Cloning and identification of a novel tyrosinase and its overexpression in Streptomyces kathirae SC-1 for enhancing melanin production | Zendy

Jing Guo | Zendy; Zhiming Rao | Zendy; Taowei Yang | Zendy; Zaiwei Man | Zendy; Meijuan Xu | Zendy; Xian Zhang | Zendy; ShangTian Yang | Zendy

Open Access

Cloning and identification of a novel tyrosinase and its overexpression in Streptomyces kathirae SC-1 for enhancing melanin production

Author(s) -

Jing Guo,

Zhiming Rao,

Taowei Yang,

Zaiwei Man,

Meijuan Xu,

Xian Zhang,

ShangTian Yang

Publication year - 2015

Publication title -

fems microbiology letters

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.899

H-Index - 151

eISSN - 1574-6968

pISSN - 0378-1097

DOI - 10.1093/femsle/fnv041

Subject(s) - tyrosinase , melanin , streptomyces , microbiology and biotechnology , recombinant dna , chemistry , cloning (programming) , enzyme , tyrosine , biochemistry , gene , molecular cloning , peptide sequence , biology , genetics , bacteria , computer science , programming language

A 30-kDa novel tyrosinase was purified to homogeneity. The Km for L-Dopa and L-tyrosine were determined as 0.42 and 0.25 mM. The 1231 bp (base pair) melC gene and its 167 bp promoter Pskmel were obtained by thermal asymmetric interlaced polymerase chain reaction based on the amino acids fragment obtained from MS results of the purified enzyme. The protein sequence of tyrosinase shows maximum identity (84%) to tyrosinase from Streptomyces galbus. The melC was introduced into S. kathirae. The melanin production and the transcriptional level of melC in recombinant S. kathirae [pIJPskmelmelC] were about 2.1-fold and 2-fold higher than the wild-type strain, respectively. The melanin concentration was maximized at 28.8 g L(-1).

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