CN105505791B - One plant of monascus purpureus bacterial strain and its preparing the application in food - Google Patents
One plant of monascus purpureus bacterial strain and its preparing the application in food Download PDFInfo
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N1/00—Microorganisms, 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
- C12N1/14—Fungi; Culture media therefor
- C12N1/145—Fungal isolates
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12R—INDEXING SCHEME ASSOCIATED WITH SUBCLASSES C12C - C12Q, RELATING TO MICROORGANISMS
- C12R2001/00—Microorganisms ; Processes using microorganisms
- C12R2001/645—Fungi ; Processes using fungi
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Abstract
The invention discloses a kind of monascus purpureus (Monascus purpureus) and its purposes in food production.The monascus purpureus is deposited in China Committee for Culture Collection of Microorganisms's common micro-organisms center, deposit number are as follows: CGMCC No.11319.It does not produce citrinin, and it can produce natural monascorubin, possesses higher color value, can be used for preparing in dairy products or other food processing technologies.
Description
Technical field
The present invention relates to microorganism fields, and in particular to one plant of monascus purpureus bacterial strain and its is preparing the application in food.
Background technique
Monascus (Monascus sp.) is a kind of highly important medicinal fungi, is that China is applied to food processing earliest
In one of fungi.And use scope is extensive, is mainly used for culinary art, production fermented bean curd, wine brewing and treatment disease etc..Using purplish red
Red yeast rice Gu made from aspergillus fermentation rice claims red song, with a long history, originating from China, be mainly intensively applied in traditional distiller's yeast,
The fields such as vinegar, coloring and health care product processed are the tradition materials of dietotherapeutic.Modern medicine study proves that red yeast rice has reduction gallbladder
The effects of sterol, hypoglycemic and blood pressure lowering.In addition, monascus purpureus can generate a variety of generations with physiological activity during the fermentation
Thank to product, such as: monascorubin, citrinin (Monacolin K) substance, γ-aminobutyric acid and a variety of enzymes etc..
Although monascus purpureus is longer in the edible history of China and pouplarity is higher, due to some monascus purpureus bacteriums
Kind can generate mycotoxin during the fermentation --- citrinin (citrinin), and citrinin is to human body poison with higher
Property, therefore the application range of monascus purpureus bacterial strain is limited to a certain extent.Before food safety is food production and sells
It mentioning, European and American countries have stringent limitation to the content of the citrinin in imported food especially monascus product, meanwhile, in middle Chinese
Also define that the content of citrinin in red yeast rice (powder) must not exceed 50 μ g/ in people republic light industry standard QB/T2847-2007
Kg.Research shows that the content of citrinin and the strain variety of monascus purpureus bacterium are closely related, therefore, monascus purpureus fermentation is produced
The product of class needs strictly to select bacterial strain and optimized production process, guarantees food safety.
Meanwhile monascus purpureus submerged fermentation generates monascorubin, since tone is relatively low in fermentation liquid, in addition in extraction process
The loss of aubergine ingredient, so that monascorubin low output, tone are partially yellow, coloring effect is poor.It would therefore be highly desirable to find to generate color value
High monascorubin and the monascus purpureus bacterial strain for being nearly free from citrinin.
Summary of the invention
The technical problem to be solved by the present invention is to combine for current shortage and do not generate citrinin and generate
The deficiency of the monascus purpureus (Monascus purpureus) of the very high monascorubin of color value provides a kind of citrinin, red of not producing
The high monascus purpureus bacterial strain of bent pigment color value and its preparing the application in food.The bacterial strain is provided simultaneously with that not generate tangerine mould
Element and the generation very high good characteristic of monascorubin color value, can safely apply to food-processing industry.
Technical solution of the present invention first is that: a kind of monascus purpureus (Monascus purpureus) is deposited in China
Microbiological Culture Collection administration committee common micro-organisms center, deposit number are as follows: CGMCC No.11319.From China Guangzhou Meizhou
Red kojic rice powder in separation obtain the monascus purpureus CGMCC No.11319.The CGMCC No.11319 can produce
The monascorubin of natural High color values, does not generate citrinin, can safely apply to food-processing industry.The bacterial strain is carried out
Identification, result are monascus purpureus (Monascus purpureus), are named as BD-Y-5.The bacterial strain is on September 23rd, 2015
It is preserved in China Committee for Culture Collection of Microorganisms's common micro-organisms center, and receives collection and registers on the books number
CGMCC No.11319, with Microbiological Characteristics below:
1, morphologic characteristic
It is very fast in MEA cultured on solid medium, it is cultivated 10 days under 25 DEG C of dark conditions, 45~50mm of colony diameter.Gas
Raw mycelia is luxuriant, edge white, and middle part is orange;The bacterium colony back side dissolves in MEA culture medium in dark orange.
