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巨大心脏膜片法:MgATP对外向Na(+)-Ca2+交换电流的刺激作用

The giant cardiac membrane patch method: stimulation of outward Na(+)-Ca2+ exchange current by MgATP.

作者信息

Collins A, Somlyo A V, Hilgemann D W

机构信息

Department of Physiology, University of Texas Southwestern Medical Center, Dallas 75235-9040.

出版信息

J Physiol. 1992 Aug;454:27-57. doi: 10.1113/jphysiol.1992.sp019253.

Abstract
  1. A giant patch method was used to study the stimulatory effect of cytoplasmic MgATP on outward Na(+)-Ca2+ exchange current in inside-out cardiac membrane patches (1-10 G omega seals with 14-24 microns pipette tip diameters) excised from guinea-pig, rabbit and mouse myocytes. 2. To establish the validity of the method with respect to structure, bleb formation was examined with electron microscopy and with confocal fluorescence light microscopy. The blebs, which form as the sarcolemma detaches, excluded intracellular organelles and transverse tubules. The blebbed cells contained normal sarcomeres, sarcoplasmic reticulum, triads and diads. 3. To further establish the validity of the method for ion transport studies, measurements of Na(+)-K+ pump currents and charge movements are described briefly which demonstrate (i) free access to the cytoplasmic membrane side, (ii) MgATP dependence comparable to reconstituted pump (Kd, 94 microns), (iii) fast, rigorous concentration control and (iv) Na(+)-K+ pump densities in the range of whole-cell densities. 4. Stimulation of outward Na(+)-Ca2+ exchange current by MgATP attenuated exchange current decay during step increments of cytoplasmic sodium, shifted the secondary activation of outward exchange current by cytoplasmic calcium to lower free calcium concentrations and, particularly in mouse cardiac sarcolemma, induced cytoplasmic calcium-independent current. 5. Upon removal of MgATP the stimulatory effect usually decayed with a t50 (half-time) of about 3 min. However, the reversal took place much more rapidly (t50, 5-20 s) in patches from individual guinea-pig and rabbit myocyte batches. When decay was rapid, secondary activation by cytoplasmic calcium was shifted to higher free cytoplasmic calcium concentrations (Kd, 10-65 microns-free calcium). 6. With repeated applications of MgATP the rate and magnitude of the stimulatory effect progressively decreased. 7. The Kd for MgATP of the initial rate of stimulation of outward exchange current was 3 mM or greater. When decay was rapid, the steady-state dependence of exchange current on MgATP also had a Kd of 3 mM or greater. 8. Stimulation of Na(+)-Ca2+ exchange current by MgATP occurred in the absence of cytoplasmic calcium with 9 mM-EGTA. 9. The stimulatory effect of 2 mM-MgATP was not inhibited by up to 200 microM of the protein kinase inhibitor 1-(5-isoquinoline sulphonyl)-2-methylpiperazine (H7), or by peptide inhibitors of cyclic AMP-dependent protein kinase, protein kinase C and calcium-calmodulin-dependent protein kinase II.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 采用巨斑片钳法研究了胞质MgATP对豚鼠、兔和小鼠心肌细胞内翻式细胞膜片(吸管尖端直径14 - 24微米,封接值1 - 10 GΩ)外向Na⁺-Ca²⁺交换电流的刺激作用。2. 为从结构方面证实该方法的有效性,用电子显微镜和共聚焦荧光显微镜检查了小泡形成情况。小泡是在肌膜分离时形成的,排除了细胞内细胞器和横管。有小泡的细胞含有正常的肌节、肌浆网、三联体和二联体。3. 为进一步证实该方法用于离子转运研究的有效性,简要描述了Na⁺-K⁺泵电流和电荷移动的测量结果,这些结果表明:(i)可自由接触细胞质膜侧;(ii)对MgATP的依赖性与重组泵相当(解离常数Kd为94微摩尔);(iii)能快速、严格地控制浓度;(iv)Na⁺-K⁺泵密度在全细胞密度范围内。4. MgATP对外向Na⁺-Ca²⁺交换电流的刺激作用减弱了细胞质钠阶跃增加期间交换电流的衰减,将细胞质钙对外向交换电流的二次激活转移到更低的游离钙浓度,特别是在小鼠心肌肌膜中,诱导了不依赖细胞质钙的电流。5. 去除MgATP后,刺激作用通常以约3分钟的半衰期(t50)衰减。然而,在来自单个豚鼠和兔心肌细胞批次的膜片中,反转发生得更快(t50为5 - 20秒)。当衰减迅速时,细胞质钙的二次激活转移到更高的游离细胞质钙浓度(Kd为10 - 65微摩尔游离钙)。6. 重复应用MgATP时,刺激作用的速率和幅度逐渐降低。7. 外向交换电流初始刺激速率的MgATP解离常数Kd为3毫摩尔或更高。当衰减迅速时,交换电流对MgATP的稳态依赖性的Kd也为3毫摩尔或更高。8. 在含有9毫摩尔乙二醇双四乙酸(EGTA)且无细胞质钙的情况下,MgATP刺激了Na⁺-Ca²⁺交换电流。9. 2毫摩尔MgATP的刺激作用不受高达200微摩尔的蛋白激酶抑制剂1 -(5 - 异喹啉磺酰基)- 2 - 甲基哌嗪(H7)、环磷酸腺苷依赖性蛋白激酶、蛋白激酶C和钙调蛋白依赖性蛋白激酶II的肽类抑制剂的抑制。(摘要截断于400字)
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3109/1175594/8fc68c6b81ef/jphysiol00428-0061-a.jpg

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