Artificially modified glucose oxidase gene and expression application thereof
A glucose oxidase and gene technology, applied in the fields of oxidoreductase, application, genetic engineering, etc., can solve the problems of insufficient comprehensiveness of enzyme molecular structure and catalytic mechanism
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Embodiment 1
[0052] The amplification of embodiment 1 Aspergillus niger Z-25 glucose oxidase gene
[0053] 1.1 Strains and plasmids
[0054] Aspergillus niger Z-25 (Aspergillus.niger Z-25);
[0055] Escherichia coli BWTOP10 (Escherichia.coli BMTOP10) strain was purchased from Beijing Bomed Technology Development Co., Ltd.;
[0056] The synthesis of amplification primers was completed by BGI;
[0057] The sequencing vector pMD19-T was purchased from Takara Company;
[0058] 1.2 Amplification of the glucose oxidase gene
[0059] First, the genome of Aspergillus niger was extracted from the Aspergillus niger Z-25 mycelium used in the glucose oxidase fermentation experiment.
[0060] The genome of Aspergillus niger Z-25 was extracted by the improved benzyl chloride method.
[0061] (1) Suction filter the mycelial ball obtained in Chase's culture medium, and use filter paper to dry up the moisture in the culture medium as much as possible
Embodiment 2
[0077] Embodiment 2 Construction of glucose oxidase mutant gene library
[0078] 2.1 DNaseI randomly cuts the glucose oxidase gene
[0079] Firstly, use DNaseI to randomly cut the amplified glucose oxidase. DNaseI can cut any gene non-specifically. The system is as follows:
[0080] glucose oxidase gene
[0081] 2.2 Glucose oxidase fragment reunion (DNA shuffling)
[0082] Take a certain amount of glucose oxidase fragments as a substrate, add enzyme and dNTP to carry out PCR without primers, this process is the process of DNA shuffling.
[0083] The specific system is as follows:
[0084] Tag Mix
[0085] The shuffling PCR program is:
[0086] 1
[0087] 3
[0088] Then add primers to the above shuffling product to obtain the mutant group of glucose oxidase (GOD-Mtt), the specific system is as follows:
[0089] Shuffling products
[0090] In the process of reuniting glucose oxidase fragments, the biggest difficulty in the w...
Embodiment 3
[0101] Example 3 Introduction of glucose oxidase variant gene library into Pichia pastoris GS115 and its screening
[0102] 3.1 Strains and plasmids
[0103] Yeast expression strain Pichia GS115;
[0104] The shuttle expression vector pPIC9K was purchased from Invitrogen;
[0105] The sequencing vector pMD19-T was purchased from Takara Company.
[0106] 3.2 Culture medium and enzyme activity assay substrate
[0107] Refer to EasySelect for specific components of conventional medium YPD, yeast enrichment medium BMGY and yeast induction medium BMMY for yeast culture TM Pichia Expression Kit A Manual of Methods for Expression of Recombinant Proteins Using pPICZ and pPICZα in Pichia pastoris Catalog no. K1740-01.
[0108] The formulation of the 3L amplified fermentation medium for the screened high-enzyme-activity-expressing yeast refers to the composition of the medium involved in "Research on High-Density Culture Conditions for the Production of Recombinant Human Serum Albu...
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