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红细胞膜蛋白中自由翻转的棕榈酸酯并不负责脂筏与血影蛋白骨架的锚定:一项使用生物正交化学探针的研究。

Freely turning over palmitate in erythrocyte membrane proteins is not responsible for the anchoring of lipid rafts to the spectrin skeleton: a study with bio-orthogonal chemical probes.

作者信息

Ciana Annarita, Achilli Cesare, Hannoush Rami N, Risso Angela, Balduini Cesare, Minetti Giampaolo

机构信息

University of Pavia, Department of Biology and Biotechnology, Pavia, Italy.

出版信息

Biochim Biophys Acta. 2013 Mar;1828(3):924-31. doi: 10.1016/j.bbamem.2012.11.029. Epub 2012 Dec 3.

Abstract

Erythrocyte lipid rafts are anchored to the underlying spectrin membrane skeleton [A. Ciana, C. Achilli, C. Balduini, G. Minetti, On the association of lipid rafts to the spectrin skeleton in human erythrocytes, Biochim. Biophys. Acta 1808 (2011) 183-190]. The nature of this linkage and the molecules involved are poorly understood. The interaction is sensitive to the increase in pH and ionic strength induced by carbonate. Given the role of palmitoylation in modulating the partitioning of certain proteins between various sub-cellular compartments and the plasma membrane, we asked whether palmitoylation of p55, a peripheral protein located at the junctional complex between spectrin-actin-protein 4.1 that anchors the membrane skeleton to the lipid bilayer via the transmembrane protein glycophorin C, could contribute to the anchoring of lipid rafts to the membrane skeleton. We adopted a new, non-radioactive method for studying protein palmitoylation, based on bio-orthogonal chemical analogues of fatty acids, containing an omega-alkynyl group, to metabolically label cell proteins, which are then revealed by a "click chemistry" reaction of the alkynyl moiety with an azide-containing reporter tag. We show that the membrane localization and palmitoylation levels of p55 did not change after carbonate treatment. 2-bromopalmitate and cerulenin, two known palmitoylation inhibitors, completely inhibited p55 palmitoylation, and protein palmitoyl thioesterase-1 (PPT1) reduced it, without affecting the association between lipid rafts and membrane-skeleton, indicating, on the one hand, that p55 palmitoylation is enzymatic, and, on the other, that it is not involved in the modulation of the linkage of lipid rafts to the membrane-skeleton.

摘要

红细胞脂筏锚定在其下方的血影蛋白膜骨架上[A. 恰纳、C. 阿基利、C. 巴尔杜伊尼、G. 米内蒂,《关于人红细胞中脂筏与血影蛋白骨架的关联》,《生物化学与生物物理学报》1808 (2011) 183 - 190]。这种连接的本质以及所涉及的分子尚不清楚。这种相互作用对碳酸盐诱导的pH值和离子强度增加敏感。鉴于棕榈酰化在调节某些蛋白质在不同亚细胞区室和质膜之间的分配中的作用,我们询问位于血影蛋白 - 肌动蛋白 - 蛋白4.1连接复合体处的外周蛋白p55的棕榈酰化是否有助于脂筏与膜骨架的锚定,血影蛋白 - 肌动蛋白 - 蛋白4.1通过跨膜蛋白血型糖蛋白C将膜骨架锚定到脂质双层。我们采用了一种新的非放射性方法来研究蛋白质棕榈酰化,该方法基于脂肪酸的生物正交化学类似物,含有一个ω - 炔基,用于代谢标记细胞蛋白,然后通过炔基部分与含叠氮化物的报告标签的“点击化学”反应来揭示这些蛋白。我们表明,碳酸盐处理后p55的膜定位和棕榈酰化水平没有变化。两种已知的棕榈酰化抑制剂2 - 溴棕榈酸酯和浅蓝菌素完全抑制了p55的棕榈酰化,而蛋白棕榈酰硫酯酶 - 1 (PPT1) 降低了它的棕榈酰化,且不影响脂筏与膜骨架之间的关联,这一方面表明p55的棕榈酰化是酶促反应,另一方面表明它不参与脂筏与膜骨架连接的调节。

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