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与非P-糖蛋白多药耐药相关的MRP基因编码一种190 kDa的膜结合糖蛋白。

The MRP gene associated with a non-P-glycoprotein multidrug resistance encodes a 190-kDa membrane bound glycoprotein.

作者信息

Krishnamachary N, Center M S

机构信息

Division of Biology, Kansas State University, Manhattan 66506.

出版信息

Cancer Res. 1993 Aug 15;53(16):3658-61.

PMID:8101765
Abstract

HL60 cells isolated for resistance to Adriamycin (HL60/ADR) overexpress a 190-kDa ATP binding protein which has a minor sequence homology with P-glycoprotein. It has also been observed that HL60/ADR overexpress the MRP gene which was first identified as a component of a non-P-glycoprotein mediated multidrug resistance of H69/ADR cells [Cole et al., Science (Washington DC), 258: 1650, 1992]. A complementary DNA of MRP has been cloned and based on the deduced sequence encodes a member of the superfamily of proteins which bind ATP and function in various transport processes [Cole et al., Science (Washington DC), 258: 1650, 1992]. In view of this it was of interest to identify the protein encoded by MRP and determine if it may be related to p190. In the present study we have prepared antisera against three synthetic peptides which correspond to the deduced sequence of the MRP protein. Proteins reactive with the antisera have been examined in HL60/ADR cells using Western blot analysis. All antisera react with a 190 kDa protein contained in membranes of resistant but not sensitive cells. One antiserum used for further studies is not reactive with P-glycoprotein contained in membranes of HL60 cells isolated for resistance to vincristine. Analysis of subcellular fractions demonstrates that p190 is present primarily in the endoplasmic reticulum with lower levels also present in plasma membranes. Treatment of HL60/ADR cells with tunicamycin results in the appearance of a 165-kDa resistance associated protein which reacts with the antipeptide serum. The results of this study therefore demonstrate that the MRP gene encodes a 190-kDa membrane bound glycoprotein.

摘要

为对阿霉素产生抗性而分离出的HL60细胞(HL60/ADR)过表达一种190 kDa的ATP结合蛋白,该蛋白与P-糖蛋白有微小的序列同源性。还观察到HL60/ADR过表达MRP基因,该基因最初被鉴定为H69/ADR细胞非P-糖蛋白介导的多药耐药性的一个组成部分[科尔等人,《科学》(华盛顿特区),258: 1650,1992]。MRP的互补DNA已被克隆,根据推导序列编码一个蛋白质超家族的成员,该超家族的蛋白质结合ATP并在各种转运过程中起作用[科尔等人,《科学》(华盛顿特区),258: 1650,1992]。鉴于此,确定MRP编码的蛋白质并确定其是否可能与p190相关是很有意义的。在本研究中,我们制备了针对三种合成肽的抗血清,这些肽对应于MRP蛋白的推导序列。使用蛋白质印迹分析在HL60/ADR细胞中检测了与抗血清反应的蛋白质。所有抗血清都与耐药细胞而非敏感细胞的膜中所含的190 kDa蛋白质发生反应。用于进一步研究的一种抗血清与为对长春新碱产生抗性而分离出的HL60细胞的膜中所含的P-糖蛋白不发生反应。亚细胞组分分析表明,p190主要存在于内质网中,质膜中也有较低水平的存在。用衣霉素处理HL60/ADR细胞会导致出现一种与抗肽血清反应的165 kDa抗性相关蛋白。因此,本研究结果表明,MRP基因编码一种190 kDa的膜结合糖蛋白。

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