Super engineering bacteria, expressed detoxification enzyme thereof, and construction method and application therefor
A super-engineering and construction method technology, applied in the direction of botany equipment and methods, microorganism-based methods, biochemical equipment and methods, etc., can solve the problems of pesticide residue pollution, people's health hazards, etc., and achieve the effect of broadening the degradation spectrum
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Embodiment 1
[0051] Example 1, construction of super engineered bacteria expressed by the recombinant plasmid pETDuet-CYP-POR of the present invention
[0052] The cloning of the super engineered bacteria containing the genes of cytochrome oxidoreductase P450 CYP9G2 and cytochrome P450 reductase provided by the present invention is as follows:
[0053] 1.1 Plasmid and recipient bacteria
[0054] Cloning of Plutella xylostella CYP9G2 Gene
[0055] 1) Extraction of total RNA
[0056] 1-1) According to the operating procedures of the TRIzol kit, extract the total RNA of diamondback moth larvae: 2RT-PCR reaction
[0057] 1-2) Perform a PCR reaction using the reverse-transcribed first-strand cDNA as a template, add the following reagents to the PCR reaction tube, and gently mix the reaction system;
[0058] 10×PCR buffer 2.5μl
[0059] 50mM MgCl 2 0.75μl
[0060] 10mM dNTPs mixture 0.5μl
[0061] Forward primer (10μM) 0.5μ1
[0062] Reverse primer (10μM) 0.5μl
[0063...
Embodiment 2
[0125] Embodiment 2, Detoxifying enzyme of the present invention is to the determination of the degradative effect of fenitrothion (fenitrothion), dimethoate (dimethoate), methyl parathion (methyl parathion) etc.
[0126] Add 20ml of water and 1ml of 2% TritonX-100 to a 100ml Erlenmeyer flask, add an appropriate amount of ethanol solution of pesticides, so that the final concentration of pesticides is 10ppm, add 0.02M, pH7.0 phosphate buffer to make up the volume, so that the total volume is 10mL . After fully mixing it, add 4 mL of the detoxifying enzyme crude enzyme solution prepared in Example 1 (approximately 30 mg of total protein), and shake on a shaker at 30°C-32°C. Samples were taken at 0min, 20min, 40min, 60min, 80min and 120min. Two repetitions were taken at each time point, and the CYP9G2 P450 single-expressing P450 9G2 enzyme prepared in Example 1 was used as the control group in the experiment. Take out 1ml of the treatment solution and put it in a 5ml test tube...
Embodiment 3
[0133] Embodiment 3, detoxification enzyme of the present invention is to the mensuration of the degradative effect of carbamate insecticide
[0134] Add 20ml of water and 1ml of 2% TritonX-100 to a 100ml Erlenmeyer flask, add an appropriate amount of ethanol solution of pesticides, so that the final concentration of fenitrothion pesticide is 10ppm, add 0.02M, pH 7.0 phosphate buffer to make up the volume, so that the total The volume is 10 mL. After fully mixing it, add 4 mL of the detoxifying enzyme crude enzyme solution prepared in Example 1 (approximately 30 mg of total protein), and shake on a shaker at 30°C-32°C. Samples were taken at 0min, 20min, 40min, 60min, 80min and 120min. Two repetitions were taken at each time point, and the CYP9G2 P450 single-expressing P450 9G2 enzyme prepared in Example 1 was used as the control group in the experiment. Take out 1ml of the treatment solution and put it in a 5ml test tube, add 1ml of redistilled n-hexane, shake it on the mixe...
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