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肝小管质膜囊泡中的钠-甘氨酸共转运

Na+-glycine cotransport in canalicular liver plasma membrane vesicles.

作者信息

Moseley R H, Ballatori N, Murphy S M

机构信息

Department of Internal Medicine, Veterans Administration Medical Center, Ann Arbor, Michigan.

出版信息

Am J Physiol. 1988 Aug;255(2 Pt 1):G253-9. doi: 10.1152/ajpgi.1988.255.2.G253.

DOI:10.1152/ajpgi.1988.255.2.G253
PMID:3407780
Abstract

By use of purified rat canalicular liver plasma membrane (cLPM) vesicles, the present study determined the driving forces for glycine transport across this membrane domain. Initial rates of [3H]glycine uptake (10 microM) in cLPM vesicles were stimulated by an inwardly directed Na+ gradient but not by a K+ gradient. Na+ gradient-dependent uptake of glycine demonstrated cation specificity for Na+, dependence on extravesicular Cl-, stimulation by an intravesicular-negative membrane potential, and inhibition by dissipation of the Na+ gradient with gramicidin D. Na+ gradient-dependent glycine cotransport also demonstrated greater sensitivity to inhibition by sarcosine than 2-(methylamino)-isobutyric acid. Accelerated exchange diffusion of [3H]glycine was demonstrated in the presence of Na+ when cLPM vesicles were preloaded with glycine but not with L-alanine or L-proline. Substrate velocity analysis of net Na+-dependent [3H]glycine uptake over the range of amino acid concentrations from 5 microM to 5 mM demonstrated two saturable transport systems, one of high capacity (2.2 +/- 0.2 nmol.mg protein-1.15 s-1) and low affinity (11.2 +/- 1.7 mM) and one of low capacity (51 +/- 14 pmol.mg protein.15 s-1) and comparatively high affinity (66 +/- 12 microM). These results indicate that, in addition to previously described neutral and anionic amino acid transport systems, Na+ gradient-dependent glycine transport mechanisms are present on the canalicular domain of the liver plasma membrane. These canalicular reabsorptive mechanisms may serve to reclaim some of the glycine generated within the canalicular lumen from the intrabiliary hydrolysis of glutathione.

摘要

本研究利用纯化的大鼠肝小管质膜(cLPM)囊泡,确定了甘氨酸跨该膜结构域转运的驱动力。cLPM囊泡中[3H]甘氨酸摄取(10微摩尔)的初始速率受内向Na+梯度刺激,但不受K+梯度刺激。甘氨酸的Na+梯度依赖性摄取表现出对Na+的阳离子特异性、对囊泡外Cl-的依赖性、受囊泡内负膜电位刺激以及被短杆菌肽D消除Na+梯度所抑制。Na+梯度依赖性甘氨酸共转运对肌氨酸抑制的敏感性也高于对2-(甲基氨基)异丁酸的敏感性。当cLPM囊泡预先加载甘氨酸而非L-丙氨酸或L-脯氨酸时,在存在Na+的情况下证明了[3H]甘氨酸的加速交换扩散。在5微摩尔至5毫摩尔氨基酸浓度范围内对净Na+依赖性[3H]甘氨酸摄取进行底物速度分析,结果表明存在两个可饱和转运系统,一个高容量(2.2±0.2纳摩尔·毫克蛋白-1·15秒-1)、低亲和力(11.2±1.7毫摩尔),另一个低容量(51±14皮摩尔·毫克蛋白·15秒-1)、相对高亲和力(66±12微摩尔)。这些结果表明,除了先前描述的中性和阴离子氨基酸转运系统外,肝质膜小管结构域存在Na+梯度依赖性甘氨酸转运机制。这些小管重吸收机制可能有助于从谷胱甘肽的胆管内水解产物中回收一些在胆管腔内产生的甘氨酸。

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