Integrated isotope-assisted metabolomics and (13)C metabolic flux analysis reveals metabolic flux redistribution for high glucoamylase production by Aspergillus niger.

Hongzhong Lu,Ju Chu,Jianye Xia,Yingping Zhuang,Xiaoyun Liu,Siliang Zhang,Henk Noorman,Mingzhi Huang

doi:10.1186/s12934-015-0329-y

Abstract

BackgroundAspergillus niger is widely used for enzyme production and achievement of high enzyme production depends on the comprehensive understanding of cell’s metabolic regulation mechanisms.ResultsIn this paper, we investigate the metabolic differences and regulation mechanisms between a high glucoamylase-producing strain A. niger DS03043 and its wild-type parent strain A. niger CBS513.88 via an integrated isotope-assisted metabolomics and 13C metabolic flux analysis approach. We found that A. niger DS03043 had higher cell growth, glucose uptake, and glucoamylase production rates but lower oxalic acid and citric acid secretion rates. In response to above phenotype changes, A. niger DS03043 was characterized by an increased carbon flux directed to the oxidative pentose phosphate pathway in contrast to reduced flux through TCA cycle, which were confirmed by consistent changes in pool sizes of metabolites. A higher ratio of ATP over AMP in the high producing strain might contribute to the increase in the PP pathway flux as glucosephosphate isomerase was inhibited at higher ATP concentrations. A. niger CBS513.88, however, was in a higher redox state due to the imbalance of NADH regeneration and consumption, resulting in the secretion of oxalic acid and citric acid, as well as the accumulation of intracellular OAA and PEP, which may in turn result in the decrease in the glucose uptake rate.ConclusionsThe application of integrated metabolomics and 13C metabolic flux analysis highlights the regulation mechanisms of energy and redox metabolism on flux redistribution in A. niger. Graphical abstractAn integrated isotope-assisted metabolomics and 13C metabolic flux analysis was was firstly systematically performed in A. niger. In response to enzyme production, the metabolic flux in A. niger DS03043 (high-producing) was redistributed, characterized by an increased carbon flux directed to the oxidative pentose phosphate pathway as well as an increased pool size of pentose. The consistency in 13C metabolic flux analysis and metabolites quantification indicated that an imbalance of NADH formation and consumption led to the accumulation and secretion of organic acids in A. niger CBS513.88 (wild-type)Electronic supplementary materialThe online version of this article (doi:10.1186/s12934-015-0329-y) contains supplementary material, which is available to authorized users.

Highlights

Aspergillus niger is widely used for enzyme production and achievement of high enzyme production depends on the comprehensive understanding of cell’s metabolic regulation mechanisms
For fructofuranosidase production by A. niger, Driouch et al [15] reported that the production of recombinant enzyme led to a flux redistribution and in the recombinant strain the cytosolic pentose phosphate pathway (PPP) and mitochondrial malic enzyme was activated, indicating that the supply of NADPH is essential for efficient production of this protein
Though the specific growth and glucose uptake rate of A. niger DS03043 was about 40 and 25 % higher than those of A. niger CBS513.88, respectively, the two strains showed no statistically significant differences in the yields of biomass (YX/S) and CO2 (YCO2/S), initially indicating that mainly the reduction in byproducts formation was compensated for the large increase in glucoamylase production by A. niger DS03043

Summary

Introduction

Aspergillus niger is widely used for enzyme production and achievement of high enzyme production depends on the comprehensive understanding of cell’s metabolic regulation mechanisms. Aspergillus niger, one of the most important filamentous fungi, has been widely used for the production of organic acids [1,2,3], such as citric and gluconic acid, and for the production of enzymes [4, 5] including glucoamylase, proteases, cellulase and glucose oxidase due to its excellent capacity in expression and secretion of proteins. Despite the wide usage of A. niger for enzyme production, metabolic regulation mechanisms for high enzyme. The latest 13C metabolic flux analysis revealed that the imbalance in regeneration and utilization of cofactors result in the secretion of by-products [17]

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Conclusion