Quantitative approach for detection and characterization of formyl peptide receptor in solution using a photoaffinity ligand.

Peptide research Pub Date : 1996-03-01
A Lala, H T Sojar, E De Nardin
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Abstract

In this paper we describe an assay method for the rapid detection and quantitation of human neutrophil FMLP (N-formyl-methionyl-leucyl-phenylalanine) receptor molecules. Although different assay methods are available to detect the receptor, none are rapid and at the same time allow quantitative detection of the binding affinity of the receptor molecule in solution. In our modified method, following a binding reaction using photoaffinity ligand, the amount of labeled ligand bound to the receptor is separated from the unbound one, thereby determining the binding affinity of the receptor protein. This simple procedure not only makes it possible to detect the recombinant FMLP receptor protein very rapidly, but also provides quantitative assessment of binding. This technique therefore allows a partial characterization (identification, determination of size and assessment of binding affinity) of receptor molecule in solution in less than 24 hours.

利用光亲和配体在溶液中检测和表征甲酰基肽受体的定量方法。
本文描述了一种快速检测和定量人中性粒细胞FMLP (n -甲酰基-甲硫基-亮基-苯丙氨酸)受体分子的方法。虽然有不同的检测方法可用于检测受体,但没有一种方法是快速的,同时可以定量检测溶液中受体分子的结合亲和力。在我们改进的方法中,使用光亲和配体进行结合反应后,与受体结合的标记配体的数量从未结合的配体中分离出来,从而确定受体蛋白的结合亲和力。这一简单的方法不仅可以非常快速地检测重组FMLP受体蛋白,而且可以提供结合的定量评估。因此,该技术可以在不到24小时内对溶液中的受体分子进行部分表征(鉴定、确定大小和评估结合亲和力)。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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