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修改区域洗脱法检测涉及配体交换的瞬时蛋白-蛋白相互作用。

Modification of the zonal elution method for detection of transient protein-protein interactions involving ligand exchange.

机构信息

Department of Chemistry, University of Massachusetts-Amherst, Amherst, Massachusetts 01003, United States.

出版信息

Anal Chem. 2012 May 15;84(10):4608-12. doi: 10.1021/ac300104d. Epub 2012 Apr 25.

Abstract

A new affinity chromatography method was developed by modifying a zonal elution method. The new method targets transient protein-protein interactions, such as those encountered during direct ligand transfer between the ligand transporter and its cognate receptor. A ligand-loaded transport protein is immobilized on the solid support, and a plug containing a putative receptor is flowed through the column. Elution profiles of proteins not interacting with the immobilized transporter can be approximated with a simple Gaussian curve, while the elution profiles of cognate receptors show significant delay and exhibit complex shape. Ligand transfer from the immobilized transporter molecules to the receptors is verified by both UV absorbance measurements and mass spectrometry. The sensitivity of the method is demonstrated using retinoic acid (RA) transfer from various isoforms of cellular RA binding proteins (CRABPs) and RA receptor γ (RARγ). Although these interactions have been hypothesized long ago to proceed via direct mechanism (i.e., via transient docking of the receptor and the transporter), the existing biophysical techniques failed to detect the presence of the transporter-receptor complexes. However, the modified zonal elution method provides unequivocal evidence of direct interaction between RARγ and one of the CRABP isoforms (CRABP II) during the ligand transfer to the receptor.

摘要

一种新的亲和层析方法是通过修改区域洗脱方法开发的。该新方法针对瞬时蛋白-蛋白相互作用,例如在配体转运蛋白与其同源受体之间直接配体转移过程中遇到的相互作用。负载配体的转运蛋白固定在固体载体上,包含假定受体的塞子流过柱子。未与固定转运蛋白相互作用的蛋白质的洗脱曲线可以用简单的高斯曲线近似,而同源受体的洗脱曲线则显示出明显的延迟并呈现复杂的形状。通过 UV 吸收测量和质谱法验证配体从固定转运蛋白分子向受体的转移。该方法的灵敏度通过从各种细胞视黄酸结合蛋白 (CRABP) 和视黄酸受体 γ (RARγ) 的不同异构体中转移视黄酸 (RA) 来证明。尽管这些相互作用很久以前就被假设通过直接机制(即通过受体和转运蛋白的瞬时对接)进行,但现有的生物物理技术未能检测到转运蛋白-受体复合物的存在。然而,改良的区域洗脱方法提供了明确的证据,证明在配体向受体转移过程中,RARγ 与一种 CRABP 异构体(CRABP II)之间存在直接相互作用。

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