KR100469332B1 - Method for production of glycinebetaine by yeast - Google Patents

Method for production of glycinebetaine by yeast Download PDF

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KR100469332B1
KR100469332B1 KR10-2002-0024868A KR20020024868A KR100469332B1 KR 100469332 B1 KR100469332 B1 KR 100469332B1 KR 20020024868 A KR20020024868 A KR 20020024868A KR 100469332 B1 KR100469332 B1 KR 100469332B1
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yeast
glycinebetaine
copper sulfate
culturing
producing
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KR20030086742A (en
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허남응
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(주)진바이오
허남응
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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12PFERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
    • C12P13/00Preparation of nitrogen-containing organic compounds
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N1/00Microorganisms, e.g. protozoa; Compositions thereof; Processes of propagating, maintaining or preserving microorganisms or compositions thereof; Processes of preparing or isolating a composition containing a microorganism; Culture media therefor
    • C12N1/14Fungi; Culture media therefor
    • C12N1/16Yeasts; Culture media therefor
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12PFERMENTATION OR ENZYME-USING PROCESSES TO SYNTHESISE A DESIRED CHEMICAL COMPOUND OR COMPOSITION OR TO SEPARATE OPTICAL ISOMERS FROM A RACEMIC MIXTURE
    • C12P13/00Preparation of nitrogen-containing organic compounds
    • C12P13/007Carnitine; Butyrobetaine; Crotonobetaine

Abstract

본 발명은 식물체의 삼투압조정제, 동맥 혈액질환 개선제, 가축·어류의 스트레스 완화제, 치매치료제 등에 사용되는 글리신베타인 생산 방법에 관한 것이다.The present invention relates to a glycinebetaine production method used in osmotic pressure regulators of plants, arterial blood disease improving agents, stress relief agents of livestock and fish, dementia treatment agents and the like.

본 발명에 따른 효모를 이용한 글리신베타인 생산 방법은 효모를 황산동이 첨가된 영양배지에서 1회 배양하는 과정, 상기 배양된 효모를 황산동이 배제된 영양배지에서 3 내지 5회 연속배양하여 종균을 생산하는 과정, 상기 종균을 무기염류를 함유한 사탕무 당밀액 또는 사탕무 추출액에 접종하여 배양하는 과정, 상기 배양액을 동결건조하는 과정, 상기 동결건조물에서 글리신베타인을 추출하는 과정으로 이루어진다.In the method for producing glycinebetaine using yeast according to the present invention, a process of culturing yeast in a nutrient medium to which copper sulfate is added and producing the seed by culturing the cultured yeast three to five times in a nutrient medium excluding copper sulfate The seed is inoculated with sugar beet molasses or sugar beet extract containing inorganic salts, and the step of culturing, lyophilizing the culture solution, extracting glycine betaine from the lyophilisate.

Description

효모를 이용한 글리신베타인 생산 방법{METHOD FOR PRODUCTION OF GLYCINEBETAINE BY YEAST}Glycinebetaine production using yeast {METHOD FOR PRODUCTION OF GLYCINEBETAINE BY YEAST}

본 발명은 식물체의 삼투압조정제, 동맥 혈액질환 개선제, 가축·어류의 스트레스 완화제, 치매치료제 등에 사용되는 글리신베타인을 생산하는 방법에 관한 것이다.The present invention relates to a method for producing glycine betaine used in osmotic pressure regulators of plants, arterial blood disease improving agents, stress relieving agents of animals and fish, dementia treatment agents and the like.

글리신베타인은 아래와 같은 구조식을 가진다.Glycinebetaine has the following structural formula.

