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Engineering of Pseudomonas putida for accelerated co-utilization of glucose and cellobiose yields aerobic overproduction of pyruvate explained by an upgraded metabolic model

恶臭假单胞菌 纤维二糖 生产过剩 生物化学 周质间隙 代谢工程 戊糖 生物生产 生物 化学 突变体 大肠杆菌 木质纤维素生物量 细菌纤维素 纤维素 发酵 纤维素酶 基因
作者
Dalimil Bujdoš,Barbora Popelářová,Daniel C. Volke,Pablo I. Nikel,Nikolaus Sonnenschein,Pavel Dvořák
出处
期刊:Metabolic Engineering [Elsevier]
卷期号:75: 29-46 被引量:18
标识
DOI:10.1016/j.ymben.2022.10.011
摘要

Pseudomonas putida KT2440 is an attractive bacterial host for biotechnological production of valuable chemicals from renewable lignocellulosic feedstocks as it can valorize lignin-derived aromatics or glucose obtainable from cellulose. P. putida EM42, a genome-reduced variant of strain KT2440 endowed with advantageous physiological properties, was recently engineered for growth on cellobiose, a major cellooligosaccharide product of enzymatic cellulose hydrolysis. Co-utilization of cellobiose and glucose was achieved in a mutant lacking periplasmic glucose dehydrogenase Gcd (PP_1444). However, the cause of the co-utilization phenotype remained to be understood and the Δ gcd strain had a significant growth defect. In this study, we investigated the basis of the simultaneous uptake of the two sugars and accelerated the growth of P. putida EM42 Δ gcd mutant for the bioproduction of valuable compounds from glucose and cellobiose. We show that the gcd deletion lifted the inhibition of the exogenous β-glucosidase BglC from Thermobifida fusca exerted by the intermediates of the periplasmic glucose oxidation pathway. The additional deletion of hexR gene, which encodes a repressor of the upper glycolysis genes, failed to restore rapid growth on glucose. The reduced growth rate of the Δ gcd mutant was partially compensated by the implantation of heterologous glucose and cellobiose transporters (Glf from Zymomonas mobilis and LacY from Escherichia coli , respectively). Remarkably, this intervention resulted in the accumulation of pyruvate in aerobic P. putida cultures. We demonstrated that the excess of this key metabolic intermediate can be redirected to the enhanced biosynthesis of ethanol and lactate. The pyruvate overproduction phenotype was then unveiled by an upgraded genome-scale metabolic model constrained with proteomic and kinetic data. The model pointed to the saturation of glucose catabolism enzymes due to unregulated substrate uptake and it predicted improved bioproduction of pyruvate-derived chemicals by the engineered strain. This work sheds light on the co-metabolism of cellulosic sugars in an attractive biotechnological host and introduces a novel strategy for pyruvate overproduction in bacterial cultures under aerobic conditions. • Co-utilization of glucose and cellobiose by a Δ gcd mutant of P. putida EM42. • Growth defect of the mutant compensated by implanting exogenous sugar transporters. • Enhanced carbon influx caused aerobic overproduction of pyruvate and acetate. • Carbon from excess pyruvate streamed into ethanol or L-lactate. • Pyruvate overproduction unveiled by a mathematical model of P. putida metabolism.
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