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Engineering Pseudomonas putida S12 for Efficient Utilization of d-Xylose and l-Arabinose

机译:工程化恶臭假单胞菌S12以有效利用d-木糖和l-阿拉伯糖

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摘要

The solvent-tolerant bacterium Pseudomonas putida S12 was engineered to utilize xylose as a substrate by expressing xylose isomerase (XylA) and xylulokinase (XylB) from Escherichia coli. The initial yield on xylose was low (9% [g CDW g substrate−1], where CDW is cell dry weight), and the growth rate was poor (0.01 h−1). The main cause of the low yield was the oxidation of xylose into the dead-end product xylonate by endogenous glucose dehydrogenase (Gcd). Subjecting the XylAB-expressing P. putida S12 to laboratory evolution yielded a strain that efficiently utilized xylose (yield, 52% [g CDW g xylose−1]) at a considerably improved growth rate (0.35 h−1). The high yield could be attributed in part to Gcd inactivity, whereas the improved growth rate may be connected to alterations in the primary metabolism. Surprisingly, without any further engineering, the evolved d-xylose-utilizing strain metabolized l-arabinose as efficiently as d-xylose. Furthermore, despite the loss of Gcd activity, the ability to utilize glucose was not affected. Thus, a P. putida S12-derived strain was obtained that efficiently utilizes the three main sugars present in lignocellulosic hydrolysate: glucose, xylose, and arabinose. This strain will form the basis for a platform host for the efficient production of biochemicals from renewable feedstock.
机译:通过表达大肠杆菌的木糖异构酶(XylA)和木酮糖激酶(XylB),将耐溶剂细菌恶臭假单胞菌S12工程化为利用木糖作为底物。木糖的初始产率较低(9%[g CDW g底物 -1 ],其中CDW为细胞干重),且生长速率较差(0.01 h -1 )。产量低的主要原因是木糖被内源性葡萄糖脱氢酶(Gcd)氧化为木糖末端产物。对表达XylAB的恶臭假单胞菌S12进行实验室进化,得到了一种可以有效利用木糖的菌株(收率52%[g CDW g木糖sup-1],大大提高了生长速度(0.35 h < sup> -1 )。高产量可能部分归因于Gcd的无活性,而生长速度的提高可能与初级代谢的改变有关。令人惊讶地,无需任何进一步的工程设计,进化的利用d-木糖的菌株与d-木糖一样有效地代谢了1-阿拉伯糖。此外,尽管Gcd活性丧失,但是利用葡萄糖的能力并未受到影响。因此,获得了恶臭假单胞菌S12来源的菌株,该菌株有效地利用了木质纤维素水解产物中存在的三种主要糖:葡萄糖,木糖和阿拉伯糖。该菌株将为从可再生原料高效生产生化药品的平台主机奠定基础。

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