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Preparation method for producing pig haemocyte active small peptide powder through one-step method

A technology of active small peptides and porcine blood cells, which is applied in the field of animal blood protein deep processing, can solve the problems of simplicity and operability, insufficient nutritional value and functionality of products, no report on active small molecular peptide content, and easy denaturation of hemoglobin. Achieve the effect of improving animal immunity and disease resistance, easy absorption and utilization, and low cost

Inactive Publication Date: 2016-08-17
陈石良
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  • Abstract
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  • Claims
  • Application Information

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Problems solved by technology

However, this technical method requires two-step enzymatic hydrolysis treatment, especially in the acidic protease hydrolysis process, under acidic conditions (PH2-3) part of hemoglobin is prone to denaturation, and precipitates together with heme, and is removed by centrifugation. The recovery rate of protein is low, especially the loss of organic porphyrin iron (heme iron), which is an important source of iron supplementation for animals. At the same time, due to the repeated adjustment of the pH value, more salt is brought in, resulting in a relatively low ash content in the prepared product. High, the content of active small molecule peptides (relative molecular weight between 180 and 1000Da) in the product has not been reported
CN201410547593.3 discloses a preparation method of porcine blood globulin powder, using whole porcine blood as raw material, preparing porcine blood hemoglobin liquid through centrifugation and ultrasonic treatment, and then performing physical deoxygenation, ultrasonic treatment, and compound enzyme separation on the hemoglobin liquid in sequence Stage enzymatic hydrolysis, activated carbon decolorization, membrane ultrafiltration concentration, spray drying and other complex process processes, and finally milky white porcine hemoglobin polypeptide powder and heme peptide, although this method completely removes the color of hemoglobin polypeptide powder And bloody smell, the sensory properties of the product have been greatly improved, and the digestion and absorption rate of protein has been improved, but it requires multiple ultrasonic treatments, segmental enzymatic hydrolysis, repeated centrifugation, and decolorization and concentration. The process is cumbersome and the cost is high. Protein peptide powder, does not contain active small molecular peptides, and the economic value is not high
Therefore, the prior art solutions have deficiencies both in the ease and operability of the preparation process and in the nutritional value and functionality of the product.

Method used

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  • Preparation method for producing pig haemocyte active small peptide powder through one-step method
  • Preparation method for producing pig haemocyte active small peptide powder through one-step method
  • Preparation method for producing pig haemocyte active small peptide powder through one-step method

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Effect test

Embodiment 1

[0028] (1) Preparation of porcine blood cells: collect 1000L of fresh pig blood that has been anticoagulated, and use a tubular centrifuge to continuously centrifuge to obtain 440L of blood cells and 560L of plasma, collect the blood cells, and spray dry the plasma to make plasma protein powder Add food-grade sodium citrate during anticoagulant treatment, the addition amount is 0.4% of fresh pig blood weight, the sodium citrate that weighs is mixed with 10% sodium citrate solution first, then in the process of collecting fresh pig blood Slowly add the sodium citrate solution while stirring;

[0029] (2) Hemolysis: pump the blood cell solution into the reaction tank, add 440L of deionized water, and stir continuously for 60 minutes to break the blood cells. The stirring speed is 30r / min, and 880L of hemolysis is obtained;

[0030] (3) Enzymolysis: Heat the hemolysis to 50°C with continuous stirring, adjust the pH value to 8.5 with NaOH solution, then add 0.4% protease (enzyme act...

Embodiment 2

[0036] (1) Preparation of pig blood cells: collect 2000L of fresh pig blood that has been anticoagulated, and use a tubular centrifuge to continuously centrifuge to obtain 850L of blood cells and 1150L of plasma. Add food-grade sodium citrate during anticoagulant treatment, and the addition amount is 0.5% of fresh pig blood weight. Slowly add the sodium citrate solution while stirring;

[0037] (2) Hemolysis: pump the blood cell solution into the reaction tank, add 850L of deionized water, and stir continuously for 60 minutes to break the blood cells. The stirring speed is 50r / min to prepare 1700L of hemolysis;

[0038] (3) Enzymolysis: Heat the hemolysis to 55°C with continuous stirring, adjust its pH value to 8.5 with NaOH solution, then add 0.3% protease (enzyme activity 200,000U / ml) by weight of the blood cell solution, and keep stirring, every interval Check the pH value of the enzymolysis solution for one hour. When the pH value drops below 8.0, adjust the pH value of t...

Embodiment 3

[0044] (1) Preparation of porcine blood cells: collect 5000L of fresh pig blood that has been anticoagulated, and use a tubular centrifuge to continuously centrifuge to obtain 2160L of blood cells and 2840L of plasma, collect the blood cells, and spray dry the plasma to make plasma protein powder Add food-grade sodium citrate during anticoagulant treatment, and the addition amount is 0.5% of fresh pig blood weight. Slowly add the sodium citrate solution while stirring;

[0045] (2) Hemolysis: pump the blood cell solution into the reaction tank, add 2200L of deionized water, and stir continuously for 60 minutes to break the blood cells. The stirring speed is 50r / min to prepare 4360L of hemolysis;

[0046] (3) Enzymolysis: Heat the hemolysis to 55°C with continuous stirring, adjust the pH value to 8.5 with NaOH solution, then add 0.2% protease (enzyme activity 200,000U / ml) by weight of the blood cell solution, keep stirring, every interval Check the pH value of the enzymolysis ...

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Abstract

The invention relates to a preparation method for producing pig haemocyte active small peptide powder through a one-step method. The preparation method mainly comprises the steps of collecting fresh pig blood subjected to anticoagulation treatment, conducting centrifugal separation to obtain haemocyte liquid, conducting hemolysis, enzymolysis and centrifugation to obtain enzymatic hydrolysate, conducting ultrafiltration membrane filtration and nanofiltration membrane concentration on the enzymatic hydrolysate, and then conducting spray drying, so that the pig haemocyte active small peptide powder is obtained. According to the preparation method, efficient endo protease is selected, the one-step method is adopted, the ultrafiltration membrane and nanofiltration membrane separation technology is combined, the process procedure is simple, the production cycle is short, production efficiency is high, cost is low, and the preparation method is suitable for large-scale industrialized production. In the prepared pig haemocyte active small peptide powder, the content of active small peptide (with the relative molecular weight ranging from 180 Da to 1000 Da) reaches 75% or above, the content of organic hemin (heme iron) reaches 0.2% or above, the content of ash is lower than 5.0%, and the content of free amino acid is lower than 11%. The product can promote growth of animals and enhance immunity and disease resistance of animals and is a novel functional protein feed raw material.

Description

technical field [0001] The invention relates to the technical field of deep processing of animal blood protein, in particular to a preparation method for producing porcine blood cell active small peptide powder by one-step enzymatic hydrolysis. Background technique [0002] According to the number of amino acid residues, peptides can be divided into polypeptides, oligopeptides, and small peptides. Generally speaking, those containing more than 50 amino acid residues are usually called proteins, those with less than 50 and more than 10 amino acid residues are called polypeptides, and those with less than 10 amino acid residues are called oligopeptides. Small peptides refer to dipeptides, tripeptides and tetrapeptides with a relative molecular weight between 180 and 1000 Da. A large number of studies have shown that there is a small peptide absorption mechanism in animals, and small peptides can enter the body circulation through intestinal mucosal cells intact. Animals abso...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C07K14/805C12P21/06C07K1/34
CPCC07K14/805C12P21/06
Inventor 陈石良
Owner 陈石良
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