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Glycolipid acquisition by human glycolipid transfer protein dramatically alters intrinsic tryptophan fluorescence: insights into glycolipid binding affinity.人糖脂转移蛋白对糖脂的摄取显著改变了色氨酸的固有荧光:对糖脂结合亲和力的见解。
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真菌糖脂转移蛋白(GLTP)异核不亲和性 C2 蛋白(HET-C2)的结构测定和色氨酸荧光为 GLTP 折叠提供了糖脂特异性和膜相互作用的新见解。

Structural determination and tryptophan fluorescence of heterokaryon incompatibility C2 protein (HET-C2), a fungal glycolipid transfer protein (GLTP), provide novel insights into glycolipid specificity and membrane interaction by the GLTP fold.

机构信息

Hormel Institute, University of Minnesota, Austin, Minnesota 55912, USA.

出版信息

J Biol Chem. 2010 Apr 23;285(17):13066-78. doi: 10.1074/jbc.M109.093203. Epub 2010 Feb 17.

DOI:10.1074/jbc.M109.093203
PMID:20164530
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2857133/
Abstract

HET-C2 is a fungal protein that transfers glycosphingolipids between membranes and has limited sequence homology with human glycolipid transfer protein (GLTP). The human GLTP fold is unique among lipid binding/transfer proteins, defining the GLTP superfamily. Herein, GLTP fold formation by HET-C2, its glycolipid transfer specificity, and the functional role(s) of its two Trp residues have been investigated. X-ray diffraction (1.9 A) revealed a GLTP fold with all key sugar headgroup recognition residues (Asp(66), Asn(70), Lys(73), Trp(109), and His(147)) conserved and properly oriented for glycolipid binding. Far-UV CD showed secondary structure dominated by alpha-helices and a cooperative thermal unfolding transition of 49 degrees C, features consistent with a GLTP fold. Environmentally induced optical activity of Trp/Tyr/Phe (2:4:12) detected by near-UV CD was unaffected by membranes containing glycolipid but was slightly altered by membranes lacking glycolipid. Trp fluorescence was maximal at approximately 355 nm and accessible to aqueous quenchers, indicating free exposure to the aqueous milieu and consistent with surface localization of the two Trps. Interaction with membranes lacking glycolipid triggered significant decreases in Trp emission intensity but lesser than decreases induced by membranes containing glycolipid. Binding of glycolipid (confirmed by electrospray injection mass spectrometry) resulted in a blue-shifted emission wavelength maximum (approximately 6 nm) permitting determination of binding affinities. The unique positioning of Trp(208) at the HET-C2 C terminus revealed membrane-induced conformational changes that precede glycolipid uptake, whereas key differences in residues of the sugar headgroup recognition center accounted for altered glycolipid specificity and suggested evolutionary adaptation for the simpler glycosphingolipid compositions of filamentous fungi.

摘要

HET-C2 是一种真菌蛋白,可在膜之间转移糖脂,并与人类糖脂转移蛋白 (GLTP) 具有有限的序列同源性。人类 GLTP 折叠在脂质结合/转移蛋白中是独特的,定义了 GLTP 超家族。在此,研究了 HET-C2 的 GLTP 折叠形成、其糖脂转移特异性以及其两个色氨酸残基的功能作用。X 射线衍射 (1.9 A) 揭示了具有所有关键糖头基识别残基 (Asp(66)、Asn(70)、Lys(73)、Trp(109)和 His(147)) 的 GLTP 折叠,这些残基被正确定向以结合糖脂。远紫外线 CD 显示以 alpha-螺旋为主的二级结构和 49 摄氏度的协同热变性过渡,这些特征与 GLTP 折叠一致。近紫外线 CD 检测到的色氨酸/酪氨酸/苯丙氨酸 (2:4:12) 的环境诱导旋光性不受含有糖脂的膜影响,但受缺乏糖脂的膜轻微影响。色氨酸荧光在约 355nm 处最大,并可被水性淬灭剂淬灭,表明其自由暴露于水性环境中,与两个色氨酸的表面定位一致。与缺乏糖脂的膜相互作用会导致色氨酸发射强度显着降低,但低于含有糖脂的膜引起的降低。糖脂的结合 (通过电喷雾注入质谱证实) 导致发射波长最大值蓝移 (约 6nm),从而可以确定结合亲和力。色氨酸 (208) 在 HET-C2 C 末端的独特定位揭示了膜诱导的构象变化,该变化先于糖脂摄取,而糖头基识别中心的关键残基差异解释了糖脂特异性的改变,并表明了对丝状真菌更简单的糖脂组成的进化适应。