Abstract

Lipolytic enzymes are produced by animals, plants and microorganisms. With their chemo-, regio-, and enantio-specific characteristics, lipolytic enzymes are important biocatalysts useful in several industrial applications. They are widely used in the processing of fats and oils, detergents, food processing, paper and cosmetics production. In this work, we used a new functional metaproteomics approach to screen sediment samples of the Indian Bakreshwar hot spring for novel thermo- and solvent-stable lipolytic enzymes. We were able to identify an enzyme showing favorable characteristics. DS-007 showed high hydrolytic activity with substrates with shorter chain length (<C8) with the maximum activity observed against p-nitrophenyl butyrate (C4). For substrates with a chain length >C10, significantly less hydrolytic activity was observed. A preference for short chain acyl groups is characteristic for esterases, suggesting that DS-007 is an esterase. Consistent with the high temperature at its site of isolation, DS-007 showed a temperature optimum at 55°C and retained 80% activity even after prolonged exposure to temperatures as high as 60°C. The enzyme showed optimum activity at pH 9.5, with more than 50% of its optimum activity between pH 8.0 and pH 9.5. DS-007 also exhibited tolerance toward organic solvents at a concentration of 1% (v/v). One percent of methanol increased the activity of DS-007 by 40% in comparison to the optimum conditions without solvent. In the presence of 10% methanol, DMSO or isopropanol DS-007 still showed around 50% activity. This data indicates that DS-007 is a temperature- and solvent-stable thermophilic enzyme with reasonable activity even at lower temperatures as well as a catalyst that can be used at a broad range of pH values with an optimum in the alkaline range, showing the adaptation to the habitat’s temperature and alkaline pH.

Highlights

  • All kingdoms of life, including animals, plants and microorganisms produce lipolytic enzymes (Carriere et al, 1994; Bhardwaj et al, 2001; Olempska-Beer et al, 2006)

  • We examined the microbiome of the sediment of the Bakreshwar hot spring, which has a temperature of 60◦C and a pH of 9.4

  • The metaproteome from an enrichment culture from this spring was screened for its lipolytic activity on a 2D gel

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Summary

Introduction

All kingdoms of life, including animals, plants and microorganisms produce lipolytic enzymes (Carriere et al, 1994; Bhardwaj et al, 2001; Olempska-Beer et al, 2006). Their chemo-, regio- and enantio-specific characteristics make them attractive catalysts used in several industrial applications (Andualema and Gessesse, 2012). They are widely used in both, low value applications, such as the processing of fats and oils, detergents, food processing, paper and cosmetics production and high value processes, such as the synthesis of fine chemicals and pharmaceuticals (Rubin and Dennis, 1997). This, and the fact that they act over a wide range of pH and temperature makes them highly attractive for intensive studies (Huang, 1984; Jaeger et al, 1994; Bornscheuer, 2000; Jaeger and Eggert, 2002)

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