Development and Applications of a Calmodulin-Based Fusion Protein System for the Expression and Purification of WW and Zinc Finger Modules.

Christopher G Toomey, D. Weiss, A. Chant, Megan M. Ackerman, B. Ahlers, Y. Lam, Christopher Ricciardi, D. Bourne, Christina M. Kraemer-Chant
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Abstract

Calmodulin from Homo sapiens is an α-helical calcium-binding protein that expresses to high levels in E. coli. When the N-terminus of a calmodulin variant is bound to Ca2+, it undergoes a conformational change, exposing hydrophobic pockets. This property can be utilized for purification purposes, as these pockets bind to phenyl sepharose resin with high affinity. Washing with EDTA chelates the Ca2+ ions from the protein, inducing a conformational change back to the more folded state and eluting the protein from the column. We describe herein the use of a protein expression and purification technique using the calmodulin variant and a short linker for proteolytic cleavage by the mutant NIa-Pro tobacco etch virus protease. We have shown this approach to be useful in obtaining purified quantities of various small proteins that could not be expressed using other methods, including high enough concentrations of a designed WW domain protein for NMR structural analysis. We have also obtained promising results on the usefulness of this procedure to express and purify zinc finger proteins without the addition of zinc ions or other cofactors.
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基于钙调素的WW和锌指蛋白表达纯化融合蛋白体系的建立与应用。
来自智人的钙调素是一种在大肠杆菌中高水平表达的α-螺旋钙结合蛋白。当钙调素变体的N末端与Ca2+结合时,它会发生构象变化,暴露出疏水性口袋。这种性质可用于纯化目的,因为这些口袋以高亲和性与苯基琼脂糖树脂结合。用EDTA洗涤可以螯合蛋白质中的Ca2+离子,诱导构象变化回到更折叠的状态,并将蛋白质从柱中洗脱。我们在本文中描述了使用钙调素变体和短连接体的蛋白质表达和纯化技术通过突变体NIa Pro烟草蚀刻病毒蛋白酶进行蛋白水解切割的用途。我们已经证明,这种方法可用于获得纯化量的各种小蛋白,这些小蛋白不能使用其他方法表达,包括用于NMR结构分析的足够高浓度的设计WW结构域蛋白。我们还获得了关于该程序在不添加锌离子或其他辅因子的情况下表达和纯化锌指蛋白的有用性的有希望的结果。
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