RU2052253C1 - Method of preparing bacterial ferment for lactic acid product - Google Patents

Abstract

FIELD: milk industry. SUBSTANCE: method involves preparing hydrolyzate-milk medium which contains skimmed milk hydrolyzate and prepared mixture is mixed with glacial acetic acid, boiled, filtered, sterilized and 24 hr-old culture of bifidobacteria and/or lactobacteria, and/or lactic acid streptococci were added to prepared hydrolyzate-milk medium and cultivated. Before sterilization enriched hydrolyzate amino acid mixture can be added to the hydrolyzate-milk medium at concentration 1-3% of medium volume. Also, before sterilization fir residues or honey or honey mixture with fir residues can be added to the hydrolyzate-milk medium at the ratio (0.5-2.0): (1-2) at concentration 1-3% of ferment volume. EFFECT: improved method of preparing. 3 cl, 3 tbl

Description

 The invention relates to the dairy industry and can be used in the production of starter cultures for the preparation of therapeutic and dietary products.

 At the same time, produced starter cultures can be used as an independent product of therapeutic and dietary nutrition, as well as biologically valuable food additives.

A known method of producing yeast containing bifidobacteria, lactobacilli, thermophilic streptococci. For example, a method of producing starter culture to produce an adapted fermented milk product. These microorganisms increase the dietary properties and biological value of the product. The disadvantage of this method is the possibility of seeding of manufactured products by extraneous microflora, which is due to the sparing sterilization regime, as well as the reduced number and biological activity of lacto and bifidobacteria (10 ⁷ -10 ⁸ microbial bodies per ml.), Due to the use of lysozyme. The result is a short shelf life (1-2 days).

 The closest technical solution to the claimed one is a method of preparing a starter culture to produce fermented milk bifidumbacterin in dairy kitchens.

A known method of preparing yeast includes the following stages:
preparation of a hydrolyzate-milk medium (GM medium) based on a hydrolyzate of skim milk (skim milk) and its sterilization;
introducing bacteria into the sterile environment and GM-cultivation at 37.5-38 ^{° C} for 24 hours in a test tube;
reseeding of bacterial cultures from test tubes into vials in the amount of 3-5% of seed to volume.

The GM medium has the following composition: 500 ml hydrolyzate of distilled water Distilled water 500 ml of NaCl to 5% (taking into account
chloride volume
in hydrolysis
those) Lactose 10 g L-cystine hydrochloric acid 100 mg Peptone 2 g Agar agar 750 mg
Preparation of the GM environment is as follows: boil the return for 2-3 minutes; cooled to 45 ^about ; set the pH to 8.0 with 10-20% sodium hydroxide solution; carry out enzymatic hydrolysis using pancreatin (1 g / l) for 4 hours with periodic pH adjustment to 7.0-8.0; add chloroform 1-2% incubated at 37 ^about C for 14-16 hours; adjust the pH to 4.5 with a 30% solution of acetic acid; boil for 15 minutes; filtered through a paper filter. The resulting hydrolyzate is stored for 6-8 months under chloroform (1% by volume) and is used as needed. Next, the hydrolyzate is diluted with water 1: 1, agar-agar is added at the rate of 750 mg per 1 liter of solution and melted. NaCl, peptone are added to the remaining part, heated to 80 ^° C and combined with molten agar. The pH is adjusted to 7.5-7.6, boiled for 15 minutes, allowed to stand, drained from the precipitate without filtering, adjusted to 1 liter with hot distilled water, lactose, cysteine or hydrochloric cystine (water soluble) are added, sterilized at 0.5 atm. 30 min, the pH of the finished medium is 7.2-7.4. A daily culture of bifidobacteria is introduced into the GM medium prepared in this way at the rate of 3-5% of seed to the volume of medium. Seeding was kept at 37 ^{° C} for 18-20 h. The obtained leaven has the form of a turbid liquid of light brown color with a sour taste. 1 ml of starter culture contains at least 10 ⁷ -10 ⁸ live bacteria. The product has a fairly high antagonistic activity to pathogenic and conditionally pathogenic microbes. However, for the treatment of a number of diseases, especially acute infectious processes, an even higher antagonistic activity is required. The disadvantage of this method is also a rather short shelf life of the starter culture (1-2 days).

 The aim of the invention is to increase the shelf life and improve the therapeutic and dietary properties of the starter culture.

 A method of producing a starter culture is as follows.

