| Literature DB >> 28599919 |
Kenta Imao1, Rie Konishi2, Mayumi Kishida2, Yuuki Hirata2, Shota Segawa1, Noriko Adachi1, Rena Matsuura1, Yota Tsuge2, Takuya Matsumoto2, Tsutomu Tanaka1, Akihiko Kondo3.
Abstract
Xylooligosaccharide-assimilating Corynebacterium glutamicum strains were constructed using metabolic engineering and cell surface display techniques. First, C. glutamicum was metabolically engineered to create lysine-producing strains. Beta-xylosidase BSU17580 derived from Bacillus subtilis was then expressed on the C. glutamicum cell surface using PorH anchor protein, and enzymes involved in the xylose assimilation pathway were also expressed. Metabolic engineering had no effect on the activity of beta-xylosidase. The engineered strains efficiently consumed xylooligosaccharides and produced 12.4mM of lysine from 11.9g/L of xylooligosaccharides as the carbon source. Finally, co-expression of lysine decarboxylase enabled production of 11.6mM of 1,5-diaminopentane (cadaverine) from 13g/L of consumed xylooligosaccharides.Entities:
Keywords: 1,5-Diaminopentane; Cell surface display; Corynebacterium glutamicum; Metabolic engineering; Xylosidase
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Year: 2017 PMID: 28599919 DOI: 10.1016/j.biortech.2017.05.135
Source DB: PubMed Journal: Bioresour Technol ISSN: 0960-8524 Impact factor: 9.642