首页> 外文OA文献 >Enzymatic Synthesis of Dithiolopyrrolone Antibiotics Using Cell-Free Extract of Saccharothrix algeriensis NRRL B-24137 and Biochemical Characterization of Two Pyrrothine N-Acyltransferases in This Extract.
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Enzymatic Synthesis of Dithiolopyrrolone Antibiotics Using Cell-Free Extract of Saccharothrix algeriensis NRRL B-24137 and Biochemical Characterization of Two Pyrrothine N-Acyltransferases in This Extract.

机译:使用阿尔氏酵母糖浆NRRL B-24137的无细胞提取物酶促合成二硫代吡咯烷酮抗生素,并提取该提取物中的两种酪氨酸N-酰基转移酶。

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摘要

Saccharothrix algeriensis NRRL B-24137 produces naturally different dithiolopyrrolone derivatives. The enzymatic activity of pyrrothine N-acyltransferase was determined to be responsible for the transfer of an acyl group from acyl-CoA to pyrrothine core. This activity was also reported to be responsible for the diversity of the dithiolopyrrolone derivatives. Based on this fact, nine dithiolopyrrolone derivatives were produced in vitro via the crude extract of Sa. algeriensis. Three of them have never been obtained before by natural fermentation: acetoacetyl-pyrrothine, hydroxybutyryl-pyrrothine, and dimethyl thiolutin (holomycin). Two acyltransferase activities, acetyltransferase and benzoyltransferase catalyzing the incorporation of linear and cyclic acyl groups to the pyrrothine core, respectively, were biochemically characterized in this crude extract. The first one is responsible for formation of acetyl-pyrrothine and the second for benzoyl-pyrrothine. Both enzymes were sensitive to temperature changes: For example, the loss of acetyltransferase and benzoyltransferase activity was 53% and 80% respectively after pre-incubation of crude extract for 60 min at 20°C. The two enzymes were more active in neutral and basal media (pH 7-10) than in the acidic one (pH 3-6). The optimum temperature and pH of acetyltransferase were 40°C and 7, with a Km value of 7.9 μM and a Vmax of 0.63 μM/min when acetyl-CoA was used as limited substrate. Benzoyltransferase had a temperature and a pH optimum at 55°C and 9, a Km value of 14.7 μM, and a Vmax of 0.67 μM/min when benzoyl- CoA was used as limited substrate.
机译:酿酒酵母NRRL B-24137天然产生不同的二硫代吡咯烷酮衍生物。确定吡咯烷N-酰基转移酶的酶促活性负责酰基从酰基-CoA到吡咯烷核的转移。还据报道,该活性是二硫代吡咯烷酮衍生物的多样性的原因。基于这一事实,通过Sa的粗提物体外生产了九种二硫代吡咯烷酮衍生物。阿尔及利亚。它们中的三个以前从未通过自然发酵获得:乙酰乙酰基-酪氨酸,羟基丁酰基-酪氨酸和二甲基硫代鲁汀(holomycin)。在该粗提物中,通过生化表征了两个酰基转移酶活性,分别是乙酰基转移酶和苯甲酰基转移酶,分别催化线性和环状酰基结合到吡咯烷核中。第一个负责乙酰基-酪氨酸的形成,第二个负责苯甲酰基-酪氨酸的形成。两种酶均对温度变化敏感:例如,将粗提取物在20°C下预孵育60分钟后,乙酰转移酶和苯甲酰转移酶活性的损失分别为53%和80%。这两种酶在中性和碱性介质(pH 7-10)中比在酸性介质(pH 3-6)中更具活性。当使用乙酰辅酶A作为有限的底物时,乙酰转移酶的最佳温度和pH为40°C和7,Km值为7.9μM,Vmax为0.63μM/ min。当使用苯甲酰基-CoA作为有限的底物时,苯甲酰转移酶的温度和最佳pH在55°C和9下最佳,Km值为14.7μM,Vmax为0.67μM/ min。

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