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A comparative analysis of recombinant expression and solubility screening of two phytases in E. coli

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dc.contributor.author Ushasree, M V
dc.contributor.author Salim, S H B
dc.contributor.author Pandey, A
dc.date.accessioned 2013-12-06T08:59:19Z
dc.date.available 2013-12-06T08:59:19Z
dc.date.issued 2011
dc.identifier.citation Food Technology and Biotechnology 49(3)Special Issue:304-309;Jul-Sep 2011 en_US
dc.identifier.issn 1330-9862
dc.identifier.uri http://ir.niist.res.in:8080/jspui/handle/123456789/902
dc.description.abstract Microbial phytases, especially from fungal and bacterial sources, have received much attention as food additives in human nutrition and as feed supplements for monogastric animals. An effective expression screening method for recombinant production of this enzyme on a small scale is industrially desirable. An effort has been made in this work to clone and express phytase genes from Aspergillus sp. and Escherichia coli with the selected host, vector and inducer combination. Albeit the formation of insoluble inclusion bodies by fungal phytase, recombinant E. coli appA was effectively expressed in a cost-effective manner in the periplasm of Bl.21plysS using an inducer concentration of 0.01 mM in 4 h of growth. Enzyme was purified in three consecutive steps and functional studies were carried out. en_US
dc.language.iso en en_US
dc.publisher Faculty Food Technology Biotechnology en_US
dc.subject Niger phytase en_US
dc.subject Inducer concentration en_US
dc.subject Escherichia-coli en_US
dc.subject Recombinant appA en_US
dc.subject Aspergillus-ficuum en_US
dc.subject Inositol phosphates en_US
dc.subject RNA-polymerase en_US
dc.subject Gene cloning en_US
dc.title A comparative analysis of recombinant expression and solubility screening of two phytases in E. coli en_US
dc.type Article en_US


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