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Gap junctional conductance between pairs of ventricular myocytes is modulated synergistically by H+ and Ca++

机译:H +和Ca ++协同调节成对的心室心肌细胞之间的间隙连接电导

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摘要

Gap junctional conductance (gj) between cardiac ventricular myocyte pairs is rapidly, substantially, and reversibly reduced by sarcoplasmic acidification with CO2 when extracellular calcium activity is near physiological levels (1.0 mM CaCl2 added; 470 microM Ca++). Intracellular calcium concentration (Cai), measured by fura-2 fluorescence in cell suspensions, was 148 +/- 39 nM (+/- SEM, n = 6) and intracellular pH (pHi), measured with intracellular ion-selective microelectrodes, was 7.05 +/- 0.02 (n = 5) in cell pair preparations bathed in medium equilibrated with air. Cai increased to 515 +/- 12 nM (n = 6) and pHi decreased to 5.9-6.0 in medium equilibrated with 100% CO2. In air-equilibrated low-calcium medium (no added CaCl2; 2-5 microM Ca++), Cai was 61 +/- 9 nM (n = 13) at pHi 7.1. Cai increased to only 243 +/- 42 nM (n = 9) at pHi 6.0 in CO2-equilibrated low-calcium medium. Junctional conductance, in most cell pairs, was not substantially reduced by acidification to pHi 5.9-6.0 in low-calcium medium. Cell pairs could still be electrically uncoupled reversibly by the addition of 100 microM octanol, an agent which does not significantly affect Cai. In low-calcium low-sodium medium (choline substitution for all but 13 mM sodium), acidification with CO2 increased Cai to 425 +/- 35 nM (n = 11) at pHi 5.9-6.0 and gj was reduced to near zero. Junctional conductance could also be reduced to near zero at pHi 6.0 in low-calcium medium containing the calcium ionophore, A23187. The addition of the calcium ionophore did not uncouple cell pairs in the absence of acidification. In contrast, acidification did not substantially reduce gj when intracellular calcium was low. Increasing intracellular calcium did not appreciably reduce gj at pHi 7.0. These results suggest that, although other factors may play a role, H+ and Ca++ act synergistically to decrease gj.
机译:当细胞外钙离子活性接近生理水平(添加1.0 mM CaCl2; 470 microM Ca ++)时,通过用CO2进行肌浆酸化,可快速,显着且可逆地降低心肌对心肌细胞之间的间隙连接电导(gj)。通过细胞悬浮液中呋喃2荧光测得的细胞内钙浓度(Cai)为148 +/- 39 nM(+/- SEM,n = 6),而用细胞内离子选择性微电极测得的细胞内pH(pHi)为浸入空气平衡的培养基中的细胞对制剂中的浓度为7.05 +/- 0.02(n = 5)。在用100%CO2平衡的培养基中,Cai增至515 +/- 12 nM(n = 6),pHi降至5.9-6.0。在空气平衡的低钙培养基(未添加CaCl2; 2-5 microM Ca ++)中,Cai在pHi 7.1下为61 +/- 9 nM(n = 13)。在pHi 6.0下,在二氧化碳平衡的低钙培养基中,Cai仅增加到243 +/- 42 nM(n = 9)。在低钙培养基中,通过酸化至pHi 5.9-6.0,在大多数细胞对中,结电导率并没有显着降低。通过添加100 microM辛醇(一种不会显着影响Cai的试剂),仍然可以使细胞对可逆地电解除偶联。在低钙低钠培养基(除13 mM钠以外的所有盐中都用胆碱替代)中,在pH值为5.9-6.0时,用CO2酸化会使Cai升高至425 +/- 35 nM(n = 11),并且gj降低至接近零。在含有钙离子载体A23187的低钙培养基中,pHi 6.0时,结电导也可以降低至接近零。在没有酸化的情况下,添加钙离子载体不会使细胞对解偶联。相反,当细胞内钙含量低时,酸化作用并没有实质性地降低gj。在pHi 7.0下,细胞内钙的增加并没有明显降低gj。这些结果表明,尽管其他因素可能起作用,但H +和Ca ++协同作用以降低gj。

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