大鼠脑阿片受体分子的增溶纯化。

Y C Jin, C Y Ye, Y Li, C L Suo, L Y Li, M Q Liu, X M Jin, Z M Mao
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引用次数: 0

摘要

将不含小脑的大鼠脑P2膜制备物与CHAPS溶解于含有DTT和胰蛋白酶抑制剂的Tris中。用Liu等制备的两种阿片配体10b和10cd连续进行亲和层析,其中OPR用Nx洗脱。洗脱液随后通过WGA亲和柱,OPR用N-GluNAc洗脱。通过制备颗粒凝胶等电聚焦SG200对该洗脱液进行进一步纯化和浓缩。pH值为5和7.8时分别出现两个蛋白峰。用银染色法检测两峰洗脱液的蛋白质含量,用3H-etor的RRA法测定其结合活性。结果表明,两种样品均含有活性OPR,纯化倍数均在8万倍以上。通过凝胶过滤估计,OPR在pH 5和pH 7.8样品中的Mr分别为52 kD和42 kD。通过与3H-ohm的结合活性,确定pH 5样品中的OPR为mu型。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Solubilization and purification of opioid receptor molecules of rat brain.

A P2 membrane preparation of rat brain (without cerebellum) was solubilized with CHAPS in Tris containing DTT and trypsin inhibitor. Two opiate ligands, 10b and 10cd, prepared by Liu et al, were employed consecutively in affinity chromatography, from which OPR's were eluted with Nx. The eluate was subsequently passed through a WGA affinity column and the OPR's eluted with N-GluNAc. This eluate was further purified and concentrated by preparative granular gel isoelectric focusing on SG200. Two protein peaks appeared separately at pH 5 and 7.8. The eluates from both peaks were examined for protein contents using the silver staining method, and binding activity was measured by RRA with 3H-etor. The results revealed that both samples contained active OPR purified to over 80,000 fold. The Mr was estimated by gel filtration to be 52 kD and 42 kD for OPR in the pH 5 and pH 7.8 samples respectively. OPR in the pH 5 sample have been determined to be of mu-type by their binding activity with 3H-ohm.

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