Simple enzymatic procedure for L-carnosine synthesis: Whole-cell biocatalysis and efficient biocatalyst recycling

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Abstract

β-Peptides and their derivates are usually stable to proteolysis and have an increased half-life compared with α-peptides. Recently, β-aminopeptidases were described as a new enzyme class that enabled the enzymatic degradation and formation of β-peptides. As an alternative to the existing chemical synthesis routes, the aim of the present work was to develop a whole-cell biocatalyst for the synthesis and production of β-peptides using this enzymatic activity. For the optimization of the reaction system we chose the commercially relevant β,α-dipeptide L-carnosine (β-alanine-L-histidine) as model product. We were able to show that different recombinant yeast and bacteria strains, which overexpress a β-peptidase, could be used directly as whole-cell biocatalysts for the synthesis of L-carnosine. By optimizing relevant reaction conditions for the best-performing recombinant Escherichia coli strain, such as pH and substrate concentrations, we obtained high L-carnosine yields of up to 71%. Long-time as well as biocatalyst recycling experiments indicated a high stability of the developed biocatalyst for at least five repeated batches. Application of the recombinant E. coli in a fed-batch process enabled the accumulation of L-carnosine to a concentration of 3.7 g l-1. © 2009 The Authors.

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Heyland, J., Antweiler, N., Lutz, J., Heck, T., Geueke, B., Kohler, H. P. E., … Schmid, A. (2010). Simple enzymatic procedure for L-carnosine synthesis: Whole-cell biocatalysis and efficient biocatalyst recycling. Microbial Biotechnology, 3(1), 74–83. https://doi.org/10.1111/j.1751-7915.2009.00143.x

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