupunoture.

钙指示剂Fura－2／AM对血小板功能及细胞内游离钙测定结果的影响

本实验结果表明，以Ｆｕｒａ－２／ＡＭ负载家兔洗脱血小板，当Ｆｕｒａ－２／ＡＭ的浓度低于２μｍｏｌ／Ｌ时，３μｍｏｌ／Ｌ和１０μｍｏｌ／Ｌ花生四稀酸（ＡＡ）诱导的血小板聚集（透光度增加：７２．５±７．８４％）及释放反应（ＡＴＰ释放：１．１２±０．２１μｍｏｌ／４×１０５血小板）不受影响，但随Ｆｕｒａ－２／ＡＭ浓度增加，ＡＡ的聚集和释放反应明显减弱（Ｐ＜０．０５或Ｐ＜０．０１）。Ｆｕｒａ－２／ＡＭ浓度对单一血小板内钙（［Ｃａ２＋］ｉ）的静息水平无影响，但Ｆｕｒａ－２／ＡＭ为２μｍｏｌ／Ｌ时，ＡＡ诱导的［Ｃａ２＋］ｉ动员最明显。另外，标本中血小板的数量也明显影响［Ｃａ２＋］ｉ的测定结果（Ｐ＜０．０５或Ｐ＜０．０１）。提示，Ｆｕｒａ－２／ＡＭ浓度过高，很可能导致过多的钙离子被螯合，降低了血小板的功能，同时，细胞内游离钙与Ｆｕｒａ－２／ＡＭ的结合过程存在着饱和性。

Current Injection Provokes Rapid Expansion of the Guard Cell Cytosolic Volume and Triggers Ca^2＋ Signals

High-resolution microscopy opens the door for detailed single-cell studies with fluorescent reporter dyes and proteins. We used a confocal spinning disc microscope to monitor fluorescent dyes and the fluorescent protein Venus in tobacco and Arabidopsis guard cells. Multi-barreled microelectrodes were used to inject dyes and apply voltage pulses, which provoke transient rises in the cytosolic Ca^2＋ level. Voltage pulses also caused changes in the distribution of Lucifer Yellow and Venus, which pointed to a reversible increase of guard cell cytosolic volume. The dynamic cytosolic volume changes turned out to be provoked by current injection of ions. A reduction of the clamp current, by blocking K^＋ uptake channels with Cs^＋, strongly suppressed the cytosolic volume changes. Cs^＋ not only inhibited the expansion of the cytosol, but also inhibited hyperpolarization-induced elevations of the cytosolic Ca^2＋ concentration. A complete loss of voltage-induced Ca^2＋ signals occurred when Ca^2＋-permeable plasma membrane channels were simultaneously blocked with La^3＋. This shows that two mechanisms cause hyperpolarization-induced elevation of the cytosolic Ca^2＋-concentration： （i） activation of voltage-dependent Ca^2＋-permeable channels, （ii） osmotically induced expansion of the cytosol, which leads to a release of Ca^2＋ from intracellular stores.

麝香糖蛋白成分对大鼠中性白细胞血小板活化因子生成及细胞内钙水平的影响

目的 :观察麝香 1对大鼠中性白细胞血小板活化因子生成及细胞内钙水平的影响。方法 :采用体外温孵系统 ,以同位素参入法测定PAF生成和乙酰转移酶活性 ,以Fura 2标记荧光法测定细胞内游离钙水平。结果 :麝香 1在 1～ 10 0 μg·ml-1浓度下可明显抑制中性白细胞PAF生成、乙酰转移酶活性和细胞内游离钙水平的升高。结论 :麝香 1对中性白细胞PAF生成、乙酰转移酶活性和胞内钙水平的抑制可能涉及其部分抗炎作用机制。

配子体自交不亲和信号转导的研究进展

自然界中大多数自交不亲和(selfincompatibility,SI)显花植物表现为配子体SI。配子体SI植物虽然都具有其SI的功能而阻止自我受精,但它们采取的信号转导途径是不同的。目前关于配子体SI信号转导的途径主要有两种:一是茄科、玄参科、蔷薇科中以雌蕊SRNase为基础的信号转导途径;另一是罂粟科中以花粉管胞质自由钙离子为第二信使的转导途径。文章就配子体SI信号转导的研究进展作一综述。

牛磺酸对顺铂导致培养的原代兔肾小管细胞损伤的保护作用

目的 :研究牛磺酸对顺铂导致培养的原代兔肾近端小管细胞 (PTC)损伤的保护作用。方法 :在体外建立原代兔肾近端小管细胞培养。采用溴乙锭荧光法测量DNA链间交联和Fur-2 /AM测量细胞内游离钙离子浓度。首先将牛磺酸 ( 0 .1,1,10g .L 1 )与PTC保温 2 4小时 ,然后 ,加入顺铂使其终浓度达到 2 6μmo1.L 1 ,再继续保温 2 4小时。顺铂损伤组同样培养 48小时 ,前 2 4小时不加入牛磺酸和顺铂 ,后 2 4小时加入顺铂使其终浓度为 2 6μmo1.L 1 。对照组不加入牛磺酸和顺铂 ,同样培养 48小时。结果 :顺铂导致损伤组形成DNA链间交联和细胞内游离钙离子浓度升高 ,牛磺酸 1,10g.L 1 可明显降低DNA链间交联和细胞内游离钙离子浓度。结论