Saccharification of chitin using solid-state culture of Aspergillus sp. S1-13 with shellfish waste as a substrate

Saccharification of chitin using solid-state culture of Aspergillus sp. S1-13 with shellfish waste as a substrate

Saccharification of chitin was performed in a suspension (mash) of a solid-state culture of chitinase-producing Aspergillus sp. S1-13 with acid-treated shellfish waste as a substrate. The conditions for the saccharifying reaction and the solid-state cultivation were examined from the view-point of s...

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Main Authors: Rattanakit N., Yano S., Wakayama M., Plikomol A., Tachiki T.
Format: Article
Language:English
Published: 2014
Online Access:http://www.scopus.com/inward/record.url?eid=2-s2.0-0037691506&partnerID=40&md5=15fcebad1c6e1082de98901fb02b98b7
http://cmuir.cmu.ac.th/handle/6653943832/6090
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Institution: Chiang Mai University
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spelling th-cmuir.6653943832-60902014-08-30T03:23:49Z Saccharification of chitin using solid-state culture of Aspergillus sp. S1-13 with shellfish waste as a substrate Rattanakit N. Yano S. Wakayama M. Plikomol A. Tachiki T. Saccharification of chitin was performed in a suspension (mash) of a solid-state culture of chitinase-producing Aspergillus sp. S1-13 with acid-treated shellfish waste as a substrate. The conditions for the saccharifying reaction and the solid-state cultivation were examined from the view-point of saccharification in the mash. Optimum cultivation conditions were defined: a solid-state medium consisting of 5 g of 10% lactic acid-treated crab shells (0.50-2.36 mm in size) and 3 ml of a basal medium (0.028% KH2PO4, 0.007% CaCl2·2H2O, and 0.025% MgSO4·7H2O) supplemented with 0.3% peptone was inoculated with 4 ml of spore suspension (1×107 spores/ml), and the water content of the medium was adjusted to 75%; static cultivation at 37°C for 7 d. When a culture obtained under the optimum conditions was suspended in 70 ml of 50 mM sodium phosphate-citrate buffer (pH 4.0) and incubated at 45°C for 11-13 d, 55 mM N-acetylglucosamine (GlcNAc) was formed in the solid-state culture mash, indicating that at least 33% of the initial chitin in the solid material was hydrolyzed. Through the experiments, the amounts of GlcNAc formed in the solid-state culture mash varied in a way similar to that of the water-extractable p-nitrophenyl β-D-N-acetylglucosaminide-hydrolyzing enzyme in the culture, but not to that of the colloidal chitin-hydrolyzing enzyme. GlcNAc-assimilating lactic acid bacteria, which were inoculated into the mash after or at the start of the saccharification, formed lactic acid with decreasing GlcNAc. 2014-08-30T03:23:49Z 2014-08-30T03:23:49Z 2003 Article 13891723 10.1263/jbb.95.391 JBBIF http://www.scopus.com/inward/record.url?eid=2-s2.0-0037691506&partnerID=40&md5=15fcebad1c6e1082de98901fb02b98b7 http://cmuir.cmu.ac.th/handle/6653943832/6090 English
institution Chiang Mai University
building Chiang Mai University Library
country Thailand
collection CMU Intellectual Repository
language English
description Saccharification of chitin was performed in a suspension (mash) of a solid-state culture of chitinase-producing Aspergillus sp. S1-13 with acid-treated shellfish waste as a substrate. The conditions for the saccharifying reaction and the solid-state cultivation were examined from the view-point of saccharification in the mash. Optimum cultivation conditions were defined: a solid-state medium consisting of 5 g of 10% lactic acid-treated crab shells (0.50-2.36 mm in size) and 3 ml of a basal medium (0.028% KH2PO4, 0.007% CaCl2·2H2O, and 0.025% MgSO4·7H2O) supplemented with 0.3% peptone was inoculated with 4 ml of spore suspension (1×107 spores/ml), and the water content of the medium was adjusted to 75%; static cultivation at 37°C for 7 d. When a culture obtained under the optimum conditions was suspended in 70 ml of 50 mM sodium phosphate-citrate buffer (pH 4.0) and incubated at 45°C for 11-13 d, 55 mM N-acetylglucosamine (GlcNAc) was formed in the solid-state culture mash, indicating that at least 33% of the initial chitin in the solid material was hydrolyzed. Through the experiments, the amounts of GlcNAc formed in the solid-state culture mash varied in a way similar to that of the water-extractable p-nitrophenyl β-D-N-acetylglucosaminide-hydrolyzing enzyme in the culture, but not to that of the colloidal chitin-hydrolyzing enzyme. GlcNAc-assimilating lactic acid bacteria, which were inoculated into the mash after or at the start of the saccharification, formed lactic acid with decreasing GlcNAc.
format Article
author Rattanakit N.
Yano S.
Wakayama M.
Plikomol A.
Tachiki T.
spellingShingle Rattanakit N.
Yano S.
Wakayama M.
Plikomol A.
Tachiki T.
Saccharification of chitin using solid-state culture of Aspergillus sp. S1-13 with shellfish waste as a substrate
author_facet Rattanakit N.
Yano S.
Wakayama M.
Plikomol A.
Tachiki T.
author_sort Rattanakit N.
title Saccharification of chitin using solid-state culture of Aspergillus sp. S1-13 with shellfish waste as a substrate
title_short Saccharification of chitin using solid-state culture of Aspergillus sp. S1-13 with shellfish waste as a substrate
title_full Saccharification of chitin using solid-state culture of Aspergillus sp. S1-13 with shellfish waste as a substrate
title_fullStr Saccharification of chitin using solid-state culture of Aspergillus sp. S1-13 with shellfish waste as a substrate
title_full_unstemmed Saccharification of chitin using solid-state culture of Aspergillus sp. S1-13 with shellfish waste as a substrate
title_sort saccharification of chitin using solid-state culture of aspergillus sp. s1-13 with shellfish waste as a substrate
publishDate 2014
url http://www.scopus.com/inward/record.url?eid=2-s2.0-0037691506&partnerID=40&md5=15fcebad1c6e1082de98901fb02b98b7
http://cmuir.cmu.ac.th/handle/6653943832/6090
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