글리신베타인은 종래에는 사탕무에서 추출되어 왔으나 사탕무는 농작물인 관계로 작황에 따라 사탕무의 글리신베타인 함량이 일정치 않아 균질성이 낮고, 원료의 연속적인 공급을 위해서는 저장시설이 추가로 필요하게 된다. 이에 대한 대안으로 미생물을 반응기에 배양하여 글리신베타인을 생산하는 방법이 개발되었는 바, 이는 미생물 배양을 통한 발효로 생산할 경우 원료를 안정적으로 확보할 수 있고 또 부패하기 쉬운 사탕무의 냉동 저장에 필요한 공간 및 유지비는 물론, 연속적인 발효로 균질한 제품을 생산할 수 있기 때문이다. 글리신베타인을 생산하는 미생물은 호기성 헤테로트로픽 유박테리아(heterotrophic eubacteria)중에는 유일하게 액티노폴리스포라 할로필리아(Actinopolyspora halophilia)가 알려져 있고, 그밖에 내염 및 호염성 시아노박테리아(cyanobacteria)와 같은 일부의 박테리아가 알려져 있으나, 이들 미생물들은 광합성 미생물이어서 체내 글리신베타인 축적을 유도하기 위해서는 효율적인 광합성에 필요한 고강도의 빛을 조사하는 광자가영양(photo autotroph)조건으로 배양하여야만 한다. 뿐만 아니라 이들 미생물에 의한 발효로 글리신베타인을 생산하기 위해서는 초기기질인 코린(choline)을 배양액에 추가로 첨가해 주어야 하는데, 코린(choline)은 고가이어서 종래 방법은 채산성이 낮아 상업화되지 못하고 있다.Glycine betaine has been conventionally extracted from sugar beet, but the sugar beet has a low homogeneity because the glycine betaine content of sugar beet is not constant, and storage facilities are needed for continuous supply of raw materials. As an alternative to this, a method of producing glycinebetaine by culturing microorganisms in a reactor has been developed, which is a space required for freezing storage of sugar beet, which can stably obtain raw materials, and is susceptible to decay when produced by fermentation through microbial culture. Maintenance costs, as well as continuous fermentation can produce a homogeneous product. The only microorganism that produces glycinebetaine is Actinopolyspora halophilia, the only known aerobic heterotrophic eubacteria. Although known, these microorganisms are photosynthetic microorganisms and must be cultured under photo autotroph conditions for irradiating high-intensity light for efficient photosynthesis to induce glycine betaine accumulation in the body. In addition, in order to produce glycine betaine by fermentation by these microorganisms, an initial substrate, choline, should be added to the culture solution. However, choline is expensive and conventional methods have not been commercialized due to low profitability.

본 발명은 상기와 같은 미생물을 이용한 글리신베타인 생산시의 고비용 문제를 해결하기 위하여, 고강도의 빛 및 코린을 포함하지 않고서도 글리신베타인을 합성할 수 있는 효모를 이용하여 낮은 비용으로 글리신베타인을 생산하는 방법을 제공함에 그 목적이 있다.The present invention produces glycinebeta at low cost by using a yeast that can synthesize glycinebetaine without including high intensity light and corin, in order to solve the high cost problem when producing glycinebetaine using the microorganisms as described above. The purpose is to provide a way to.

상기와 같은 목적을 달성하기 위한 본 발명의 효모를 이용한 글리신베타인 생산 방법은, 효모를 황산동이 첨가된 영양배지에서 1회 배양하는 과정, 상기 배양된 효모를 황산동이 배제된 영양배지에서 3 내지 5회 연속배양하여 종균을 생산하는 과정, 상기 종균을 무기염류를 함유한 사탕무 당밀액 또는 사탕무 추출액에 접종하여 배양하는 과정, 상기 배양액을 동결건조하는 과정, 상기 동결건조물에서 글리신베타인을 추출하는 과정에 의하여 달성될 수 있다.Glycine betaine production method using the yeast of the present invention for achieving the above object, the process of culturing yeast once in a nutrient medium with copper sulfate added, the cultured yeast in a nutrient medium without copper sulfate 3 to 3 Process of producing spawn by five consecutive cultures, inoculating the spawn with beet molasses or sugar beet extract containing inorganic salts, culturing, lyophilizing the culture, extraction of glycinebetaine from the freeze-dried Can be achieved by.

도 1은 효모를 이용한 글리신베타인의 생산 과정을 나타낸 공정도이다.1 is a process chart showing a production process of glycinebetaine using yeast.

