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一种用于透明质酸盐的蛋白质结合测定法。

A protein binding assay for hyaluronate.

作者信息

Lacy B E, Underhill C B

出版信息

Anal Biochem. 1986 Nov 1;158(2):436-42. doi: 10.1016/0003-2697(86)90572-5.

Abstract

A relatively quick and simple assay for hyaluronate was developed using the specific binding protein, hyaluronectin. The hyaluronection was obtained by homogenizing the brains of Sprague-Dawley rats, and then centrifuging the homogenate. The resulting supernatant was used as a source of crude hyaluronectin. In the binding assay, the hyaluronectin was mixed with [3H]hyaluronate, followed by an equal volume of saturated (NH4)2SO4, which precipitated the hyaluronectin and any [3H]hyaluronate associated with it, but left free [3H]hyaluronate in solution. The mixture was then centrifuged, and the amount of bound [3H]hyaluronate in the precipitate was determined. Using this assay, we found that hyaluronectin specifically bound hyaluronate, since other glycosaminoglycans failed to compete for the binding protein. In addition, the interaction between hyaluronectin and hyaluronate was of relatively high affinity (Kd = 5.7 X 10(-10) M), and the size of the hyaluronate did not appear to substantially alter the amount of binding. To determine the amount of hyaluronate in an unknown sample, we used a competition assay in which the binding of a set amount of [3H]hyaluronate was blocked by the addition of unlabeled hyaluronate. By comparing the degree of competition of the unknown samples with that of known amounts of hyaluronate, it was possible to determine the amount of hyaluronate in the unknowns. We have found that this method is sensitive to 1 microgram or less of hyaluronate, and is unaffected by the presence of proteins.

摘要

利用特异性结合蛋白透明质酸结合素,开发了一种相对快速简便的透明质酸盐检测方法。通过将斯普拉格-道利大鼠的大脑匀浆,然后对匀浆进行离心,获得透明质酸结合素。所得上清液用作粗制透明质酸结合素的来源。在结合试验中,将透明质酸结合素与[3H]透明质酸盐混合,随后加入等体积的饱和硫酸铵,硫酸铵会沉淀透明质酸结合素及其相关的任何[3H]透明质酸盐,但溶液中会留下游离的[3H]透明质酸盐。然后将混合物离心,测定沉淀中结合的[3H]透明质酸盐的量。使用该检测方法,我们发现透明质酸结合素能特异性结合透明质酸盐,因为其他糖胺聚糖无法竞争结合蛋白。此外,透明质酸结合素与透明质酸盐之间的相互作用具有相对较高的亲和力(解离常数Kd = 5.7×10⁻¹⁰ M),并且透明质酸盐的大小似乎不会显著改变结合量。为了测定未知样品中透明质酸盐的量,我们使用了一种竞争试验,即通过加入未标记的透明质酸盐来阻断一定量的[3H]透明质酸盐的结合。通过比较未知样品与已知量透明质酸盐的竞争程度,可以确定未知样品中透明质酸盐的量。我们发现该方法对1微克或更少的透明质酸盐敏感,并且不受蛋白质存在的影响。

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