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结合抗体片段的刀豆脲酶的结晶及初步X射线晶体结构测定

Crystallization and preliminary X-ray structure determination of jack bean urease with a bound antibody fragment.

作者信息

Sheridan Louisa, Wilmot Carrie M, Cromie Karen D, van der Logt Paul, Phillips Simon E V

机构信息

Department of Biochemistry and Molecular Biology, University of Leeds, Leeds LS2 9JT, England.

出版信息

Acta Crystallogr D Biol Crystallogr. 2002 Feb;58(Pt 2):374-6. doi: 10.1107/s0907444901021503. Epub 2002 Jan 24.

Abstract

Urease allows organisms to use exogenous and internally generated urea as a nitrogen source, by catalyzing the hydrolysis of urea to form ammonia and carbon dioxide. Urease may also participate in the systemic nitrogen-transport pathways and possibly acts as a toxic defence protein. Jack bean urease (JBU) was the first nickel-metalloenzyme identified and was crystallized as early as 1926. Despite this, the structure has not yet been determined. An antibody fragment, Fv, that has a high affinity for JBU has been used to aid crystallization. The complex, which retains full enzyme activity, forms very small crystals that diffract weakly to 3.3 A. The crystals belong to the rhombohedral space group R32, with unit-cell parameters a = b = 228.6, c = 130.9 A. The structure of the urease molecule has been solved by molecular replacement using the structure of homogenous enzyme from Klebsiella aerogenes as a search model.

摘要

脲酶可通过催化尿素水解生成氨和二氧化碳,使生物体将外源性和内源性产生的尿素用作氮源。脲酶还可能参与全身氮转运途径,并可能作为一种毒性防御蛋白发挥作用。刀豆脲酶(JBU)是最早被鉴定出的镍金属酶,早在1926年就已结晶。尽管如此,其结构尚未确定。一种对JBU具有高亲和力的抗体片段Fv已被用于辅助结晶。该复合物保留了完整的酶活性,形成的晶体非常小,衍射能力较弱,分辨率为3.3埃。这些晶体属于菱面体空间群R32,晶胞参数a = b = 228.6,c = 130.9埃。脲酶分子的结构已通过分子置换法解析,使用产气克雷伯菌同源酶的结构作为搜索模型。

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