이하, 본 발명에 따른 효모를 이용한 글리신베타인 생산 방법을 상세히 설명한다.Hereinafter, a method for producing glycinebetaine using yeast according to the present invention will be described in detail.

도 1은 효모발효를 이용한 글리신베타인의 생산과정을 나타낸 것이다.Figure 1 shows the production process of glycine betaine using yeast fermentation.

본 발명에 따른 효모를 이용한 글리신베타인 생산 방법은 효모를 황산동이 첨가된 영양배지에서 1회 배양하는 과정, 상기 배양된 효모를 황산동이 배제된 영양배지에서 3 내지 5회 연속배양하여 종균을 생산하는 과정, 상기 종균을 무기염류를 함유한 사탕무 당밀액 또는 사탕무 추출액에 접종하여 배양하는 과정, 상기 배양액을 동결건조하는 과정, 상기 동결건조물에서 글리신베타인을 추출하는 과정으로 이루어진다.In the method for producing glycinebetaine using yeast according to the present invention, a process of culturing yeast in a nutrient medium to which copper sulfate is added and producing the seed by culturing the cultured yeast three to five times in a nutrient medium excluding copper sulfate The seed is inoculated with sugar beet molasses or sugar beet extract containing inorganic salts, and the step of culturing, lyophilizing the culture solution, extracting glycine betaine from the lyophilisate.

상기 글리신베타인 생산에 이용되는 효모는 빵효모(Saccharomyces cerevisiae)로서, 바람직하게는 KCTC 1552, 1813, 7928 중 어느 하나를 사용한다. 상기 KCTC 1552, 1813, 및 7928는 한국생명공학연구원 유전자 은행실에서 구입할 수 있다.Yeast used for the production of glycinebetaine is Saccharomyces cerevisiae, and preferably any one of KCTC 1552, 1813 and 7928 is used. The KCTC 1552, 1813, and 7928 can be purchased from the Korea National Institute of Biotechnology Gene Bank.

상기 황산동첨가 배양과정에서, 상기 황산동은 10mM 황산동을 첨가하는 것이 바람직하다. 황산동을 첨가하는 이유는 효모에 인위적인 환경스트레스를 가하여 효모로 하여금 글리신베타인을 합성하도록 하는 것이다. 이것은 환경스트레스에 대한 효모의 자기보호작용에 기인하는 것으로 이해된다. 또한, 상기 영양배지는 효모배양에 일반적으로 사용되는 효모추출물, 펩톤 및 포도당으로 조성된 공시의 표준 YPD액체배지를 사용하는 것이 바람직하다.In the copper sulfate addition culture process, the copper sulfate is preferably added 10mM copper sulfate. The reason for adding copper sulfate is to apply artificial environmental stress to the yeast to allow the yeast to synthesize glycinebetaine. It is understood that this is due to yeast's self-protective action against environmental stress. In addition, it is preferable to use a standard YPD liquid medium of the composition consisting of yeast extract, peptone and glucose commonly used in yeast culture.

상기 종균 생산과정은, 상기 과정에서 배양된 효모를 황산동이 배제된 영양배지에서 연속배양하여 종균을 생산한다. 배양횟수는 3 내지 5회 연속배양하는 것이 바람직하다.In the spawn production process, the yeast cultured in the process is continuously cultured in a nutrient medium excluding copper sulfate to produce spawn. The number of cultures is preferably 3 to 5 consecutive cultures.

상기 사탕무 당밀액 또는 사탕무 추출액 접종 배양과정에 있어서, 배양 시간은 상기 효모종균을 당밀액 또는 추출액에 접종한 다음, 48 내지 120시간 배양하되 성장기 중 대수기 말 혹은 정지기 초까지 배양하는 것이 바람직하다.In the beet molasses or beet extract inoculation cultivation process, the incubation time is inoculated into the molasses or extract of the yeast, and then cultured for 48 to 120 hours, it is preferable to incubate until the end of the logarithmic phase or early phase of the growth phase .

