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首页> 外文期刊>Protein Expression and Purification >Production of reagents and optimization of methods for studying calmodulin-binding proteins.
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Production of reagents and optimization of methods for studying calmodulin-binding proteins.

机译:试剂的生产和钙调蛋白结合蛋白研究方法的优化。

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摘要

Owing to subtle but potentially crucial structural and functional differences between calmodulin (CaM) of different species, the biochemical study of low-affinity CaM-binding proteins from Dictyostelium discoideum likely necessitates the use of CaM from the same organism. In addition, most of the methods used for identification and purification of CaM-binding proteins require native CaM in nonlimiting biochemical quantities. The gene encoding D. discoideum CaM has previously been cloned allowing production of recombinant protein. The present study describes the expression of D. discoideum CaM in Escherichia coli and its straightforward and rapid purification. Furthermore, we describe the optimization of a complete palette of assays to detect as little as nanogram quantities of proteins binding CaM with middle to low affinities. Purified CaM was used to raise high-affinity polyclonal antibodies suitable for immunoblotting, immunofluorescence, and immunoprecipitation experiments. The purified CaM was also used to optimize a specific and sensitive nonradioactive CaM overlay assay as well as to produce a high-capacity CaM affinity chromatography matrix. The effectiveness of this methods is illustrated by the detection of potentially novel D. discoideum CaM-binding proteins and the preparatory purification of one of these proteins, a short tail myosin I. Copyright 1999 Academic Press.
机译:由于不同物种的钙调蛋白(CaM)之间存在细微但潜在的至关重要的结构和功能差异,来自盘基网柄菌的低亲和力CaM结合蛋白的生化研究可能需要使用同一生物的CaM。另外,用于鉴定和纯化CaM结合蛋白的大多数方法需要非限制性生化量的天然CaM。先前已克隆了编码迪斯科球菌CaM的基因,可生产重组蛋白。本研究描述了D.discoideum CaM在大肠杆菌中的表达及其直接,快速的纯化。此外,我们描述了完整检测方法的优化,以检测低至纳克级的中低亲和力结合CaM的蛋白质。纯化的CaM用于产生适合免疫印迹,免疫荧光和免疫沉淀实验的高亲和力多克隆抗体。纯化的CaM还可用于优化特异性和灵敏的非放射性CaM重叠测定,以及产生高容量的CaM亲和色谱基质。该方法的有效性通过检测潜在的新型迪斯科螺旋藻CaM结合蛋白和对其中一种蛋白(短尾肌球蛋白I)的制备纯化进行了说明。版权所有1999,Academic Press。

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