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一种用于缺氧诱导因子脯氨酰羟化酶的基于荧光偏振的相互作用检测方法。

A fluorescence polarization-based interaction assay for hypoxia-inducible factor prolyl hydroxylases.

作者信息

Cho Hyunju, Park Hyunsung, Yang Eun Gyeong

机构信息

Life Sciences Division, Korea Institute of Science and Technology, Seoul, Republic of Korea.

出版信息

Biochem Biophys Res Commun. 2005 Nov 11;337(1):275-80. doi: 10.1016/j.bbrc.2005.09.041.

Abstract

Oxygen-dependent ubiquitination and degradation of hypoxia-inducible factor 1alpha (HIF-1alpha) plays a central role in regulating transcriptional responses to hypoxia. This process requires hydroxylation of specific prolines in HIF-1alpha by HIF prolyl hydroxylase domain (PHD)-containing enzymes, leading to its specific interactions with von Hippel-Lindau protein-Elongin B-Elongin C (VBC). Here we describe a straightforward approach to apply these interactions to measure PHD activities. Employing fluorescently labeled HIF-1alpha peptides containing hydroxyproline, we developed a quantitative method based on fluorescence polarization for a systematic evaluation of binding of hydroxylated HIF-1alpha to recombinant VBC. The method was then successfully utilized for measuring the activity of the truncated, purified PHD2. The applicability of the assay was further demonstrated by examining effects of various cofactors and inhibitors for PHD2. The developed homogeneous assay would provide a convenient way of probing the biochemical properties of the HIF-1alpha-VBC interaction and PHDs, and of screening modulators for the interaction as well as the enzyme.

摘要

缺氧诱导因子1α(HIF-1α)的氧依赖性泛素化和降解在调节对缺氧的转录反应中起核心作用。该过程需要含HIF脯氨酰羟化酶结构域(PHD)的酶对HIF-1α中的特定脯氨酸进行羟基化,从而导致其与冯·希佩尔-林道蛋白-Elongin B-Elongin C(VBC)发生特异性相互作用。在此,我们描述了一种直接的方法,利用这些相互作用来测量PHD活性。我们使用含有羟脯氨酸的荧光标记HIF-1α肽,开发了一种基于荧光偏振的定量方法,用于系统评估羟基化HIF-1α与重组VBC的结合。该方法随后成功用于测量截短的纯化PHD2的活性。通过检查各种辅因子和PHD2抑制剂的作用,进一步证明了该测定法的适用性。所开发的均相测定法将为探究HIF-1α-VBC相互作用和PHD的生化特性、筛选该相互作用以及该酶的调节剂提供一种便捷的方法。

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