상기 동결건조과정은 효모균체가 생산하는 글리신베타인 뿐 아니라, 사탕무 당밀액 내에 남아 있는 잔여분의 글리신베타인 또는 사탕무 추출액에 포함된 다량의 글리신베타인을 함께 추출하기 위한 것이다.The freeze-drying process is intended to extract not only glycinebetaine produced by the yeast cells, but also glycinebetaine in the remaining amount of glycinebetaine or beet extract remaining in the sugar beet molasses.

상기 글리신베타인 추출과정은, 상기 동결건조물을 최소 용적의 물로 용해시킨 후, 상기 용해액에 용해액용적의 약 4배용적의 에탄올을 첨가하고 가온하여 효모균체를 완전히 해체시키고, 12,000 ×g 하에서 원심분리하여 잔여물을 제거하고 상등액만을 추출하고, 건조시킴으로써 글리신베타인을 얻는다.In the glycine betaine extraction process, the lyophilisate is dissolved in a minimum volume of water, and then about 4 times the volume of ethanol is added to the solution and heated to completely dissolve the yeast cells, and then under 12,000 × g. Glycinebetaine is obtained by centrifugation to remove the residue, extracting only the supernatant and drying.

이하 본 발명을 실시예에 의하여 상세히 설명한다.Hereinafter, the present invention will be described in detail by examples.

다음의 실시예는 본 발명을 구체적으로 예시하는 것으로 본 발명이 실시예에 의하여 한정되는 것은 아니다.The following examples illustrate the invention in detail and are not intended to limit the invention.

[실시예 1]Example 1

본 실시예는 효모로부터 효모종균을 생산하는 과정, 상기 효모종균을 배지에서 배양하여 효모균체를 생산하는 과정, 상기 효모균체로부터 글리신베타인을 추출하는 과정을 포함한다.This embodiment includes a process of producing yeast seed from yeast, a process of producing yeast cells by culturing the yeast seed in a medium, and extracting glycinebetaine from the yeast cells.

상기 효모종균 생산과정은 효모추출물, 펩톤 및 포도당으로 조성한 공시의 표준 YPD액체배지에 10mM의 황산동을 첨가하여 스트레스 가격용 멸균배지를 준비하고, 상기 스트레스 가격용 멸균배지에 KCTC 7928를 접종하고 30℃의 진탕 배양기에서 중간 대수 성장기(mid-log phase)까지 배양한 다음, 상기 배양액 중 일부를 황산동이 배제된 표준 YPD액체배지에서 접종하여 중간대수 성장기(mid-log phase)까지 배양하여는 과정으로 이루어진다.The yeast seed production process is prepared by the addition of 10mM copper sulfate to the standard YPD liquid medium of the yeast extract, peptone and glucose prepared sterilization medium for the stress price, inoculated KCTC 7928 in the stress price sterilization medium and 30 ℃ Incubated in a shaker incubator up to the mid-log phase, and then incubated part of the culture in a standard YPD liquid medium without copper sulfate to incubate to the mid-log phase. .

상기 효모균체 생산과정은 상기 배양액 중 일부를 표준 YPD액체배지 100ml에 접종하여 성장말기 (stationary phase)까지 배양한 후 원심분리하여 효모균체를 회수하는 과정으로 이루어진다.The yeast cell production process consists of inoculating a portion of the culture solution in 100ml standard YPD liquid medium to incubate until the end of growth (stationary phase) and centrifugation to recover the yeast cells.

상기 글리신베타인 추출과정은 상기 회수한 효모균체에 4배용적의 끓는 에탄올을 가한 다음 80℃에서 20분간 추가로 가온하여 효모균체를 완전히 해체한 후, 해체된 효모균체액을 12,000 ×g 하에서 고속 원심분리하여 효모균체 잔여물을 제거하고 상등액만 취하여 80℃에서 건조하여 글리신베타인을 추출하는 과정으로 이루어진다.The glycine betaine extraction process was added to the recovered yeast cells 4 times the volume of boiling ethanol and then further heated at 80 ℃ for 20 minutes to completely disassemble the yeast cells, centrifuged at 12,000 × g Separation removes the yeast cell residues, take only the supernatant and dry at 80 ℃ to extract glycinebetaine.

