4.5 Article

Expression and characterization of a new esterase with GCSAG motif from a permafrost metagenomic library

Journal

FEMS MICROBIOLOGY ECOLOGY
Volume 92, Issue 5, Pages -

Publisher

OXFORD UNIV PRESS
DOI: 10.1093/femsec/fiw046

Keywords

permafrost; metagenome; microcosm; esterase; HSL family; GCSAG motif

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Funding

  1. Russian Scientific Foundation [14-14-01115, 14-24-00114]
  2. Russian Science Foundation [14-14-01115] Funding Source: Russian Science Foundation

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As a result of construction and screening of a metagenomic library prepared from a permafrost-derived microcosm, we have isolated a novel gene coding for a putative lipolytic enzyme that belongs to the hormone-sensitive lipase family. It encodes a polypeptide of 343 amino acid residues whose amino acid sequence displays maximum likelihood with uncharacterized proteins from Sphingomonas species. A putative catalytic serine residue of PMGL2 resides in a new variant of a recently discovered GTSAG sequence in which a Thr residue is replaced by a Cys residue (GCSAG). The recombinant PMGL2 was produced in Escherichia coli cells and purified by Ni-affinity chromatography. The resulting protein preferably utilizes short-chain p-nitrophenyl esters (C4 and C8) and therefore is an esterase. It possesses maximum activity at 45. C in slightly alkaline conditions and has limited thermostability at higher temperatures. Activity of PMGL2 is stimulated in the presence of 0.25-1.5 M NaCl indicating the good salt tolerance of the new enzyme. Mass spectrometric analysis demonstrated that N-terminal methionine in PMGL2 is processed and cysteine residues do not form a disulfide bond. The results of the study demonstrate the significance of the permafrost environment as a unique genetic reservoir and its potential for metagenomic exploration.

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