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In Vitro Assembly, Purification, and Crystallization of the Rab Geranylgeranyl Transferase:Substrate Complex

拉布 预酸化 三元络合物 香叶基锗化 GTP酶 生物化学 重组DNA 化学 立体化学 生物物理学 生物 基因
作者
Alexey Rak,Anca Niculae,Alexandr Kalinin,Nicolas H. Thomä,Vadim Sidorovitch,Roger S. Goody,Kirill Alexandrov
出处
期刊:Protein Expression and Purification [Elsevier]
卷期号:25 (1): 23-30 被引量:18
标识
DOI:10.1006/prep.2001.1605
摘要

Posttranslational modification with the geranygeranyl moiety is essential for the ability of Rab GTPases to control processes of membrane docking and fusion. This modification is conferred by Rab geranylgeranyltransferase (RabGGTase), which catalyzes the transfer of two 20-carbon geranylgeranyl groups from geranylgeranyl pyrophosphate onto C-terminal cysteine residues of Rab proteins. The enzyme consists of a catalytic alpha/beta heterodimer and an accessory protein termed Rab escort protein (REP-1) that delivers the newly prenylated Rab proteins to their target membrane. In order to understand the structural basis of Rab prenylation, we have investigated in vitro assembly and crystallization of the RabGGTase:REP-1:Rab complex. In order to ensure maximal stability of the ternary complex, we generated its monoprenylated form, which corresponds to a reaction intermediate and displays the highest affinity between the components. This was achieved by expressing the individual components in baculovirus and Escherichia coli systems with subsequent purification followed by in vitro monoprenylation of Rab7 with immobilized recombinant RabGGTase. Purified monoprenylated REP-1:Rab7 was complexed with recombinant RabGGTase and crystallized in hanging drops. The crystals obtained initially diffract to 8 A on an in-house X-ray source.
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