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渗透压诱导的体积变化和细胞质酸化对淋巴细胞中Na+/H+交换的激活作用。

Activation of Na+/H+ exchange in lymphocytes by osmotically induced volume changes and by cytoplasmic acidification.

作者信息

Grinstein S, Clarke C A, Rothstein A

出版信息

J Gen Physiol. 1983 Nov;82(5):619-38. doi: 10.1085/jgp.82.5.619.

Abstract

After swelling in hypotonic solutions, peripheral blood mononuclear cells (PBM) shrink toward their original volumes. Upon restoration of isotonicity, the cells initially shrink but then regain near-normal size again. This regulatory volume increase (RVI) is abolished by removal of Na+o or Cl-o or by addition of amiloride. RVI is unaffected by removal of K+o or by ouabain and is only partially inhibited by 1 mM furosemide. As a result of increased influx, the cells gain both Na+ and K+ during reswelling. In contrast, only Na+ content increases in the presence of ouabain. Amiloride largely eliminates the changes in the content of both cations. Using diS-C3-(5), no significant membrane potential changes were detected during RVI, which suggests that the fluxes are electroneutral. The cytoplasmic pH of volume-static cells was measured with 5,6-dicarboxyfluorescein. After acid loading, the addition of extracellular Na+ induced an amiloride-inhibitable alkalinization, which is consistent with Na+/H+ exchange. Cytoplasmic pH was not affected by cell shrinkage itself, but an internal alkalinization, which was also amiloride sensitive and Na+ dependent, developed during reswelling. In isotonic lightly buffered solutions without HCO-3, an amiloride-sensitive acidification of the medium was measurable when Na+ was added to shrunken PBM. K+ was unable to mimic this effect. The observations are compatible with the model proposed by Cala (J. Gen. Physiol. 1980. 76:683-708), whereby an electroneutral Na+o/H+i exchange is activated by osmotic shrinking. Cellular volume gain occurs as Cl-o simultaneously exchanges for either HCO-3i or OH-i. Na+i is secondarily replaced by K+ through the pump, but this step is not essential for RVI.

摘要

在低渗溶液中肿胀后,外周血单核细胞(PBM)会朝着其原始体积收缩。等渗性恢复后,细胞最初会收缩,但随后又会再次恢复到接近正常的大小。这种调节性容积增加(RVI)可通过去除细胞外Na⁺或Cl⁻或添加氨氯吡咪而被消除。去除细胞外K⁺或使用哇巴因对RVI没有影响,而1 mM呋塞米仅部分抑制RVI。由于流入增加,细胞在再膨胀过程中同时获得Na⁺和K⁺。相比之下,在存在哇巴因的情况下,只有Na⁺含量增加。氨氯吡咪在很大程度上消除了两种阳离子含量的变化。使用二硫代-C3-(5),在RVI过程中未检测到明显的膜电位变化,这表明离子通量是电中性的。用5,6-二羧基荧光素测量体积稳定细胞的细胞质pH。酸负荷后,添加细胞外Na⁺会诱导氨氯吡咪可抑制的碱化,这与Na⁺/H⁺交换一致。细胞质pH不受细胞自身收缩的影响,但在再膨胀过程中会出现一种同样对氨氯吡咪敏感且依赖于Na⁺的内部碱化。在没有HCO₃⁻的等渗轻度缓冲溶液中,当向收缩的PBM中添加Na⁺时,可测量到培养基中氨氯吡咪敏感的酸化。K⁺无法模拟这种效应。这些观察结果与Cala提出的模型(《普通生理学杂志》1980年。76:683 - 708)一致,即通过渗透收缩激活电中性的细胞外Na⁺/细胞内H⁺交换。细胞容积增加是因为Cl⁻同时与HCO₃⁻i或OH⁻i进行交换。Na⁺i随后通过泵被K⁺取代,但这一步骤对于RVI不是必需的。

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