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去硫生物素合成酶:7,8-二氨基壬酸的羰基化反应通过N7-氨基甲酸酯区域特异性地进行。

Dethiobiotin synthetase: the carbonylation of 7,8-diaminonanoic acid proceeds regiospecifically via the N7-carbamate.

作者信息

Gibson K J, Lorimer G H, Rendina A R, Taylor W S, Cohen G, Gatenby A A, Payne W G, Roe D C, Lockett B A, Nudelman A

机构信息

Dupont Central Research and Development, Experimental Station, Wilmington, Delaware 19880-0407, USA.

出版信息

Biochemistry. 1995 Sep 5;34(35):10976-84. doi: 10.1021/bi00035a003.

DOI:10.1021/bi00035a003
PMID:7669755
Abstract

Dethiobiotin synthetase (DTBS) catalyzes the penultimate step in biotin biosynthesis, the formation of the ureido ring of dethiobiotin from (7R,8S)-7,8-diaminononanoic acid (7,8-diaminopelargonic acid, DAPA), CO2, and ATP. Solutions of DAPA at neutral pH readily formed a mixture of the N7- and N8-carbamates in the presence of CO2. However, four lines of evidence together indicated that only the N7-carbamate of DAPA was an intermediate in the reaction catalyzed by DTBS. (1) Addition of diazomethane to mixtures of DAPA and [14C]CO2 yielded a mixture of the N7- and N8-methyl carbamate esters, consistent with carbamate formation in free solution. In the presence of excess DTBS (over DAPA), the ratio of N7:N8-methyl carbamate esters recovered was roughly doubled, suggesting that the enzyme preferentially bound the N7-DAPA-carbamate. (2) Both N7- and N8-DAPA-carbamates were observed directly by 1H and 13C NMR in solutions containing DAPA and [13C]CO2. In the presence of excess DTBS (over DAPA) only one carbamate was observed, showing that carbamate binding to the enzyme was regiospecific. 13C NMR of mixtures containing enzyme, [7-15N]DAPA, and [13C]CO2 showed that the enzyme-bound carbamate was at N7 of DAPA. In addition, pulse-chase experiments showed that the binary complex of DTBS and N7-DAPA-carbamate became kinetically committed upon addition of MgATP. (3) The N7-DAPA-carbamate mimic, 3-(1-aminoethyl)nonanedioic acid, in which the carbamate nitrogen was replaced with a methylene group, cyclized to the corresponding lactam in the presence of DTBS and ATP; ADP and P(i) were also formed.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

去硫生物素合成酶(DTBS)催化生物素生物合成的倒数第二步反应,即由(7R,8S)-7,8-二氨基壬酸(7,8-二氨基壬二酸,DAPA)、二氧化碳和ATP形成去硫生物素的脲基环。在中性pH条件下,DAPA溶液在有二氧化碳存在时很容易形成N7-和N8-氨基甲酸酯的混合物。然而,四条证据共同表明,只有DAPA的N7-氨基甲酸酯是DTBS催化反应的中间体。(1)向DAPA和[14C]二氧化碳的混合物中加入重氮甲烷,得到N7-和N8-甲基氨基甲酸酯的混合物,这与在自由溶液中形成氨基甲酸酯一致。在过量DTBS(相对于DAPA)存在的情况下,回收的N7:N8-甲基氨基甲酸酯的比例大致翻倍,表明该酶优先结合N7-DAPA-氨基甲酸酯。(2)在含有DAPA和[13C]二氧化碳的溶液中,通过1H和13C NMR直接观察到了N7-和N8-DAPA-氨基甲酸酯。在过量DTBS(相对于DAPA)存在的情况下,只观察到一种氨基甲酸酯,表明氨基甲酸酯与酶的结合具有区域特异性。含有酶、[7-15N]DAPA和[13C]二氧化碳的混合物的13C NMR表明,与酶结合的氨基甲酸酯位于DAPA的N7位。此外,脉冲追踪实验表明,加入MgATP后,DTBS和N7-DAPA-氨基甲酸酯的二元复合物在动力学上变得不可逆。(3)N7-DAPA-氨基甲酸酯模拟物3-(1-氨基乙基)壬二酸,其中氨基甲酸酯氮被亚甲基取代,在DTBS和ATP存在下环化生成相应的内酰胺;同时还生成了ADP和无机磷酸。(摘要截于250字)

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