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牛磺酸对钙结合至心肌肌膜的调节作用。

Taurine modulation of calcium binding to cardiac sarcolemma.

作者信息

Sebring L A, Huxtable R J

出版信息

J Pharmacol Exp Ther. 1985 Feb;232(2):445-51.

PMID:3918160
Abstract

A sarcolemma-enriched membrane fraction (SL) was prepared from the hearts of Sprague-Dawley rats and its ability to bind Ca++ was measured by equilibrium dialysis. We found that the effect of taurine on SL Ca++ binding varied with the buffer and with Na+ concentration. In Tris, in the presence of Na+ (140 mM), taurine (10 mM) increased the affinity but decreased the maximal binding of Ca++ (0.5-7 mM). In the absence of Na+, taurine decreased the affinity without altering the maximal binding. These effects on Ca++ binding were absent in bicarbonate or Krebs-Henseleit buffers. However, incubations with A23187, a Ca++ ionophore, and lanthanum, a Ca++ antagonist, indicated that SL membranes incubated in Tris, but not in buffers containing bicarbonate, were sealed vesicles with internal environments low in Ca++. High-affinity binding of Ca++ (10(-6)-10(-4) M) was measured in modified Krebs-Henseleit buffers. Taurine decreased Ca++ binding in a high-Na+ (145 mM), low-K+ (4.7 mM) buffer. Taurine increased Ca++ binding in both 4.7 mM Na+-145 mM K+ and 25 mM Na+-4.7 mM K+ buffers. Taurine also increased Ca++ binding in the presence of ATP. Thus, taurine increased high-affinity Ca++ binding in "intracellular" buffers, but it did not affect low-affinity Ca++ binding in "extracellular" buffers. These results suggest taurine may exert its cardiotonic actions through modulation of the high-affinity Ca++ binding sites on the internal aspect of the SL.

摘要

从Sprague-Dawley大鼠心脏制备富含肌膜的膜组分(SL),并通过平衡透析测量其结合Ca++的能力。我们发现,牛磺酸对SL结合Ca++的影响随缓冲液和Na+浓度而变化。在Tris缓冲液中,存在Na+(140 mM)时,牛磺酸(10 mM)增加了亲和力,但降低了Ca++(0.5 - 7 mM)的最大结合量。在无Na+的情况下,牛磺酸降低了亲和力,但未改变最大结合量。在碳酸氢盐或Krebs-Henseleit缓冲液中未观察到这些对Ca++结合的影响。然而,用Ca++离子载体A23187和Ca++拮抗剂镧进行孵育表明,在Tris缓冲液中孵育的SL膜是密封的囊泡,其内部环境中Ca++含量低,而在含碳酸氢盐的缓冲液中孵育的膜则不是。在改良的Krebs-Henseleit缓冲液中测量到了Ca++(10(-6)-10(-4) M)的高亲和力结合。在高Na+(145 mM)、低K+(4.7 mM)缓冲液中,牛磺酸降低了Ca++结合。在4.7 mM Na+-145 mM K+和25 mM Na+-4.7 mM K+缓冲液中,牛磺酸均增加了Ca++结合。在ATP存在的情况下,牛磺酸也增加了Ca++结合。因此,牛磺酸在“细胞内”缓冲液中增加了高亲和力Ca++结合,但在“细胞外”缓冲液中不影响低亲和力Ca++结合。这些结果表明,牛磺酸可能通过调节SL内侧的高亲和力Ca++结合位点发挥其强心作用。

相似文献

1
Taurine modulation of calcium binding to cardiac sarcolemma.牛磺酸对钙结合至心肌肌膜的调节作用。
J Pharmacol Exp Ther. 1985 Feb;232(2):445-51.
2
Modulation by taurine of calcium binding to phospholipid vesicles and cardiac sarcolemma.
Proc West Pharmacol Soc. 1987;30:153-5.
3
Taurine enhancement of calcium binding to rat heart sarcolemma.牛磺酸增强钙与大鼠心脏肌膜的结合。
Biochim Biophys Acta. 1979 Feb 20;551(1):129-35. doi: 10.1016/0005-2736(79)90359-6.
4
Effect of inorganic calcium channel blockers on dihydropyridine binding to cardiac sarcolemma.无机钙通道阻滞剂对二氢吡啶与心肌肌膜结合的影响。
Mol Pharmacol. 1990 Jan;37(1):80-9.
5
Effect of amrinone on sodium-calcium exchange in cardiac sarcolemmal vesicles.
Res Commun Chem Pathol Pharmacol. 1983 Aug;41(2):197-210.
6
[Propranolol beta-blocker decrease in the concentration of high-affinity binding sites for calcium ions by sarcolemma membranes of the rat heart].[普萘洛尔β受体阻滞剂使大鼠心脏肌膜上钙离子高亲和力结合位点的浓度降低]
Biull Eksp Biol Med. 1982 May;93(5):72-4.
7
Low affinity binding of taurine to phospholiposomes and cardiac sarcolemma.牛磺酸与磷脂体和心肌肌膜的低亲和力结合。
Biochim Biophys Acta. 1986 Dec 10;884(3):559-66. doi: 10.1016/0304-4165(86)90208-4.
8
[Passive Ca2+ permeability of vesicular sarcolemmal preparations from myocardium].[心肌囊泡肌膜制剂的被动钙离子通透性]
Biokhimiia. 1981 Oct;46(10):1863-79.
9
Calcium regulation by the low-affinity taurine binding sites of cardiac sarcolemma.心肌肌膜低亲和力牛磺酸结合位点对钙的调节作用
Mol Pharmacol. 1980 May;17(3):295-300.
10
Regulation of calcium homeostasis in the heart by taurine.牛磺酸对心脏钙稳态的调节
Fed Proc. 1980 Jul;39(9):2691-4.

引用本文的文献

1
Mechanisms underlying taurine-mediated alterations in membrane function.牛磺酸介导的膜功能改变的机制。
Amino Acids. 1995 Sep;8(3):231-46. doi: 10.1007/BF00806821.
2
Taurine: a preventive agent of the acute ethanol depletive action on the isolated human amniotic membrane.牛磺酸:一种预防乙醇对离体人羊膜急性消耗作用的试剂。
Amino Acids. 1995 Sep;9(3):275-83. doi: 10.1007/BF00805958.