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低钾绵羊红细胞中的被动钾离子-氯离子通量:A23187和二价阳离子的调节作用

Passive K+-Cl- fluxes in low-K+ sheep erythrocytes: modulation by A23187 and bivalent cations.

作者信息

Lauf P K

出版信息

Am J Physiol. 1985 Sep;249(3 Pt 1):C271-8. doi: 10.1152/ajpcell.1985.249.3.C271.

Abstract

A fraction of the ouabain-resistant (OR) K+ flux of low-K+ (LK) sheep erythrocytes is Cl- dependent (K+-Cl- transport) and is activated reversibly by cell swelling or irreversibly by treatment with N-ethylmaleimide (NEM). The effect of the ionophore A23187 plus bivalent cations (Me2+) or ethyleneglycol-bis(beta-aminoethylether)-N,N'-tetraacetic acid (EGTA) was studied on K+-Cl- transport in control or NEM-treated LK cells. The following observations were made. 1) A23187 (6 microM), at a hematocrit of 10% (vol/vol) and in the presence of 1 mM EGTA, activated severalfold OR K+-Cl- transport in shrunken or swollen cells but failed to stimulate further K+-Cl- flux in NEM-treated cells. 2) In the absence of EGTA, but at very low external Ca2+ concentrations [( Ca2+]o = 10(-7) M), A23187 stimulated OR K+-Cl- flux in controls less than with EGTA and inhibited it slightly in NEM-treated cells. 3) When [Ca2+]o was raised to 10(-3) M, an almost complete inhibition of OR K+-Cl- fluxes occurred in shrunken, swollen, or NEM-treated cells. 4) Other Me2+ inhibited OR K+-Cl- flux in the presence of A23187 in the following order of decreasing potency: Mn2+ much greater than Ca2+ greater than Mg2+ greater than Sr2+ much much greater than Ba2+. 5) Stimulation of OR K+-Cl- flux by A23187 +/- EGTA and inhibition by A23187 + Ca2+ were reversible and did not alter significantly cellular ATP. 6) The stimulatory effect of A23187 plus EGTA, perhaps by Me2+ removal, on K+-Cl- flux and its inhibition by Ca2+ were reversibly abolished in metabolically depleted cells.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

低钾(LK)绵羊红细胞中一部分哇巴因抗性(OR)钾离子通量是氯离子依赖性的(钾离子-氯离子转运),可通过细胞肿胀可逆性激活,或通过用N-乙基马来酰亚胺(NEM)处理不可逆性激活。研究了离子载体A23187加二价阳离子(Me2+)或乙二醇双(β-氨基乙醚)-N,N'-四乙酸(EGTA)对对照或NEM处理的LK细胞中钾离子-氯离子转运的影响。得到以下观察结果。1)在血细胞比容为10%(体积/体积)且存在1 mM EGTA的情况下,6 μM的A23187可使皱缩或肿胀细胞中的OR钾离子-氯离子转运激活数倍,但未能刺激NEM处理细胞中的钾离子-氯离子通量进一步增加。2)在不存在EGTA但细胞外钙离子浓度极低([Ca2+]o = 10^(-7) M)时,A23187刺激对照细胞中OR钾离子-氯离子通量的程度低于存在EGTA时,且在NEM处理细胞中略有抑制作用。3)当[Ca2+]o升高到10^(-3) M时,皱缩、肿胀或NEM处理细胞中的OR钾离子通量几乎完全受到抑制。4)其他Me2+在存在A23187时抑制OR钾离子-氯离子通量的效力顺序为:锰离子远大于钙离子大于镁离子大于锶离子远大于钡离子。5)A23187 +/- EGTA对OR钾离子-氯离子通量的刺激以及A23187 + Ca2+对其的抑制是可逆的,且未显著改变细胞内ATP。6)A23187加EGTA(可能通过去除Me2+)对钾离子-氯离子通量的刺激作用及其被钙离子的抑制作用在代谢耗竭的细胞中被可逆性消除。(摘要截短至250字)

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