상기와 동일한 방법으로 효모균을 10mM 황산동이 첨가된 표준 YPD액체배지에서 1회 배양한 후, 황산동을 배제한 표준 YPD액체배지에서 각각 2 내지 5회 연속배양한 후, 100㎖의 황산동을 배제한 표준 YPD액체배지에 접종하여 성장말기까지 배양하였다. 그리고, 상기와 동일한 원심분리 방법으로 효모균체를 회수 및 추출한다.In the same manner as above, the yeast was cultured once in a standard YPD liquid medium to which 10 mM copper sulfate was added, followed by two to five successive incubations in a standard YPD liquid medium without copper sulfate, followed by a standard YPD liquid excluding 100 ml of copper sulfate. Inoculated to the medium and cultured until the end of growth. Then, the yeast cells are recovered and extracted by the same centrifugation method as described above.

황산동 배제 배지에서 연속배양횟수Number of Continuous Cultures in Copper Sulfate Exclusion Medium 배양액 100ml당 글리신베타인 생산량(mg)Glycinebetaine production (mg) per 100 ml of culture 00 36.236.2 1One 40.140.1 22 59.859.8 33 83.283.2 44 81.381.3 55 78.478.4

상기 [표 1]은 상기 실시예에 따라 실시한 것으로, 황산동 배제 배지에서 연속배양횟수에 따른 글리신베타인 생산량을 나타낸 것이다.Table 1 shows the glycine betaine production according to the number of continuous cultures in the copper sulfate exclusion medium.

상기 [표 1]에서는, 황산동을 배제한 표준 YPD액체배지에서의 3회 연속배양한 경우에서 2회 연속배양한 경우보다 글리신베타인 생산량이 크게 증가하는 것을 볼 수 있다.In Table 1, it can be seen that the production of glycinebetaine is significantly increased in the case of three consecutive cultures in a standard YPD liquid medium excluding copper sulfate compared to the two consecutive cultures.

또한, 4회, 5회 연속배양한 경우에서도 3회 연속배양와 비슷한 양의 글리신베타인 생산을 보이고 있다.In addition, the production of glycinebetaine is similar to that of three consecutive cultures in the case of 4, 5 consecutive cultures.

[실시예 2]Example 2

본 실시예는 상기 [실시예 1]에서 사용한 방법과 동일하게 10mM 황산동을 첨가한 스트레스 가격용 멸균배지에서 배양한 효모균(KCTC 7928)을 황산동을 배제한 표준 YPD액체배지에서 3회 연속배양하는 과정, 상기 연속배양된 배양액을 효모종균으로 하여 10mM(154.6㎎/100㎖) 글리신베타인을 첨가한 표준 YPD액체배지 100㎖에 접종한 다음, 상기 접종액을 30℃ 진탕배양기에서 24, 48, 72 및 96시간 동안 배양한 다음 효모균체 및 상등액을 원심분리하여 각각 분리 회수 추출하는 과정으로 이루어진다.This Example is the same process as used in the above [Example 1] the same process as in the yeast (KCTC 7928) cultured in a sterile medium for stress price added 10mM copper sulfate in a standard YPD liquid medium excluding copper sulfate three times, The cultured culture medium was inoculated into 100 ml of standard YPD liquid medium to which 10 mM (154.6 mg / 100 ml) glycinebetaine was added as a yeast seed, and then the inoculum was inoculated at 24 ° C shaker in 24, 48, 72 and 96 After culturing for a period of time, the yeast cells and the supernatant are centrifuged and separated and recovered.

