Isolation and characterisation of esterases from thermophilic Actinomyces

Isolation and characterisation of esterases from thermophilic Actinomyces

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<p>Alternative sources of fuel are required worldwide, and bio-ethanol is the leading candidate. Lignocellulosic biomass, a waste component of the agricultural industry, is a promising renewable source. Due to its complex structure it is highly recalcitrant, requiring the synergistic action of...

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Main Author: Oldale, Megan
Format: Others
Language:English
Published: 2010
Subjects:
Actinomyces
Thermophilic fungi
Enzymes.
Online Access:http://etd.uwc.ac.za/index.php?module=etd&action=viewtitle&id=gen8Srv25Nme4_7994_1306756744
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spelling ndltd-UNWC-oai-UWC_ETD-http%3A%2F%2Fetd.uwc.ac.za%2Findex.php%3Fmodule%3Detd%26action%3Dviewtitle%26id%3Dgen8Srv25Nme4_7994_13067567442013-01-08T12:42:22Z Isolation and characterisation of esterases from thermophilic Actinomyces Oldale, Megan Actinomyces Thermophilic fungi Enzymes. <p>Alternative sources of fuel are required worldwide, and bio-ethanol is the leading candidate. Lignocellulosic biomass, a waste component of the agricultural industry, is a promising renewable source. Due to its complex structure it is highly recalcitrant, requiring the synergistic action of a battery of enzymes to achieve complete digestion. These enzymes include cellulases, hemicellulase and the accessory enzymes acetyl xylan esterase (AXE) and ferulic acid esterase (FAE). Thermpohilic Actinomyces isolates with the ability to hydrolyze xylan were screened for esterase activity. Two isolates (ORS10 and GSIV1), identified as Streptomyces spp, were positive for AXE activity. A cosmid library representative of isolate ORS10 was composed and screened for AXE activity using -naphthyl acetate as substrate. An 18 kb cosmid clone, 18D7, tested positive for AXE activity. Intracellular fractions extracted from ORS10 were precipitated with ammonium sulphate and partially purified 161-fold. Specific activity was measured after dialysis and ion-exchange chromatography. Overall yield of the partially purified enzyme was 34 %. Two protein bands of molecular masses 40 kDa and 60 kDa have been subjected to trypsin digestion and MALDI-TOF mass spectrometry analysis. The partially purified AXE displayed optimum activity at pH 9 and at 50&deg C. AXE activity was stable for at least 1.5 hours between 30&deg C and 40&deg C, and for 24 hours between pH 6-9. The kM and Vmax values were 16.93 mg/ml and 1645 units/mg enzyme, respectively. The stability of the partially purified AXE at 30&deg C-40&deg C suggests potential for industrial applications that utilise mesophilic fermentations.</p> 2010 Thesis and dissertation Pdf http://etd.uwc.ac.za/index.php?module=etd&action=viewtitle&id=gen8Srv25Nme4_7994_1306756744 English ZA Copyright: University of the Western Cape
collection NDLTD
language English
format Others
sources NDLTD
topic Actinomyces
Thermophilic fungi
Enzymes.
spellingShingle Actinomyces
Thermophilic fungi
Enzymes.
Oldale, Megan
Isolation and characterisation of esterases from thermophilic Actinomyces
description <p>Alternative sources of fuel are required worldwide, and bio-ethanol is the leading candidate. Lignocellulosic biomass, a waste component of the agricultural industry, is a promising renewable source. Due to its complex structure it is highly recalcitrant, requiring the synergistic action of a battery of enzymes to achieve complete digestion. These enzymes include cellulases, hemicellulase and the accessory enzymes acetyl xylan esterase (AXE) and ferulic acid esterase (FAE). Thermpohilic Actinomyces isolates with the ability to hydrolyze xylan were screened for esterase activity. Two isolates (ORS10 and GSIV1), identified as Streptomyces spp, were positive for AXE activity. A cosmid library representative of isolate ORS10 was composed and screened for AXE activity using -naphthyl acetate as substrate. An 18 kb cosmid clone, 18D7, tested positive for AXE activity. Intracellular fractions extracted from ORS10 were precipitated with ammonium sulphate and partially purified 161-fold. Specific activity was measured after dialysis and ion-exchange chromatography. Overall yield of the partially purified enzyme was 34 %. Two protein bands of molecular masses 40 kDa and 60 kDa have been subjected to trypsin digestion and MALDI-TOF mass spectrometry analysis. The partially purified AXE displayed optimum activity at pH 9 and at 50&deg === C. AXE activity was stable for at least 1.5 hours between 30&deg === C and 40&deg === C, and for 24 hours between pH 6-9. The kM and Vmax values were 16.93 mg/ml and 1645 units/mg enzyme, respectively. The stability of the partially purified AXE at 30&deg === C-40&deg === C suggests potential for industrial applications that utilise mesophilic fermentations.</p>
author Oldale, Megan
author_facet Oldale, Megan
author_sort Oldale, Megan
title Isolation and characterisation of esterases from thermophilic Actinomyces
title_short Isolation and characterisation of esterases from thermophilic Actinomyces
title_full Isolation and characterisation of esterases from thermophilic Actinomyces
title_fullStr Isolation and characterisation of esterases from thermophilic Actinomyces
title_full_unstemmed Isolation and characterisation of esterases from thermophilic Actinomyces
title_sort isolation and characterisation of esterases from thermophilic actinomyces
publishDate 2010
url http://etd.uwc.ac.za/index.php?module=etd&action=viewtitle&id=gen8Srv25Nme4_7994_1306756744
work_keys_str_mv AT oldalemegan isolationandcharacterisationofesterasesfromthermophilicactinomyces
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