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一种基于过滤的检测方法,用于定量粒细胞-巨噬细胞集落刺激因子结合。

A filtration-based assay to quantitate granulocyte-macrophage colony-stimulating factor binding.

作者信息

Scott C W, Gomes B C, Hubbs S J, Koenigbauer H C

机构信息

Pharmacology Department, Zeneca Pharmaceuticals, Wilmington, Delaware 19897, USA.

出版信息

Anal Biochem. 1995 Jun 10;228(1):150-4. doi: 10.1006/abio.1995.1326.

Abstract

Filtration-based binding assays have numerous advantages over centrifugation-based assays, yet they have not been established for many protein ligands due to the high nonspecific binding of the protein to the membrane filter. This paper describes a vacuum filtration method that permits quantitative evaluation of [125I]GM-CSF binding to its receptor on intact cells. The method includes the use of glass fiber filters presoaked in a solution of polyvinylpyrrolidone and Tween 20 to greatly reduce nonspecific binding of the protein ligand. The ratio of specific:nonspecific binding observed with this filtration assay was comparable to values reported for centrifugation assays. [125I] GM-CSF binding to HL-60 cells was shown to be time-dependent, saturable, and specific. The estimated Kd (70 pM) and Bmax (160 r/cell) were similar to values reported using centrifugation assays. This filtration method is much less labor-intensive, has greater sample throughput, and allows for a more rapid determination of GM-CSF binding compared to the centrifugation-based assay. Although developed to quantitate the binding of GM-CSF to its receptor on intact cells, this assay is also applicable to other cytokines and can be used with both intact cells and isolated plasma membrane preparations.

摘要

基于过滤的结合测定法相对于基于离心的测定法具有众多优势,但由于蛋白质与膜过滤器的非特异性结合较高,许多蛋白质配体尚未建立该方法。本文描述了一种真空过滤方法,该方法允许对完整细胞上[125I]GM-CSF与其受体的结合进行定量评估。该方法包括使用预先浸泡在聚乙烯吡咯烷酮和吐温20溶液中的玻璃纤维过滤器,以大大减少蛋白质配体的非特异性结合。用这种过滤测定法观察到的特异性:非特异性结合比率与离心测定法报道的值相当。[125I]GM-CSF与HL-60细胞的结合显示出时间依赖性、饱和性和特异性。估计的Kd(70 pM)和Bmax(160 r/细胞)与使用离心测定法报道的值相似。与基于离心的测定法相比,这种过滤方法劳动强度小得多,样品通量更大,并且能够更快地测定GM-CSF结合。尽管该方法是为了定量GM-CSF与完整细胞上其受体的结合而开发的,但该测定法也适用于其他细胞因子,并且可用于完整细胞和分离的质膜制剂。

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