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Development of a PYRG mutant of aspergillus oryzae strain S1 as a host for the production of heterologous proteins

Oh, Selina Siew Ling and Storms, Reginald and Yun, Zheng and Mohd. Rodzi, Mohd. Rohaizad and Mahadi, Nor Muhammad and Md. Illas, Rosli and Abdul Murad, Abdul Munir and Abu Bakar, Farah Diba (2013) Development of a PYRG mutant of aspergillus oryzae strain S1 as a host for the production of heterologous proteins. Scientific World Journal . ISSN 1537-744X

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Official URL: http://dx.doi.org/10.1155/2013/634317

Abstract

The ease with which auxotrophic strains and genes that complement them can be manipulated, as well as the stability of auxotrophic selection systems, are amongst the advantages of using auxotrophic markers to produce heterologous proteins. Most auxotrophic markers in Aspergillus oryzae originate from chemical or physical mutagenesis that may yield undesirable mutations along with the mutation of interest. An auxotrophic A. oryzae strain S1 was generated by deleting the orotidine-5'-monophosphate decarboxylase gene (pyrG) by targeted gene replacement. The uridine requirement of the resulting strain GR6 pyrGΔ0 was complemented by plasmids carrying a pyrG gene from either Aspergillus nidulans or A. oryzae. β -Galactosidase expression by strain GR6 pyrGΔ0 transformed with an A. niger plasmid encoding a heterologous β -galactosidase was at least 150 times more than that obtained with the untransformed strain. Targeted gene replacement is thus an efficient way of developing auxotrophic mutants in A. oryzae and the auxotrophic strain GR6 pyrGΔ0 facilitated the production of a heterologous protein in this fungus

Item Type:Article
Uncontrolled Keywords:Aspergillus oryzae, fungal proteins, genetic enhancement
Subjects:T Technology > TP Chemical technology
Divisions:Chemical Engineering
ID Code:49189
Deposited By: Siti Nor Hashidah Zakaria
Deposited On:02 Dec 2015 02:10
Last Modified:27 Sep 2018 05:21

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