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首页> 外文期刊>RSC Advances >Biochemical characterization and biocatalytic application of a novel d-tagatose 3-epimerase from Sinorhizobium sp.
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Biochemical characterization and biocatalytic application of a novel d-tagatose 3-epimerase from Sinorhizobium sp.

机译:SINORHIZOBIUM SP的新型D-Tagatose 3-eBimerase的生物化学表征及生物催化应用。

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Sinorhizobium sp. D -tagatose 3-epimerase (sDTE) catalyzes the conversion of D -tagatose to D -sorbose. It also recognizes D -fructose as a substrate for D -allulose production. The optimal temperature and pH of the purified sDTE was 50 °C and 8.0, respectively. Based on the sDTE homologous model, Glu154, Asp187, Gln213, and Glu248, form a hydrogen bond network with the active-site Mn ~(2+) and constitute the catalytic tetrad. The amino acid residues around O-1, -2, and -3 atoms of the substrates ( D -tagatose/ D -fructose) are strictly conserved and thus likely regulate the catalytic reaction. However, the residues at O-4, -5, and -6, being responsible for the substrate-binding, are different. In particular, Arg65 and Met9 were found to form a unique interaction with O-4 of D -fructose and D -tagatose. The whole cells with recombinant sDTE showed a higher bioconversion rate of 42.5% in a fed-batch bioconversion using D -fructose as a substrate, corresponding to a production of 476 g L ~(?1) D -allulose. These results suggest that sDTE is a potential industrial biocatalyst for the production of D -allulose in fed-batch mode.
机译:Sinorhizobium sp。 D -Tagatose 3-截止酶(SDTE)催化D -TAGATOSE至D光水糖的转化。它还识别D-污染作为D-冶金生产的基材。纯化的SDTE的最佳温度和pH分别为50℃和8.0。基于SDTE同源型号,GLU154,ASP187,GLN213和GLU248,形成氢键网络,与活性位点Mn〜(2+)形成并构成催化Tetrad。底物围绕O-1,-2和-3原子(D-Tagatose / D污染)的氨基酸残基被严格保守,因此可能调节催化反应。然而,O-4,-5和-6的残基对底物结合负责是不同的。特别地,发现Arg65和Met9形成与D-污染的O-4的独特相互作用和D -Tagatose。具有重组SDTE的整个细胞在FED-批量生物转化中呈42.5%的较高生物转化率,其使用D-果糖作为基材,对应于476g L〜(α1)D-冶金的产生。这些结果表明,SDTE是一种潜在的工业生物催化剂,用于生产D-Blululose在膳食批次模式下。

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