A functional peptide derived from pearls and its application
A technology of functional peptides and leucine, applied in the field of marine biological functional peptides, can solve problems such as limitations, restrictions on accurate quality control technology, and difficulty in improving product levels, and achieve good free radical effects
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Embodiment 1
[0019] Embodiment 1: Preparation of pearl enzymatic protein
[0020] 1. Raw materials and reagents
[0021] The pearl powder in the examples was provided by Guangzhou Qifu Pearl Processing Co., Ltd., passed through a 200-mesh sieve, packed in bags and sealed, and stored at -20°C.
[0022] Bromelain (enzyme activity of 400,000 U / g) was purchased from Guangbo Nanning Pangbo Bioengineering Co., Ltd.; cutinase (enzyme activity of 200,000 U / g) was purchased from Jinan Zhuodai Biotechnology Co., Ltd.; DEAE-52 Cellulose cation exchange resin was purchased from Whatman Company, and Sephadex G-15 gel resin was purchased from GE Company. Ethanol, formaldehyde, isopropanol, sodium hydroxide, disodium hydrogen phosphate, sodium dihydrogen phosphate and other reagents were of domestic analytical grade. The test water is ultrapure water.
[0023] 2. Pearl protein preparation
[0024] Weigh about 100g of pearl powder, add 100mL of water, 50mL of ethanol and stir well. Slowly add 3M hydr...
Embodiment 2
[0027] Example 2 Separation and Preparation of Novel Functional Peptides from Pearl Enzymolysis Protein
[0028] 1. Take 3 g of pearl hydrolyzed protein obtained from enzymatic hydrolysis in Example 1, dissolve it in 100 mL of water to make a sample solution, filter it with an ultrafiltration membrane with a molecular weight cut-off of 3 kDa, freeze-dry the retained part and the filtrate respectively, and obtain two samples: PPH- I (molecular weight>3kDa), PPH-II (molecular weight50 = 4.5 mg / mL, EC of PPH-II 50 =40.5mg / mL, accordingly select the more active component PPH-I to continue to separate.
[0029] 2. Separation of PPH-I with G15 gel column to obtain four component fragments PPH-I-1-4, after freeze-drying respectively, detect the EC of DPPH free radical scavenging activity 50 The values are 7.53mg / ml, 7.33mg / ml, 5.88mg / ml, 10.461mg / ml respectively.
[0030] Described G15 gel column separation, its condition is: get PPH-I sample 1g to be dissolved in 5mL deionized w...
Embodiment 3
[0036] Example 3. Determination of DPPH radical scavenging effect.
[0037] In this experiment, the DPPH test was used to evaluate the free radical scavenging ability of the samples. According to the literature (Hsu, K.C.; Lu, G.H.; Jao, C.L., Antioxidative properties of peptides prepared from tuna cookingjuice hydrolysates with orientase (Bacillus subtilis). Food Research International 2009, 42, (5-6), 647-652.) method , Determining the ability of scavenging DPPH free radical activity of pearl protein hydrolyzate. According to the preset initial concentration, take a corresponding amount of sample dissolved in water to obtain a sample solution, take 100 μl of the sample solution and add it to the first row of a 96-well plate, dilute the concentration gradient with ultrapure water, and then add 100 μl of the sample solution to a concentration of 2x10 - 4 mol / L DPPH ethanol solution, three parallel experiments were done for each concentration, and the blank test was made of a...
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