배양시간(hr)Incubation time (hr) 글리신베타인 무첨가배지(mg)Glycinebetaine-free medium (mg) 글리신베타인 154.6 mg첨가 배지(mg)Glycinebetaine 154.6 mg addition medium (mg) 균체내 함유Intracellular Content 상등액 함유Contains supernatant 2424 47.847.8 55.155.1 143.8143.8 4848 69.7569.75 91.4491.44 148.4148.4 7272 78.078.0 90.990.9 147.2147.2 9696 83.783.7 78.378.3 146.7146.7

상기 [표 2]는 상기 실시예에 따라 실시한 결과이다. 대조구로는 동일한 효모종균을 글리신베타인을 첨가하지 않은 표준 YPD액체배지 100㎖에 접종하여 같은 시간동안 배양하고 효모균체를 원심분리로 회수 추출하여 글리신베타인을 생산하였다.Table 2 shows the results according to the above examples. As a control, the same yeast seedlings were inoculated into 100 ml of standard YPD liquid medium without glycinebetaine and incubated for the same time, and the yeast cells were recovered by centrifugation to produce glycinebetaine.

상기 [표 2]에서, 글리신베타인 154.6㎎이 첨가된 배지에서 효모발효를 통해 글리신베타인을 생산한 경우가 글리신베타인을 첨가하지 않은 배지에서 효모발효를 통해 글리신베타인을 생산한 경우보다 글리신베타인 생산량이 증가하는 것을 볼 수 있다.In [Table 2], the production of glycinebetaine through yeast fermentation in a medium to which glycinebetaine was added 154.6 mg was higher than the production of glycinebetaine through fermentation of glycinebetaine in a medium without glycinebetaine. You can see the output increase.

[실시예 3]Example 3

본 실시예는 [실시예 1]과 동일한 방법에 따라 효모종균을 준비하고, 상기 효모종균을 적당한 염 및 영양원을 첨가한 사탕무 추출액 100㎖에 접종한 다음, [실시예 2]의 방법에 따라 지정한 시간동안 30℃에서 진탕배양한 후 [실시예 1]과 동일한 방법으로 효모균체 및 상등액을 원심분리하여 각각 회수하고, 글리신베타인을 추출하는 과정으로 이루어진다.In this example, yeast spawn was prepared according to the same method as in [Example 1], and the yeast spawn was inoculated into 100 ml of beet extract with the addition of a suitable salt and nutrient source, and then designated according to the method of [Example 2]. After shaking the culture at 30 ℃ for a period of time, the yeast cells and the supernatant were recovered by centrifugation in the same manner as in [Example 1], and the process consists of extracting glycinebetaine.

배양시간(hr)Incubation time (hr) 글리신베타인 함량(mg)Glycinebetaine content (mg) B/AB / A 배양 상등액(A)Culture supernatant (A) 전체 배양액내[상등액+균체](B)In supernatant [supernatant + bacteria] (B) 00 145.2145.2 141.3141.3 0.970.97 2424 140.5140.5 193.8193.8 1.381.38 4848 136.8136.8 248.4248.4 1.821.82 7272 154.5154.5 229.1229.1 1.481.48 9696 159.4159.4 228.7228.7 1.431.43

상기 [표 3]은 상기 실시예에 따라 실시한 것으로, 사탕무 추출액 배지에서 효모발효에 의한 글리신베타인의 생산량을 나타낸 것이다.Table 3 shows the amount of glycine betaine produced by yeast fermentation in the sugar beet extract medium.

상기 [표 3]에서, 배양시간이 48시간일 때 높은 글리신베타인 생산을 보이고 있는 것을 볼 수 있다.In Table 3, it can be seen that the high glycine betaine production when the incubation time is 48 hours.

상기 본 발명의 효모발효를 이용하여 글리신베타인을 생산하는 방법은 종래 시아노박테리아(cyanobacteria) 등과 같은 종래 광합성 미생물과는 달리 고강도의 빛을 조사할 필요도 없으며, 고가인 코린(choline)을 초기기질로 배지에 첨가하지 않으므로 글리신베타인을 낮은 비용으로 생산할 수 있다. 또한, 본 발명은 사탕무 추출액을 배지로 하여 발효방법으로 생산하는 경우에는 사탕무에 함유되어 있는 글리신베타인과 더불어 사탕무 정제과정 중 불순물로 분리 및 제거 해야할 사탕무에 함유된 당을 효모발효에 의해 글리신베타인으로 전환하여 추가 수득을 할 수 있으므로 글리신베타인의 수득율을 높일 수 있다.The method for producing glycine betaine using the yeast fermentation of the present invention does not need to irradiate high-intensity light, unlike conventional photosynthetic microorganisms such as cyanobacteria. Since it is not added to the furnace medium, glycinebetaine can be produced at low cost. In the present invention, when the beet extract is produced as a medium by fermentation method, glycine betaine contained in sugar beet and sugar contained in sugar beet to be separated and removed as an impurity during the sugar beet purification process are converted into glycine betaine by yeast fermentation. By conversion can be obtained further, the yield of glycinebetaine can be increased.

