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通过红外反射吸收光谱法(IRRAS)研究脂化Ras蛋白插入脂质单分子层的情况。

Insertion of lipidated Ras proteins into lipid monolayers studied by infrared reflection absorption spectroscopy (IRRAS).

作者信息

Meister Annette, Nicolini Chiara, Waldmann Herbert, Kuhlmann Jürgen, Kerth Andreas, Winter Roland, Blume Alfred

机构信息

Institut für Physikalische Chemie, Martin-Luther-Universität Halle-Wittenberg, Halle, Germany.

出版信息

Biophys J. 2006 Aug 15;91(4):1388-401. doi: 10.1529/biophysj.106.084624. Epub 2006 May 26.

Abstract

Ras proteins have to be associated with the inner leaflet of the plasma membrane to perform their signaling functions. This membrane targeting and binding is controlled by post-translational covalent attachment of farnesyl and palmitoyl chains to cysteines in the membrane anchor region of the N- and H-Ras isoforms. Two N-Ras lipoproteins were investigated, namely a farnesylated and hexadecylated protein, presenting the natural hydrophobic modifications and a doubly hexadecylated construct, respectively. The proteins are surface active and form a Gibbs monolayer at the air-D2O interface. The contours of the amide-I bands were analyzed using infrared reflection absorption spectroscopy (IRRAS). Langmuir monolayers of a mixture of POPC, brain sphingomyelin, and cholesterol were used as half of a model biomembrane to study the insertion of these N-Ras proteins. They insert with their hydrophobic anchors into lipid monolayers but at higher surface pressures (30 mN/m); the farnesylated and hexadecylated protein desorbs completely from the monolayer, whereas the doubly hexadecylated protein remains incorporated. During the insertion process, changes in the orientation of the protein secondary structure were detected by comparison with simulated IRRA spectra, based on the information on the relative orientation of the secondary structure elements from the protein crystal structure data.

摘要

Ras蛋白必须与质膜的内小叶相关联才能发挥其信号传导功能。这种膜靶向和结合是由法尼基和棕榈酰链在N-Ras和H-Ras亚型的膜锚定区域内与半胱氨酸进行翻译后共价连接所控制的。研究了两种N-Ras脂蛋白,即一种法尼基化和十六烷基化的蛋白,分别呈现天然的疏水修饰和一种双十六烷基化构建体。这些蛋白具有表面活性,并且在空气-D2O界面形成吉布斯单层。使用红外反射吸收光谱(IRRAS)分析酰胺-I带的轮廓。将POPC、脑鞘磷脂和胆固醇混合物的朗缪尔单层用作模型生物膜的一半,以研究这些N-Ras蛋白的插入情况。它们通过疏水锚定插入脂质单层,但在较高表面压力(30 mN/m)下;法尼基化和十六烷基化的蛋白会完全从单层中解吸,而双十六烷基化的蛋白仍会结合在其中。在插入过程中,基于蛋白质晶体结构数据中二级结构元件的相对取向信息,通过与模拟的IRRA光谱进行比较,检测到蛋白质二级结构取向的变化。

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