Efficient D-allulose synthesis under acidic conditions by auto-inducing expression of the tandem D-allulose 3-epimerase genes in Bacillus subtilis

d-Allulose, a rare sugar and functional sweetener, can be biosynthesized by d-allulose 3-isomerase (DAE). However, most of the reported DAEs exhibit poor resistance under acidic conditions, which severely limited their application. Here, surface charge engineering and random mutagenesis were used to construct a mutant library of CcDAE from Clostridium cellulolyticum H10, combined with high-throughput screening to identify mutants with high activity and resistance under acidic conditions. The mutant M3 (I114R/K123E/H209R) exhibited high activity (3.36-fold of wild-type) and acid resistance (10.6-fold of wild-type) at pH 4.5. The structure–function relationship was further analyzed by molecular dynamics (MD) simulations, which indicated that M3 had a higher number of hydrogen bonds and negative surface charges than the wild type. A multienzyme cascade system including M3 was used to convert high-calorie sugars in acidic juices, and functional juices containing 7.8–15.4 g/L d-allulose were obtained. Our study broadens the manufacture of functional foods containing d-allulose.

Section: ■ Results and Discussionmentioning

confidence: 99%

Section: ■ Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Engineering of Acid-Resistant d-Allulose 3-Epimerase for Functional Juice Production

Zhang

Wang

et al. 2022

“…Thus, the blockage of fructose PTS and fructokinase resulted in a remarkable 7.0-fold increase of the D- subtilis, we screened nine constitutive promoters (P HpaII , P spovG , P luxS , P amyE , P 43 , P gsiB , P srfA , P nprE , and P sigW ), which were reported to exhibit different expression levels of heterologous proteins in B. subtilis. 33,34 For comparative analysis of promoter strength, nine constructed recombinant strains (designated WB-D3P1 to WB-D3P9) were evaluated by RT-qPCR analysis to determine the relative transcription levels of SfDAE. Compared with WB-D3P1, the relative mRNA levels of SfDAE produced by P amyE and P 43 were significantly increased in the recombinant strains WB-D3P4 and WB-D3P5, while the transcriptional activity of P spovG and P srfA was similar in WB-D3P2 and WB-D3P7 (Figure 4A).…”

Section: Functional Expression Of Sfdae For Biosynthesis Of D-allulos...mentioning

confidence: 99%

Fine-Tuning of Carbon Flux and Artificial Promoters in Bacillus subtilis Enables High-Level Biosynthesis of d-Allulose

Zhang

Wei

Sun

et al. 2022

D-Allulose is an attractive rare sugar that can be used as a low-calorie sweetener with significant health benefits. To meet the increasing market demands, it is necessary to develop an efficient and extensive microbial fermentation platform for the synthesis of D-allulose. Here, we applied a comprehensive systematic engineering strategy in Bacillus subtilis WB600 by introducing Dallulose 3-epimerase (DAEase), combined with the deactivation of fruA, levDEFG, and gmuE, to balance the metabolic network for the efficient production of D-allulose. This resulting strain initially produced 3.24 g/L of D-allulose with a yield of 0.93 g of Dallulose/g D-fructose. We further screened and obtained a suitable dual promoter combination and performed fine-tuning of its spacer region. After 64 h of fed-batch fermentation, the optimized engineered B. subtilis produced D-allulose at titers of 74.2 g/L with a yield of 0.93 g/g and a conversion rate of 27.6%. This D-allulose production strain is a promising platform for the industrial production of rare sugar.

“…subtilis for d -allulose production using an autoinducible promoter engineering and a tandem DAEase synergistic expression with Dorea sp. DAEase and Clostridium cellulolyticum DAEase . Liu et al enhanced DAEase expression through protein engineering and catabolite-responsive element box (CRE) engineering .…”

Section: Introductionmentioning

confidence: 99%

Enhancement of the d-Allulose 3-Epimerase Expression in Bacillus subtilis through Both Transcriptional and Translational Regulations

Zhang,

Ren,

Chen

et al. 2024

D-Allulose, a functional bulk sweetener, has recently attracted increasing attention because of its low-caloric-ness properties and diverse health effects. D-Allulose is industrially produced by the enzymatic epimerization of D-fructose, which is catalyzed by ketose 3-epimerase (KEase). In this study, the food-grade expression of KEase was studied using Bacillus subtills as the host. Clostridium sp. D-allulose 3-epimerase (Clsp-DAEase) was screened from nine D-allulose-producing KEases, showing better potential for expression in B. subtills WB600. Promoter-based transcriptional regulation and N-terminal coding sequence (NCS)based translational regulation were studied to enhance the DAEase expression level. In addition, the synergistic effect of promoter and NCS on the Clsp-DAEase expression was studied. Finally, the strain with the combination of a P HapII promoter and gln A-Up NCS was selected as the best Clsp-DAEase-producing strain. It efficiently produced Clsp-DAEase with a total activity of 333.2 and 1860.6 U/mL by shake-flask and fed-batch cultivations, respectively.