Literature DB >> 16890469

Engineering a beta-carotene ketolase for astaxanthin production.

Luan Tao1, Jolanta Wilczek, J Martin Odom, Qiong Cheng.   

Abstract

A new beta-carotene ketolase gene (crtW) was cloned from an environmental isolate Sphingomonas sp. DC18. A robust and reliable color screen was developed for protein engineering to improve its activity on hydroxylated carotenoids for astaxanthin production. Localized random mutagenesis was performed on the crtW gene including the upstream ribosomal binding site (RBS). Six mutations (H96L, R203W, A205V, A208V, F213L and A215T) in the crtW gene were isolated multiple times that showed improved astaxanthin production. These mutations were localized near the conserved histidine motifs, which were proposed for binding iron required for enzymatic activity. Combination of two of the mutations (R203W/F213L) further improved astaxanthin production. One mutation at the RBS (a438t) was shown to have additional effect on improving astaxanthin production. Most of the mutants still retained high activity on beta-carotene, however, the F213L single mutant and the R203W/F213L double mutant that yielded the highest improvement for astaxanthin production showed decreased activity for canthaxanthin production.

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Year:  2006        PMID: 16890469     DOI: 10.1016/j.ymben.2006.06.001

Source DB:  PubMed          Journal:  Metab Eng        ISSN: 1096-7176            Impact factor:   9.783


  11 in total

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2.  Cloning and selection of carotenoid ketolase genes for the engineering of high-yield astaxanthin in plants.

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5.  Biosynthesis of β-carotene in engineered E. coli using the MEP and MVA pathways.

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7.  Metabolic Engineering of Escherichia coli for Producing Astaxanthin as the Predominant Carotenoid.

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8.  Manipulating the position of DNA expression cassettes using location tags fused to dCas9 (Cas9-Lag) to improve metabolic pathway efficiency.

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Review 9.  Optimization of microbial cell factories for astaxanthin production: Biosynthesis and regulations, engineering strategies and fermentation optimization strategies.

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10.  Generating in vivo cloning vectors for parallel cloning of large gene clusters by homologous recombination.

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