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底物诱导非洲爪蟾卵母细胞中表达的肽转运体PEPT1密度的变化。

Substrate-induced changes in the density of peptide transporter PEPT1 expressed in Xenopus oocytes.

作者信息

Mertl Manuela, Daniel Hannelore, Kottra Gabor

机构信息

Molecular Nutrition Unit, Am Forum 5, Freising 85350, Germany.

出版信息

Am J Physiol Cell Physiol. 2008 Nov;295(5):C1332-43. doi: 10.1152/ajpcell.00241.2008. Epub 2008 Sep 17.

DOI:10.1152/ajpcell.00241.2008
PMID:18799652
Abstract

The adaptation of the capacity of the intestinal peptide transporter PEPT1 to varying substrate concentrations may be important with respect to its role in providing bulk quantities of amino acids for growth, development, and other nutritional needs. In the present study, we describe a novel phenomenon of the regulation of PEPT1 in the Xenopus oocyte system. Using electrophysiological and immunofluorescence methods, we demonstrate that a prolonged substrate exposure of rabbit PEPT1 (rPEPT1) caused a retrieval of transporters from the membrane. Capacitance as a measure of membrane surface area was increased in parallel with the increase in rPEPT1-mediated transport currents with a slope of approximately 5% of basal surface per 100 nA. Exposure of oocytes to the model peptide Gly-l-Gln for 2 h resulted in a decrease in maximal transport currents with no change of membrane capacitance. However, exposure to substrate for 5 h decreased transport currents but also, in parallel, surface area by endocytotic removal of transporter proteins from the surface. The reduction of the surface expression of rPEPT1 was confirmed by presteady-state current measurements and immunofluorescent labeling of rPEPT1. A similar simultaneous decrease of current and surface area was also observed when endocytosis was stimulated by the activation of PKC. Cytochalasin D inhibited all changes evoked by either dipeptide or PKC stimulation, whereas the PKC-selective inhibitor bisindolylmaleimide only affected PKC-stimulated endocytotic processes but not substrate-dependent retrieval of rPEPT1. Coexpression experiments with human Na(+)-glucose transporter 1 (hSGLT1) revealed that substrate exposure selectively affected PEPT1 but not the activity of hSGLT1.

摘要

肠道肽转运体PEPT1对不同底物浓度的适应性,对于其在为生长、发育及其他营养需求提供大量氨基酸方面所起的作用而言,可能至关重要。在本研究中,我们描述了非洲爪蟾卵母细胞系统中PEPT1调控的一种新现象。运用电生理和免疫荧光方法,我们证明兔PEPT1(rPEPT1)长时间暴露于底物会导致转运体从膜上回收。作为膜表面积衡量指标的电容,与rPEPT1介导的转运电流增加呈平行增加,斜率约为每100 nA基础表面积的5%。将卵母细胞暴露于模型肽Gly-l-Gln 2小时,导致最大转运电流降低,而膜电容无变化。然而,暴露于底物5小时会降低转运电流,同时也会通过从表面内吞去除转运蛋白而使表面积减小。rPEPT1表面表达的降低通过稳态前电流测量和rPEPT1的免疫荧光标记得以证实。当通过PKC激活刺激内吞作用时,也观察到电流和表面积类似的同时降低。细胞松弛素D抑制了由二肽或PKC刺激引起的所有变化,而PKC选择性抑制剂双吲哚马来酰亚胺仅影响PKC刺激的内吞过程,而不影响rPEPT1的底物依赖性回收。与人钠葡萄糖转运体1(hSGLT1)的共表达实验表明,底物暴露选择性地影响PEPT1,而不影响hSGLT1的活性。

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