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From the Cover: Evolution of D-lactate dehydrogenase activity from glycerol dehydrogenase and its utility for D-lactate production from lignocellulose

机译:从封面开始:甘油脱氢酶的D-乳酸脱氢酶活性的演变及其在木质纤维素生产D-乳酸中的应用

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摘要

Lactic acid, an attractive, renewable chemical for production of biobased plastics (polylactic acid, PLA), is currently commercially produced from food-based sources of sugar. Pure optical isomers of lactate needed for PLA are typically produced by microbial fermentation of sugars at temperatures below 40 °C. Bacillus coagulans produces L(+)-lactate as a primary fermentation product and grows optimally at 50 °C and pH 5, conditions that are optimal for activity of commercial fungal cellulases. This strain was engineered to produce D(−)-lactate by deleting the native ldh (L-lactate dehydrogenase) and alsS (acetolactate synthase) genes to impede anaerobic growth, followed by growth-based selection to isolate suppressor mutants that restored growth. One of these, strain QZ19, produced about 90 g L-1 of optically pure D(−)-lactic acid from glucose in < 48 h. The new source of D-lactate dehydrogenase (D-LDH) activity was identified as a mutated form of glycerol dehydrogenase (GlyDH; D121N and F245S) that was produced at high levels as a result of a third mutation (insertion sequence). Although the native GlyDH had no detectable activity with pyruvate, the mutated GlyDH had a D-LDH specific activity of 0.8 μmoles min-1 (mg protein)-1. By using QZ19 for simultaneous saccharification and fermentation of cellulose to D-lactate (50 °C and pH 5.0), the cellulase usage could be reduced to 1/3 that required for equivalent fermentations by mesophilic lactic acid bacteria. Together, the native B. coagulans and the QZ19 derivative can be used to produce either L(+) or D(−) optical isomers of lactic acid (respectively) at high titers and yields from nonfood carbohydrates.
机译:乳酸是一种有吸引力的可再生化学物质,用于生产生物基塑料(聚乳酸,PLA),目前是从食品中的糖类来源商业生产的。 PLA所需的乳酸纯旋光异构体通常是在低于40°C的温度下通过糖的微生物发酵生产的。凝结芽胞杆菌产生L(+)-乳酸盐作为主要发酵产物,并在50°C和pH 5下最佳生长,这是商业真菌纤维素酶活性的最佳条件。通过删除天然的ldh(L-乳酸脱氢酶)和alsS(乙酰乳酸合酶)基因来阻止厌氧生长,然后基于生长的选择以分离恢复生长的抑制突变体,将该菌株工程化以产生D(-)-乳酸。其中之一是QZ19菌株,它在<48小时内从葡萄糖中产生了约90 g L -1 光学纯的D(-)-乳酸。 D-乳酸脱氢酶(D-LDH)活性的新来源被确定为甘油脱氢酶(GlyDH; D121N和F245S)的突变形式,该突变形式是由于第三次突变(插入序列)而高水平产生的。尽管天然的GlyDH没有丙酮酸的活性,但突变的GlyDH的D-LDH比活性为0.8μmol·min -1 (mg蛋白) -1 。通过使用QZ19同时糖化和将纤维素发酵成D-乳酸(50°C和pH值5.0),纤维素酶的使用量可减少至中温乳酸菌等效发酵所需的1/3。天然凝结芽孢杆菌和QZ19衍生物一起可用于分别以高滴度和非食品碳水化合物的产率生产乳酸的L(+)或D(-)旋光异构体。

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