Application of sodium glutamate in l-lysine products
A technology of sodium glutamate and lysine, applied in the field of amino acids, can solve problems such as affecting the efficiency of animal absorption and utilization, increasing the workload of animal feeding, etc.
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[0034] In the second (1) aspect of the present invention, the present invention provides a feed additive containing L-lysine, which comprises coated core particles and a coating layer coated on the coated core particles, wherein the coating layer is Rumen fat, the preparation method of coated core particle comprises:
[0035] (1) Mix the lysine salt and filler and optional sodium glutamate evenly to form a mixture;
[0036] (2) adding an adhesive solution optionally containing xylanase to the mixture obtained in step (1), and mixing evenly to form a soft material;
[0037] (3) sieving the soft material obtained in step (2) to form coarse particles;
[0038] (4) Shot blasting the coarse particles obtained in step (3) to form round pellets; and
[0039] (5) Drying the round pellets obtained in step (4) and sieving to form coated core particles.
[0040] Preferably, the filler in step (1) is microcrystalline cellulose and / or dextrin.
[0041] Preferably, the binder in step (2...
Embodiment 1
[0155] The preparation of the expression construct of the xylanase gene of embodiment 1 mutant
[0156] According to the xylanase gene recorded in our former Chinese Patent No. 201210185883, the Arg encoding the 45th position on it is mutated into Ser, that is, the CGC at the 133-135th position of the nucleotide sequence is mutated into TCC, the mutant type The nucleotide sequence of the xylanase is shown in SEQ ID No: 1 of the sequence listing, and the amino acid sequence of the encoded xylanase is shown in SEQ ID No: 2. Then, according to the "Molecular Cloning Experiment Guide" and the operating guide of the commercial reagents used to construct the secretory expressed yeast, in short, the gene encoding the xylanase is used as a forward primer such as SEQ ID No: 3 of the sequence listing As shown (the EcoR I endonuclease site was introduced), the reverse primer was shown in SEQ ID No: 4 of the sequence table (the Not I endonuclease site was introduced) and EcoR I and Not I...
Embodiment 2
[0157] Embodiment 2 Fermentation preparation and activity determination of mutant xylanase
[0158] Inoculate the positive yeast transformant obtained in Example 1 into 50ml BMGY liquid medium (100mM potassium phosphate buffer (pH6.0), containing 1% yeast extract, 2% peptone, 1.34% yeast nitrogenous base, biological Prime 4*10 -5 %, glucose 2%, glycerol 1%), cultured at 30°C, 200rpm until OD600 reached 5.0.
[0159] Transfer the above culture to 1L BMGY liquid medium, cultivate at 30°C, 200rpm for 24 hours, add 5ml of methanol, and then continue to cultivate at 30°C, 200rpm for 8 days, during which 5ml of methanol was added every 24 hours, and the solution was controlled by ventilation. Oxygen (DO) is greater than 20%, and the pH is controlled at 6.0 (adjusted with ammonia water). After the cultivation is completed, filter with a 0.22 μm filter membrane and retain the supernatant, which is detected by SDS-PAGE to be rich in proteins corresponding to xylanase, thereby obtaini...
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