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一种作用于H-Ras蛋白和C末端N-Ras肽段的蛋白质棕榈酰转移酶的纯化

Purification of a protein palmitoyltransferase that acts on H-Ras protein and on a C-terminal N-Ras peptide.

作者信息

Liu L, Dudler T, Gelb M H

机构信息

Department of Chemistry, University of Washington, Seattle, Washington 98195-1700, USA.

出版信息

J Biol Chem. 1996 Sep 20;271(38):23269-76. doi: 10.1074/jbc.271.38.23269.

DOI:10.1074/jbc.271.38.23269
PMID:8798525
Abstract

Mammalian H-Ras and N-Ras are GTP-binding proteins that must be post-translationally lipidated to function as molecular switches in signal transduction cascades controlling cell growth and differentiation. These proteins contain a C-terminal farnesyl-cysteine alpha-methyl ester and palmitoyl groups attached to nearby cysteines. Data is presented showing that rat liver microsomes contain an enzyme that transfers the palmitoyl group from palmitoyl-coenzyme A to cysteine residues of H-Ras protein and of a synthetic peptide having the structure of the C terminus of N-Ras. This protein palmitoyltransferase (PPT) was solubilized from membranes and purified 10,500-fold to apparent homogeneity with an overall yield of 10%. On an SDS gel, PPT appears as two proteins of molecular masses of approximately 30 and approximately 33 kDa. If the palmitoylation sites of the N-Ras peptide (the non-farnesylated cysteine) or H-Ras protein (cysteines 181 and 184) are changed to serine, palmitoylation by PPT does not occur. Non-farnesylated H-Ras produced in bacteria as well as in vitro farnesylated bacterial H-Ras are not substrates for PPT nor is the non-farnesylated, methylated N-Ras peptide. These results suggest, but do not prove, that farnesylation and possibly C-terminal methylation are prerequisites for Ras palmitoylation. PPT shows a large preference for palmitoyl-coenzyme A over myristoyl-coenzyme as the acyl donor. Values of Km for palmitoyl-CoA and H-Ras are 4.3 +/- 1.2 and 0.8 +/- 0.3 microM, respectively. PPT is the first protein palmitoyltransferase to be purified, and the availability of pure enzyme should contribute to our understanding of the function and regulation of Ras palmitoylation in cells.

摘要

哺乳动物的H-Ras和N-Ras是GTP结合蛋白,必须经过翻译后脂化才能在控制细胞生长和分化的信号转导级联反应中作为分子开关发挥作用。这些蛋白质含有一个C端法尼基半胱氨酸α-甲酯和连接在附近半胱氨酸上的棕榈酰基。本文提供的数据表明,大鼠肝脏微粒体含有一种酶,该酶可将棕榈酰基从棕榈酰辅酶A转移至H-Ras蛋白以及具有N-Ras C端结构的合成肽的半胱氨酸残基上。这种蛋白质棕榈酰转移酶(PPT)从膜上溶解下来并纯化了10500倍,达到了明显的均一性,总产率为10%。在SDS凝胶上,PPT表现为两种分子量分别约为30 kDa和约33 kDa的蛋白质。如果将N-Ras肽(非法尼基化的半胱氨酸)或H-Ras蛋白(半胱氨酸181和184)的棕榈酰化位点变为丝氨酸,PPT就不会发生棕榈酰化。在细菌中产生的非法尼基化H-Ras以及体外法尼基化的细菌H-Ras都不是PPT的底物,非法尼基化、甲基化的N-Ras肽也不是。这些结果表明,但并未证明,法尼基化以及可能的C端甲基化是Ras棕榈酰化的先决条件。PPT作为酰基供体时,对棕榈酰辅酶A的偏好远高于肉豆蔻酰辅酶A。棕榈酰辅酶A和H-Ras的Km值分别为4.3±1.2和0.8±0.3 microM。PPT是首个被纯化的蛋白质棕榈酰转移酶,纯酶的可得性应有助于我们理解细胞中Ras棕榈酰化的功能和调控。

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