High-density enterococcus faecalis fermentation culture medium and fermentation process thereof

A technology of high-density fermentation and fermentation medium, applied in high-density fermentation medium of Enterococcus faecalis and its fermentation process, high-density fermentation production of Enterococcus faecalis, which can solve the problem of low fermentation level, low number of viable bacteria and high price and other problems, to achieve the effect of reducing separation costs, reducing production costs, and improving production efficiency

Active Publication Date: 2017-08-11
INST OF MICROBIOLOGY JIANGXI ACADEMY OF SCI +1
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  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

During the metabolic process of Enterococcus faecalis, substances such as hydrogen peroxide and bacteriocin can also be produced, which have a certain killing effect on pathogenic bacteria, and can produce natural antibiotics, which are beneficial to the health of the organism. Currently, they are widely used in the aquaculture industry, but Traditional Enterococcus faecalis fermentation mostly uses MRS medium, which is expensive and the number of viable bacteria after fermentation is low. In the case of a fixed effective dosage of probiotics, low fermentation level equals a disguised increase in cost

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  • High-density enterococcus faecalis fermentation culture medium and fermentation process thereof
  • High-density enterococcus faecalis fermentation culture medium and fermentation process thereof
  • High-density enterococcus faecalis fermentation culture medium and fermentation process thereof

Examples

Experimental program
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Effect test

Embodiment 1

[0030] Example 1 Utilizing different carbon sources to carry out high-density fermentation of Enterococcus faecalis

[0031] Fermentation medium: soybean meal 10g / L, ammonium sulfate 2g / L, dipotassium hydrogen phosphate trihydrate 2g / L, sodium acetate trihydrate 5g / L, sodium citrate dihydrate 2g / L, magnesium sulfate heptahydrate 0.3g / L , manganese sulfate monohydrate 0.2g / L, glycerin / glucose / sucrose / starch 20g / L, adjust to pH 7.0 with 25% ammonia water.

[0032] Seed solution preparation: Streak Enterococcus faecalis glycerol strains stored at -80°C on MRS (glucose 20g / L; peptone 10g / L; yeast powder 5g / L; diammonium hydrogen citrate 2g / L; sodium acetate 5g / L; Dipotassium Hydrogen Phosphate 2g / L; Magnesium Sulfate 0.58g / L; Manganese Sulfate 0.25g / L) on the agar medium, place in a 32°C incubator and cultivate until a single colony grows; pick a full single colony to inoculate Put into MRS liquid test tube, 37°C, 50r / min shaking flask culture for 10 hours; transfer to MRS liqui...

Embodiment 2

[0035] Embodiment 2 controls the influence of different pH on high-density fermentation of Enterococcus faecalis

[0036]Fermentation medium: soybean meal 15g / L, glycerin 25g / L, ammonium sulfate 2g / L, dipotassium hydrogen phosphate trihydrate 3g / L, sodium acetate trihydrate 5g / L, sodium citrate dihydrate 3g / L, sulfuric acid heptahydrate Magnesium 0.5g / L, manganese sulfate monohydrate 0.25g / L.

[0037] Seed solution preparation: Streak Enterococcus faecalis glycerol strains stored at -80°C on MRS (glucose 20g / L; peptone 10g / L; yeast powder 5g / L; diammonium hydrogen citrate 2g / L; sodium acetate 5g / L; Dipotassium Hydrogen Phosphate 2g / L; Magnesium Sulfate 0.58g / L; Manganese Sulfate 0.25g / L) on the agar medium, place in a 33°C incubator and cultivate until a single colony grows; pick a full single colony to inoculate Put into MRS liquid test tube, 32°C, 150r / min shaking flask culture for 10 hours; transfer to MRS liquid medium with 1% inoculum amount, 37°C, 100r / min shaking cult...

Embodiment 3

[0040] The optimization of embodiment 3 most suitable alkaline pH neutralizer

[0041] Fermentation medium: soybean meal 10g / L, glycerin 20g / L, ammonium sulfate 1g / L, dipotassium hydrogen phosphate trihydrate 2g / L, sodium acetate trihydrate 8g / L, sodium citrate dihydrate 2g / L, sulfuric acid heptahydrate Magnesium 0.4g / L, manganese sulfate monohydrate 0.25g / L.

[0042] Seed solution preparation: Streak Enterococcus faecalis glycerol strains stored at -80°C on MRS (glucose 20g / L; peptone 10g / L; yeast powder 5g / L; diammonium hydrogen citrate 2g / L; sodium acetate 5g / L; Dipotassium Hydrogen Phosphate 2g / L; Magnesium Sulfate 0.58g / L; Manganese Sulfate 0.25g / L) on the agar medium, place it in a 34°C incubator and cultivate until a single colony grows; pick a full single colony to inoculate Put into MRS liquid test tube, 39°C, 200r / min shaking flask culture for 10 hours; transfer to MRS liquid medium with 1% inoculation amount, 37°C, 100r / min shaking culture for 10 hours as seed liq...

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Abstract

The invention relates to a high-density enterococcus faecalis fermentation culture medium and a fermentation process thereof. The fermentation culture medium is prepared from 20-30 g / L of glycerol, 10-15 g / L of soybean meal, 1-3 g / L of ammonium sulfate, 2-3 g / L of potassium hydrogen phosphate, 3-8 g / L of sodium acetate trihydrate, 2-4 g / L of trisodium citrate dihydrate, 0.3-0.8g / L of magnesium sulfate heptahydrate and 0.1-0.3 g / L of manganese sulfate monohydrate. The fermentation process comprises the steps that high dissolved oxygen (25%) is adopted and combined with glycerin to serve as a fermentation carbon source, the pH value of the constant sodium carbonate fermentation liquid is 5.5, the glycerol concentration is controlled to 10 g / L by adding a supplementary material in the fermentation process in a flowing mode, culture is performed for 16 hours, and then the fermentation is completed when OD (600 nm) is greater than 35, wherein the viable count of the enterococcus faecalis contained in the fermentation liquid can be up to 8*1010 CFU / mL or above. In the fermentation mode that the high dissolved oxygen is combined with the glycerin to serve as the carbon source, the lactic acid concentration in the fermentation liquid is reduced, the enterococcus faecalis contained in the fermentation liquid can be up to 8*1010 CFU / mL or above, the biomass separation cost is reduced, a production cycle is shortened, the production cost is reduced, and the production efficiency is improved.

Description

technical field [0001] The invention relates to the technical field of microbes, in particular to a high-density fermentation medium for Enterococcus faecalis and a fermentation process thereof, which are suitable for high-density fermentation production of Enterococcus faecalis. Background technique [0002] The Catalog of Feed Additives (2013) defines Enterococcus faecalis as a strain that can be added to feed, which can form a biofilm in the intestinal tract of animals, attach to the intestinal mucosa of animals, and develop, grow and reproduce. Enterococcus faecalis belongs to the normal flora in the intestinal tract of humans and animals, and can colonize effectively after entering the intestinal tract. The fermentation of Enterococcus faecalis produces lactic acid, which is beneficial to reduce the pH of the intestinal environment and inhibit the growth of harmful bacteria. During the metabolic process of Enterococcus faecalis, substances such as hydrogen peroxide and...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12N1/20A23K10/18C12R1/46
CPCC12N1/20
Inventor 袁林郭建军曾静杨罡郭浩王林庚
Owner INST OF MICROBIOLOGY JIANGXI ACADEMY OF SCI
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