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首页> 外文期刊>Biochemistry >Gramicidin S synthetase 1 (phenylalanine racemase), a prototype of amino acid racemases containing the cofactor 4'-phosphopantetheine.
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Gramicidin S synthetase 1 (phenylalanine racemase), a prototype of amino acid racemases containing the cofactor 4'-phosphopantetheine.

机译:Gramicidin S合成酶1(苯丙氨酸消旋酶)是一种氨基酸消旋体的原型,含有辅因子4'-磷酸泛素。

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The biosynthesis of the decapeptide antibiotic gramicidin S in Bacillus brevis ATCC 9999 is catalyzed by a multienzyme system consisting of two multifunctional proteins, gramicidin S synthetase 1 and 2, encoded by the grsA and grsB genes, respectively. Gramicidin S synthetase 1 (phenylalanine racemase, EC 5.1.1.11, GS1) racemizes phenylalanine in the thioester-bound stage. The amount of 4'-phosphopantetheine liberated from highly purified GS1 was determined microbiologically using Lacto-bacillus plantarum as the test organism. It matches exactly with the amount of L-[14C]phenylalanine covalently incorporated by GS1 as thioester. The reaction center of GS1 for L-phenylalanine thiolation and racemization was labeled with [3H]iodoacetic acid. After tryptic fragmentation of the 3H-carboxymethylated enzyme, the active site peptide for thioester binding and racemization of phenylalanine was isolated in pure form by multistep methodology and investigated by sequence, amino acid, and mass spectrometric analysis. A 4'-phosphopantetheine carrier was found to be attached to the active site serine of the consensus motif LGGDSI forming the thiolation site of phenylalanine. These specific properties establish GS1 as a prototype of amino acid racemases using 4'-phosphopantetheine as a cofactor and yield further evidence that multiple Pan carriers are involved in gramicidin S formation. Our results are strong evidence for the "multiple carrier model" as a new concept of nonribosomal peptide biosynthesis at protein templates as recently proposed [Stein, T., et al. (1994) FEBS Lett. 340, 39-44].
机译:短杆菌芽孢杆菌ATCC 9999中的十肽抗生素短杆菌肽S的生物合成由多酶系统催化,该酶由两种多功能蛋白质组成,短杆菌肽S合成酶1和2,分别由grsA和grsB基因编码。 Gramicidin S合成酶1(苯丙氨酸消旋酶,EC 5.1.1.11,GS1)在硫酯结合阶段使苯丙氨酸消旋。使用植物乳杆菌作为测试生物,通过微生物学方法确定了从高度纯化的GS1中释放的4'-磷酸泛素的量。它与GS1作为硫酯共价引入的L- [14C]苯丙氨酸的量完全匹配。 GS1的L-苯丙氨酸硫醇化和外消旋反应的反应中心用[3H]碘乙酸标记。在3H-羧甲基化酶的胰蛋白酶裂解后,通过多步方法以纯净的形式分离了硫酯结合和苯丙氨酸消旋化的活性位点肽,并通过序列,氨基酸和质谱分析进行了研究。发现4'-磷酸泛素的载体附着在共有基序LGGDSI的活性位丝氨酸上,形成苯丙氨酸的硫醇化位点。这些特殊的性质将GS1建立为氨基酸外消旋体的原型,使用4'-磷酸泛素作为辅因子,并进一步证明了多个Pan载体参与了短杆菌肽S的形成。我们的结果为“多载体模型”作为蛋白质模板上非核糖体肽生物合成的新概念提供了有力的证据[Stein,T.,等。 (1994)FEBS Lett。 340,39-44]。

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