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静止和增殖状态的人及大鼠胸腺淋巴细胞的细胞内pH值

The intracellular pH of quiescent and proliferating human and rat thymic lymphocytes.

作者信息

Grinstein S, Cohen S, Lederman H M, Gelfand E W

出版信息

J Cell Physiol. 1984 Oct;121(1):87-95. doi: 10.1002/jcp.1041210112.

Abstract

We compared the cytoplasmic pH (pHi) of quiescent and actively cycling thymic lymphocytes. Human and rat thymocyte suspensions were fractionated by centrifugation on one-step albumin density gradients. The pellet was composed of small, quiescent cells and the interphase contained mostly larger, actively cycling cells with a high proliferation index. When measured using [14C]-dimethyloxazolidinedione (DMO), pHi in the large cells of both species was approximately 0.15 units more alkaline than in the small cells. However, these differences were not detectable when pHi was measured with carboxylated fluorescein derivatives generated in situ by cytoplasmic enzymes. This apparent discrepancy can be explained by compartmentation of DMO, which accumulates in the alkaline mitochondrial matrix. Comparison of the mitochondrial content of quiescent and cycling thymocytes by several methods showed that the latter contained over 2.5-fold more mitochondria per unit cell volume. Assuming a constant intramitochondrial pH, this difference can account for the observed accumulation of DMO (i.e., apparent cytoplasmic alkalinity) in the actively proliferating cells. Therefore, no evidence was found for the existence of differences in pHi between quiescent and proliferating lymphocytes. Moreover, caution must be exercised when comparing DMO partition data in cells with varying relative mitochondrial content.

摘要

我们比较了静止和活跃循环的胸腺淋巴细胞的细胞质pH(pHi)。人及大鼠胸腺细胞悬液通过在一步白蛋白密度梯度上离心进行分级分离。沉淀由小的静止细胞组成,而界面相中大多是较大的、具有高增殖指数的活跃循环细胞。当使用[14C]-二甲基恶唑烷二酮(DMO)进行测量时,两种物种的大细胞中的pHi比小细胞中的碱性约高0.15个单位。然而,当用细胞质酶原位生成的羧化荧光素衍生物测量pHi时,这些差异无法检测到。这种明显的差异可以用DMO的区室化来解释,DMO积累在线粒体碱性基质中。通过几种方法对静止和循环胸腺细胞的线粒体含量进行比较,结果表明,后者每单位细胞体积所含的线粒体比前者多2.5倍以上。假设线粒体内pH恒定,这种差异可以解释在活跃增殖细胞中观察到的DMO积累(即明显的细胞质碱化)。因此,未发现静止淋巴细胞和增殖淋巴细胞之间存在pHi差异的证据。此外,在比较线粒体相对含量不同的细胞中的DMO分配数据时必须谨慎。

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