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首页> 外文期刊>Protein Expression and Purification >EXPRESSION AND PURIFICATION OF SOLUBLE, ACTIVE HETERODIMERIC GUANYLYL CYCLASE FROM BACULOVIRUS
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EXPRESSION AND PURIFICATION OF SOLUBLE, ACTIVE HETERODIMERIC GUANYLYL CYCLASE FROM BACULOVIRUS

机译:杆状病毒中可溶性,活性异源二聚体瓜酰基环化酶的表达和纯化

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摘要

A method for expression and purification of active cytosolic heterodimeric histidine (His)-tagged guanylyl cyclase of the alpha 1/beta 1 isoform has been developed using recombinant baculovirus-transfected insect cells. Confirmation of expression of active cyclase was obtained by both Western analysis and enzymatic activity. A His tag on the COOH-terminus of the alpha 1 and beta 1 subunits allowed rapid purification of the heterodimeric form of guanylyl cyclase in a single affinity step using a nickel column. A second gel-filtration step was applied to reconstitute into the complex heme, a required cofactor. This was confirmed spectroscopically by absorbance in the Soret region. Like enzyme purified from tissue, the activity of recombinant guanylyl cyclase was increased by protoporphyrin IX and inhibited by both Zn- and Sn-protoporphyrin. The method described here should provide a general approach for the expression and purification of alternate forms of cytosolic guanylyl cyclase and facilitate mechanistic and structural studies of this important family of enzymes. Furthermore, the procedure demonstrates the utility of the His-tag system to purify multimeric proteins. (C) 1997 Academic Press. [References: 33]
机译:已经使用重组杆状病毒转染的昆虫细胞开发了一种表达和纯化活性胞质异二聚组氨酸(His)标记的鸟嘌呤环化酶的α1/β1亚型的方法。通过蛋白质印迹分析和酶促活性均获得了活性环化酶表达的确认。 α1和β1亚基的COOH末端上的His标记允许使用镍柱在单个亲和步骤中快速纯化鸟苷酸环化酶的异二聚体形式。进行第二个凝胶过滤步骤,以重构为必需的辅因子复合血红素。在光谱上通过Soret区域的吸光度证实了这一点。像从组织中纯化的酶一样,重组鸟嘌呤环化酶的活性被原卟啉IX增强,而被Zn和Sn原卟啉抑制。此处描述的方法应提供一种表达和纯化胞质鸟苷酰环化酶替代形式的通用方法,并促进对该重要酶家族的机理和结构研究。此外,该程序证明了His-tag系统可用于纯化多聚体蛋白。 (C)1997学术出版社。 [参考:33]

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