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卟啉和钴啉的生物合成。2. 胆色素原脱氨酶共价复合物的分离、纯化及核磁共振研究。

Biosynthesis of porphyrins and corrins. 2. Isolation, purification, and NMR investigations of the porphobilinogen-deaminase covalent complex.

作者信息

Evans J N, Burton G, Fagerness P E, Mackenzie N E, Scott A I

出版信息

Biochemistry. 1986 Feb 25;25(4):905-12. doi: 10.1021/bi00352a025.

Abstract

The procedures for the generation of enzyme-substrate complexes from labeled porphobilinogens [(2,11-13C]PBG and [2,6,11-3H]PBG) with deaminase and the methods employed for their purification are described. Use of 13C NMR failed to detect the substrate bound to the enzyme, suggesting that the line width must be inordinately large. The complex was found to disproportionate with time when stored at 25 degrees C. However, enzyme-bound uroporphyrinogen I (uro'gen I) was detected, both in the intact protein and in the oligopeptides from tryptic digestion and peptide mapping. The first detection of an enzyme-substrate complex by 3H NMR is described for [3H]PBG and deaminase. The line widths of the observed resonances were found to be extremely large and dependent upon temperature, giving chemical shifts that suggest the involvement of a sulfhydryl group as the nucleophilic enzyme group that binds the substrate. The catalytic competence of this complex was also demonstrated by displacing bound [3H]PBG with unlabeled PBG. During the resultant formation of [3H]uro'gen I, a transient low-intensity signal was detected that has been tentatively assigned to the highly reactive azafulvene species, proposed in several mechanistic schemes for porphyrin biosynthesis.

摘要

本文描述了用脱氨酶从标记的胆色素原([2,11 - 13C]PBG和[2,6,11 - 3H]PBG)生成酶 - 底物复合物的步骤及其纯化方法。使用13C NMR未能检测到与酶结合的底物,这表明线宽必定异常大。发现该复合物在25℃储存时会随时间发生歧化反应。然而,在完整蛋白质以及胰蛋白酶消化和肽图谱分析得到的寡肽中均检测到了与酶结合的尿卟啉原I(uro'gen I)。本文描述了首次通过3H NMR检测[3H]PBG与脱氨酶形成的酶 - 底物复合物。观察到的共振信号的线宽极大且依赖于温度,化学位移表明有一个巯基作为结合底物的亲核酶基团参与其中。通过用未标记的PBG取代结合的[3H]PBG,也证明了该复合物的催化活性。在生成[3H]uro'gen I的过程中,检测到一个短暂的低强度信号,该信号暂时被归属于在卟啉生物合成的几种机制方案中提出的高反应性氮杂富烯物种。

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