Enterobacter aerogenes zjb-17003 and its application
A ZJB-17003, Enterobacter aerogenes technology, applied in bacteria, microorganisms, microorganisms and other directions, can solve the problems of unconverted D-glufosinate-ammonium, waste of raw materials, large amount of catalyst, etc., achieves important application prospects, and is easy to cultivate and collect Application, effect of mild catalytic reaction conditions
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Embodiment 1
[0034] Example 1: Screening of Enterobacter aerogenesa ZJB-17003
[0035] 1. Primary screening
[0036] The present invention takes soil samples from all over the country, and takes 80 parts of soil samples altogether. The specific method of screening: Weigh 1g of soil sample and place it in 10mL of 0.85% physiological saline, shake it and let it stand still, take the supernatant into the enrichment medium, and cultivate it at 30°C and 150r / min for 2-3 days with shaking . Take 1mL of the enrichment solution and add it to 50mL of fresh enrichment medium, and repeat this process 3 times before separation and purification.
[0037] Bromothymol blue filter paper was selected as the indicator filter paper to detect the colony capable of degrading the substrate. The principle is: after the colony containing the target enzyme degrades the substrate, acidic by-products (phenylacetic acid, acetic acid, formic acid, benzoic acid) will be produced, thereby changing the local pH value ...
Embodiment 2
[0053] Embodiment 2: identification of bacterial strain ZJB-17003
[0054] 1. Morphological identification:
[0055] The bacterial strain ZJB-17003 screened in Example 1 of the present invention was inoculated on a solid medium and cultured at 37°C for 24 hours to form round or nearly round, soft texture, smooth surface, flat, neat edges, and shiny milky white colonies , 2-4mm in diameter. Observation by Gram staining: short pink rods without spores. Composition of solid medium: sodium chloride 10g / L, peptone 10g / L, yeast powder 5g / L, agar 20g / L, solvent is deionized water.
[0056] 2. Physiological and biochemical identification:
[0057] Using the Biolog (GENⅢ) automatic microbial identification system, 94 kinds of phenotypic tests were carried out on the strain ZJB-17003, including 71 kinds of carbon source utilization detection and 23 kinds of chemical sensitivity detection: the strain ZJB-17003 was inoculated on the BUG plate medium ( BIOLOG UNIVERSAL GROWTH AGAR), cu...
Embodiment 3
[0067] Embodiment 3: the preparation of wet thalline
[0068] (1) Incline cultivation:
[0069] Enterobacter aerogenes (Enterobacter aerogenesa) ZJB-17003 was inoculated into the slant culture medium and cultured at 30°C for 48 hours to obtain slant cells;
[0070] The final concentration of the slant culture medium is: mannitol 10g / L, sodium glutamate 7g / L, yeast extract 3g / L, K 2 HPO 4 0.75g / L, KH 2 PO 4 0.75g / L, MgSO 4 0.5g / L, caprolactam 1g / L, agar 20.0g / L, solvent is deionized water, pH 7.0~7.5.
[0071] (2) Seed cultivation
[0072] Pick an inoculation loop of bacteria from the slant and inoculate it into the seed medium, and cultivate it at 30°C for 24 hours to obtain the seed liquid;
[0073] The final concentration of the seed medium consists of: mannitol 10g / L, sodium glutamate 7g / L, yeast extract 3g / L, K 2 HPO 4 0.75g / L, KH 2 PO 4 0.75g / L, MgSO 4 0.5g / L, caprolactam 1g / L, solvent is deionized water, pH 7.0~7.5.
[0074] (3) Fermentation culture
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