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High yield production of myristoylated Arf6 small GTPase by recombinant N-myristoyl transferase

机译:重组N-肉豆蔻酰基转移酶高产肉豆蔻酰化的Arf6小GTP酶

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摘要

Small GTP-binding proteins of the Arf family (Arf GTPases) interact with multiple cellular partners and with membranes to regulate intracellular traffic and organelle structure. Understanding the underlying molecular mechanisms requires in vitro biochemical assays to test for regulations and functions. Such assays should use proteins in their cellular form, which carries a myristoyl lipid attached in N-terminus. N-myristoylation of recombinant Arf GTPases can be achieved by co-expression in E. coli with a eukaryotic N-myristoyl transferase. However, purifying myristoylated Arf GTPases is difficult and has a poor overall yield. Here we show that human Arf6 can be N-myristoylated in vitro by recombinant N-myristoyl transferases from different eukaryotic species. The catalytic efficiency depended strongly on the guanine nucleotide state and was highest for Arf6-GTP. Large-scale production of highly pure N-myristoylated Arf6 could be achieved, which was fully functional for liposome-binding and EFA6-stimulated nucleotide exchange assays. This establishes in vitro myristoylation as a novel and simple method that could be used to produce other myristoylated Arf and Arf-like GTPases for biochemical assays.
机译:Arf家族的小GTP结合蛋白(Arf GTPases)与多个细胞伴侣和膜相互作用,调节细胞内运输和细胞器结构。要了解潜在的分子机制,需要进行体外生化分析以测试法规和功能。此类测定应使用细胞形式的蛋白质,该蛋白质带有在N末端连接的肉豆蔻酰脂质。重组Arf GTPases的N-肉豆蔻酰基化可以通过在大肠杆菌中与真核N-肉豆蔻酰基转移酶共表达来实现。但是,纯化肉豆蔻酰化的Arf GTPases是困难的,并且总产率很差。在这里,我们显示人Arf6可以通过来自不同真核物种的重组N-肉豆蔻酰基转移酶在体外进行N-肉豆蔻酰基化。催化效率在很大程度上取决于鸟嘌呤的核苷酸状态,对于Arf6-GTP最高。可以实现高纯度N-肉豆蔻酰化Arf6的大规模生产,这对于脂质体结合和EFA6刺激的核苷酸交换测定具有完全的功能。这将体外肉豆蔻酰化确立为一种新颖,简单的方法,可用于生产其他肉豆蔻酰化的Arf和类似Arf的GTPases用于生化测定。

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