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(βα)8桶状酶吲哚-3-甘油磷酸合酶的N端延伸在其折叠、稳定性和催化活性中的作用。

Role of the N-terminal extension of the (betaalpha)8-barrel enzyme indole-3-glycerol phosphate synthase for its fold, stability, and catalytic activity.

作者信息

Schneider Birgit, Knöchel Thorsten, Darimont Beatrice, Hennig Michael, Dietrich Susanne, Babinger Karin, Kirschner Kasper, Sterner Reinhard

机构信息

Institut für Biophysik und physikalische Biochemie, Universität Regensburg, Universitätsstrasse 31, D-93053 Regensburg, Germany.

出版信息

Biochemistry. 2005 Dec 20;44(50):16405-12. doi: 10.1021/bi051640n.

DOI:10.1021/bi051640n
PMID:16342933
Abstract

Indole-3-glycerol phosphate synthase (IGPS) catalyzes the fifth step in the biosynthesis of tryptophan. It belongs to the large and versatile family of (betaalpha)(8)-barrel enzymes but has an unusual N-terminal extension of about 40 residues. Limited proteolysis with trypsin of IGPS from both Sulfolobus solfataricus (sIGPS) and Thermotoga maritima (tIGPS) removes about 25 N-terminal residues and one of the two extra helices contained therein. To assess the role of the extension, the N-terminally truncated variants sIGPSDelta(1-26) and tIGPSDelta(1-25) were produced recombinantly in Escherichia coli, purified, and characterized in comparison to the wild-type enzymes. Both sIGPSDelta(1-26) and tIGPSDelta(1-25) have unchanged oligomerization states and turnover numbers. In contrast, their Michaelis constants for the substrate 1-(o-carboxyphenylamino)-1-deoxyribulose 5-phosphate are increased, and their resistance toward unfolding induced by heat and guanidinium chloride is decreased. sIGPSDelta(1-26) was crystallized, and its X-ray structure was solved at 2.8 A resolution. The comparison with the known structure of sIGPS reveals small differences that account for its reduced substrate affinity and protein stability. The structure of the core of sIGPSDelta(1-26) is, however, unchanged compared to sIGPS, explaining its retained catalytic activity and consistent with the idea that it evolved from the same ancestor as the phosphoribosyl anthranilate isomerase and the alpha-subunit of tryptophan synthase. These (betaalpha)(8)-barrel enzymes catalyze the reactions preceding and following IGPS in tryptophan biosynthesis but lack an N-terminal extension.

摘要

吲哚 - 3 - 甘油磷酸合酶(IGPS)催化色氨酸生物合成的第五步。它属于庞大且多功能的(βα)8桶状酶家族,但具有约40个残基的不寻常N端延伸。来自嗜热栖热菌(tIGPS)和嗜热栖硫叶菌(sIGPS)的IGPS经胰蛋白酶有限度的蛋白水解可去除约25个N端残基以及其中包含的两个额外螺旋之一。为了评估该延伸的作用,在大肠杆菌中重组表达、纯化了N端截短的变体sIGPSΔ(1 - 26)和tIGPSΔ(1 - 25),并与野生型酶进行了比较表征。sIGPSΔ(1 - 26)和tIGPSΔ(1 - 25)的寡聚化状态和周转数均未改变。相比之下,它们对底物1 - (邻羧基苯基氨基)-1 - 脱氧核糖 - 5 - 磷酸的米氏常数增加,并且它们对热和氯化胍诱导的去折叠的抗性降低。sIGPSΔ(1 - 26)结晶后,其X射线结构在2.8 Å分辨率下解析。与sIGPS的已知结构比较发现了一些小差异,这些差异解释了其底物亲和力降低和蛋白质稳定性下降的原因。然而,sIGPSΔ(1 - 26)的核心结构与sIGPS相比没有变化,这解释了其保留的催化活性,并且与它与磷酸核糖基邻氨基苯甲酸异构酶和色氨酸合酶α亚基起源于同一祖先的观点一致。这些(βα)8桶状酶催化色氨酸生物合成中IGPS之前和之后的反应,但缺乏N端延伸。

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