 A hydrolyzate of a skim milk is prepared, which is mixed with glacial acetic acid, boiled, filtered, a hydrolyzate is prepared for the dairy medium, fir extracts or honey are added to it, or a mixture of the latter with fir extracts in a ratio of 0.5: (2.0-1.0): 2.0 in the amount of 1-3% of the fermentation volume. In the hydrolyzate-milk environment, you can enter a mixture of amino acids hydrolyzed enriched in an amount of 1-3% by volume of the medium. Daily medium and / or bifidobacteria and / or lactobacilli and / or thermophilic lactic acid streptococci are introduced into the resulting medium.

 As seed, cultures of strains of Lactobacterium plantarum 8 TIMES, Lactobacter can be used. plantarum 296 D, Lactobacillus acidophilus, Bifidum longum 379 M, Bifidum 791, Bifidum 1, Streptococcus thermophilis.

Sowing crops is first carried out in test tubes that are incubated at 37.5-38 ^about With during the day. Then, from a test tube with pronounced growth, a bacterial culture is subcultured in an amount of 1-5% of seed by volume into vials with a sterile GM medium prepared by the indicated method.

Studies have shown that the leaven obtained by the proposed method is characterized by a higher titer of lactic acid bacteria (10 ⁹ against 10 ⁸ microbial cells per ml) and their preservation in the classical form even for 15-18 days after preparation, while the leaven, obtained on a well-known GM-environment, contains lactic acid bacteria at the indicated times mainly in involutional form. In addition, when using a modified GM medium, the duration of the cultivation of bacteria in it is reduced by 2-4 hours. Extraneous microflora is absent, the shelf life of the fermenting properties is increased by 1-2 days, and the shelf life by 4-8 days (see table .1).

Exception exposure of freshly prepared skim milk hydrolyzate in the presence of chloroform at ³⁷ ° C for 12-14 hours improves the quality hydrolyzate, milk medium and accordingly to prepare a starter with a high titer of microorganisms. This eliminates the need to use chloroform as a preservative and significantly reduces the duration of the entire process cycle. Extraneous microflora never grows in the hydrolyzate prepared in a modified mode. The addition of honey or fir extracts or a mixture thereof with honey enhances the medicinal and dietary properties of the starter culture, which can be used not only for the preparation of a fermented milk product, but also as an independent medical product or biologically active food supplement. Strengthening of properties occurs due to an increase in antagonistic activity against opportunistic and pathogenic microorganisms. This increases the shelf life of the specified product up to 10-20 days (versus 1-2 days according to the known technical solution).

 The use of glacial acetic acid instead of a solution of acetic acid leads to a decrease in dilution of the nutrient medium and increase its nutritional properties.

 The main dietary supplement of fir extracts is the bottom residue after distillation of water from the aqueous extract of fir greens (paws). It is a viscous liquid of a dark color with a specific smell and taste of wood tar. Fir extracts, honey and a mixture of honey with fir extracts have a pronounced antagonistic activity against contaminating microflora while simultaneously maintaining the viability of biologically active lactic acid bacteria (up to 15-18 days). This helps to increase the healing properties and biological value of the starter culture (see table 2).

 The range of concentration of fir pomace is due to the following. When the honey content is less than 2: 0.5, the effectiveness of the mixture does not increase, and when the content is more than 2: 1, the addition of honey is impractical, as the shelf life begins to decrease compared to the addition of fir marc.

 As a source of amino acids, it is advisable to use a mixture of amino acids hydrolyzed SAG-P, which performs the function of a powerful growth factor for lactic acid bacteria. The mixture is introduced into the medium at the rate of 0.5-1% of its volume. Lower concentrations do not contribute to a noticeable increase in the titer of lactic acid bacteria, and higher concentrations significantly worsen the organoleptic properties of the product (see table 3).

 Sourdough is a daily culture of bifidobacteria, lactobacilli and thermophilic streptococci in a GM environment. If it contains fir pomace, honey and amino acids, it acquires a dark brown color and a sweet and sour taste.

 The advantage of the starter culture as an independent medical product is the possibility of its use for young children, because unlike sour-milk products, it has a liquid inviscid consistency and can be consumed through the nipple.

PRI me R 1. Method for the production of sourdough. 15 l of dye is sterilized at 1 atm for 30 minutes, a 20% sodium hydroxide solution is added to pH 8.0, then 15 g of pancreatin and 4-hour enzymatic hydrolysis is carried out. Next, the pH was adjusted to 4.5 with glacial acetic acid, boiled for 15 minutes and subjected to vacuum filtration. Then the hydrolyzate is diluted with distilled water 1: 1 and add 22.5 g of agar-agar, 150 g of NaCl, 60 g of peptone, 300 g of lactose and 3 g of cysteine. Sterilized at 0.5 atm 45 minutes with steam preheating for 30 minutes. Sterile medium is cooled to room temperature and applied to her daily culture of bifidobacteria and lactobacilli thermophilic lactic acid streptococci grown on the same medium at a ratio of seed to the volume of the medium equal to 1:20, in an amount of 3% maintained at 37 ^C. for 16 hours. The prepared sourdough is a brown muddy liquid with an acidic taste and a sour-milk smell.

