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  1. Ahmad Bazli Ramzi, Ku Nurul Aqmar Ku Bahaudin, Syarul Nataqain Baharum, Muhammad Lutfi Che Me, Hoe-han Goh, Maizom Hassan, et al.
    Sains Malaysiana, 2018;47:2969-2974.
    Microbial production of natural products using metabolic engineering and synthetic biology approaches often involves
    the assembly of multiple gene fragments including regulatory elements, especially when using eukaryotes as hosts.
    Traditional cloning strategy using restriction enzyme digestion and ligation are laborious and inflexible owing to the
    high number of sequential cloning steps, limited cutting sites and generation of undesired ‘scar’ sequences. In this study,
    a homology-based isothermal DNA assembly method was carried out for one-step simultaneous assembly of multiple DNA
    fragments to engineer plant phenylpropanoid biosynthesis in Saccharomyces cerevisiae. Rapid construction of yeast
    plasmid harboring dual gene expression cassettes was achieved via isothermal assembly of four DNA fragments designed
    with 20 bp overlapping sequences. The rate-limiting enzyme of phenylpropanoid pathway, cinnamate 4-hydroxylase
    encoded by C4H gene from Polygonum minus was cloned in tandem with yeast promoter and terminator elements of S.
    cerevisiae for efficient construction of phenylpropanoid biosynthetic pathway in recombinant yeast. The assembled pAGCAT (C4H-ADH1t-TEF1p) shuttle plasmid and transformation of S. cerevisiae with the plant C4H gene were confirmed
    via PCR analysis. Based on these findings, the yeast shuttle plasmid harboring P. minus phenylpropanoid biosynthesis
    gene was efficiently constructed to be the starting platform for the production of plant natural products in geneticallyengineered S. cerevisiae.
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