Claims (3)

금속에 내성을 가지는 효모를 황산동이 첨가된 영양배지에서 1회 배양하는 과정; 황산동이 배제된 영양배지에서 3 내지 5회 연속배양하여 효모종균을 생산하는 과정; 상기 효모종균을 무기염류를 함유한 사탕무 당밀액 또는 무기염류를 함유한 사탕무 추출액에 접종하여 배양하는 과정; 상기 배양액을 동결건조하는 과정; 상기 동결건조물로부터 글리신베타인을 추출하는 과정으로 이루어지는 것을 특징으로 하는 효모를 이용한 글리신베타인 생산 방법.A step of culturing the yeast resistant to the metal in a nutrient medium containing copper sulfate once; Producing yeast spawn by continuously culturing 3 to 5 times in a nutrient medium excluding copper sulfate; Inoculating the yeast spawn in beets molasses containing inorganic salts or beets extract containing inorganic salts and incubating the same; Lyophilizing the culture solution; Glycine betaine production method using the yeast, characterized in that the process consisting of extracting glycine betaine from the lyophilisate. 제1항에 있어서, 상기 효모는 KCTC 1552, 1813, 7928 중 어느 하나인 것을 특징으로 하는 효모를 이용한 글리신베타인 생산 방법.The method of claim 1, wherein the yeast is any one of KCTC 1552, 1813, and 7928. 제1항 또는 제2항에 있어서, 상기 황산동은 10mM 황산동인 것을 특징으로 하는 효모를 이용한 글리신베타인 생산 방법.The method for producing glycinebetaine using yeast according to claim 1 or 2, wherein the copper sulfate is 10 mM copper sulfate.
KR10-2002-0024868A 2002-05-06 2002-05-06 Method for production of glycinebetaine by yeast KR100469332B1 (en)

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JPH03209354A (en) * 1988-06-09 1991-09-12 Cultor Ltd Recovery of betaine from molasses
US5177008A (en) * 1987-12-22 1993-01-05 Kampen Willem H Process for manufacturing ethanol and for recovering glycerol, succinic acid, lactic acid, betaine, potassium sulfate, and free flowing distiller's dry grain and solubles or a solid fertilizer therefrom
US5177009A (en) * 1987-12-22 1993-01-05 Kampen Willem H Process for manufacturing ethanol and for recovering glycerol, succinic acid, lactic acid, betaine, potassium sulfate, and free flowing distiller's dry grain and solubles or a solid fertilizer therefrom
KR20000060323A (en) * 1999-03-13 2000-10-16 손달수 a deodorizer composition

Patent Citations (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US5177008A (en) * 1987-12-22 1993-01-05 Kampen Willem H Process for manufacturing ethanol and for recovering glycerol, succinic acid, lactic acid, betaine, potassium sulfate, and free flowing distiller's dry grain and solubles or a solid fertilizer therefrom
US5177009A (en) * 1987-12-22 1993-01-05 Kampen Willem H Process for manufacturing ethanol and for recovering glycerol, succinic acid, lactic acid, betaine, potassium sulfate, and free flowing distiller's dry grain and solubles or a solid fertilizer therefrom
JPH03209354A (en) * 1988-06-09 1991-09-12 Cultor Ltd Recovery of betaine from molasses
KR20000060323A (en) * 1999-03-13 2000-10-16 손달수 a deodorizer composition

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