The content of bifidobacteria is not less than 10 ⁹ microbial cells per ml. After storage at ⁴ ° C for 7 days leaven has not lost its original properties.

PRI me R 2. The method of production of starter culture is carried out analogously to example 1, except that the daily medium in the amount of 10% is introduced into the GM medium based on the calculation of 2% of seed to the volume of the medium, and the time of cultivation of the mixture at 37 ^about C is reduced to 5 hours. The resulting sourdough has a more acidic taste. The content of lactobacilli is not less than 10 ⁹ microbial cells per ml. Shelf life not less than 10 days.

PRI me R 3. It is carried out analogously to example 1, except that 0.9 l (3%) of fir extracts are added to the GM medium before sterilization. Sowing kept at ³⁷ ° C for 19 hours. The resulting yeast is a muddy brown liquid with a pleasant sour-bitter taste and odor of wood tar. The content of bifidobacteria in the leaven is not less than 10 ⁹ microbial cells per ml. After storage at 4-6 ^{° C} for 18 days yeast has not lost its original properties.

PRI me R 4. Carried out analogously to example 2, except that in the GM environment before sterilization contribute 0.9 l (3%) of honey. Seeding was kept at 37 ^{° C} for 7 hours.

The resulting sourdough is characterized by a sour taste. The content of lactobacilli is not less than 10 ⁹ microbial cells per ml. Shelf life not less than 18 days.

PRI me R 5. Carried out analogously to example 1, except that in the GM environment before applying the daily culture of bifidobacteria, a mixture of fir extracts and honey in a ratio of 2: 1 is added, based on the calculation of 3% of the mixture to the volume of medium. Seeding was incubated at ³⁷ ° C for 16 hours. The obtained leaven characterized sweet and sour taste and odor rosin.

PRI me R 6. Carried out analogously to example 2, except that in the GM environment before applying the daily culture of lactobacilli in the amount of 3% add a mixture of fir marc and honey in a ratio of 2: 0.5, based on the calculation of 1% mixtures to the volume of the medium. The incubation time seeding at ³⁷ ° C for 6 hours.

PRI me R 7. It is carried out analogously to example 1, except that in the GM environment before applying the daily culture of bifidobacteria in an amount of 5% add fir extracts (3% by volume), and as a water-soluble amino acid using a mixture of hydrolyzed amino acids enriched (SAG-P) (1% by volume). The incubation time ^of plating at 37 C is 15 hours.

Example 8. It is carried out analogously to example 2, except that fir extracts (1% by volume) are added to the GM medium before the daily culture of lactobacilli is added in an amount of 2%, and a hydrolyzed amino acid mixture is used as a water-soluble amino acid. enriched (SAG-P) (0.5% by volume). The incubation time at 37 ^about 5 hours

EXAMPLE EXAMPLE 9. A method of producing the leaven is carried out analogously to Example 1, except that in GM culture medium make daily Streptococcus thermophilus, on the basis of the rate of 3% inoculum medium to volume, and time of incubation of the mixture at 37 ^C. reduced to 8 hours

The resulting sourdough has a sour taste. The content of thermophilic streptococci is not less than 10 ⁹ microbial cells per ml. Shelf life not less than 10 days.

Claims (3)

 1. A METHOD FOR PRODUCING A BACTERIAL FERROUS FOR A DAIRY PRODUCT, which includes preparing a hydrolyzate-milk medium, including hydrolyzate of the skim milk, mixing the latter with acetic acid, boiling, filtering, sterilizing the resulting hydrolyzate-milk medium, introducing a microorganism of various cultures and daily culture into it that, in order to increase the shelf life and improve the medical and dietary properties of the starter culture, acetic acid is used in the form of glacial acetic acid, and from microorgan zmov use bifidobacteria and / or lactobacilli, and / or thermophilic lactic streptococci.  2. The method according to claim 1, characterized in that before sterilization, a mixture of amino acids is added to the hydrolyzate-milk medium enriched in hydrolyzate in an amount of 1 to 3% by volume of the medium.  3. The method according to claims 1 and 2, characterized in that before sterilization, fir extracts or honey, or a mixture of the latter with fir extracts in a ratio of 0.5: 2.0 - 1.0: 2 are introduced into the hydrolyzate-milk environment 0 in the amount of 1 - 3% of the volume of the starter culture.

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