Micro- sem observation is shown, largely generates conidium, and conidiophore specialization is unobvious, straight or slightly bent, mitogenetic
Spore is spherical in shape, colourless, and wall is slightly coarse, and base portion is truncate, concatenates, and 5.5-10.4 μm of length.Cleistothecium shallowly arrives brown, it is most not at
It is ripe, have no ascospore.
2, the characteristic that culture is learned
It can be grown under the conditions of 20~42 DEG C, proper growth temperature is 25~32 DEG C, and optimum temperature is 30 DEG C;
Suitable pH is 3.5~6.0, optimal pH 5.5.Suitable growth medium can be PDB fluid nutrient medium, the training of YES liquid
Support base or MEA fluid nutrient medium.
3, physiological property
Citrinin is not generated, can produce the monascorubin of natural relatively High color values.
Technical solution of the present invention second is that: a method of preparing the monascus purpureus CGMCC No.11319,
Include the following steps, cultivates the monascus purpureus CGMCC No.11319 in the medium.
Wherein, the culture medium is the culture medium of this field routine, can grow the monascus purpureus CGMCC
No.11319, preferably PDB fluid nutrient medium, YES fluid nutrient medium or MEA fluid nutrient medium.The PDB liquid
Culture medium is the PDB fluid nutrient medium of this field routine, preferably comprising 6~10g/L potato leaching powder and 20~40g/L
Glucose.The YES fluid nutrient medium is the YES fluid nutrient medium of this field routine, preferably comprising 4~6g/L ferment
Mother's leaching powder, 20~40g/L glucose, 5~7g/L potassium dihydrogen phosphate, 3~5g/L sodium dihydrogen phosphate and 0.5~1.5g/L hydroxide
Ammonium.The MEA fluid nutrient medium is the MEA fluid nutrient medium of this field routine, preferably comprising 20~40g/L malt
Medicinal extract and 2~4g/L soy peptone.The time of the culture be this field routine time, preferably 3~10 days, more preferably
Ground is 5~10 days.The temperature of the culture is the temperature of this field routine, and preferably 20~42 DEG C, be more preferably 25~30
℃.Preferably, the culture is shake culture.The revolving speed of the shake culture is the revolving speed of this field routine, preferably
120~220rpm is more preferably 180~220rpm.The inoculum concentration of the culture is the inoculum concentration of this field routine, preferably
5~10%, it is more preferably 5%, the percentage is percent by volume.
Preferably, further including that the monascus purpureus CGMCC No.11319 is inoculated in seed culture medium before the culture
The step of carrying out seed culture.The time of the seed culture be this field routine time, preferably 5~10 days, more preferably
Ground is 6~8 days, is most preferably 7 days.The temperature of the seed culture be this field routine temperature, preferably 15~35 DEG C,
It is more preferably 25~32 DEG C, is most preferably 30 DEG C.The culture medium of the seed culture is the culture medium of this field routine, preferably
For PDA solid medium, YES solid medium or MEA solid medium.The PDA solid medium is that this field is conventional
PDA solid medium, preferably comprising 6~10g/L potato leaching powder, 20~40g/L glucose and 20~30g/L agar.
The YES solid medium is the YES solid medium of this field routine, preferably comprising 4~6g/L yeast extract, 20
~40g/L glucose, 5~7g/L potassium dihydrogen phosphate, 3~5g/L sodium dihydrogen phosphate, 0.5~1.5g/L ammonium hydroxide and 15~
25g/L agar.The MEA solid medium is the MEA solid medium of this field routine, preferably comprising 20~
40g/L malt extract, 2~4g/L soy peptone and 12~20g/L agar.Preferably, the seed culture includes will
After the monascus purpureus bacterial strain of refrigeration slowly heats up, in the step of being coated with or crossing on seed culture medium.The temperature of the heating is
The temperature of this field routine, preferably to 15~25 DEG C.The method of the culture is the method for the culture of this field routine, compared with
It goodly is shaking flask culture or fermentation tank culture.
Technical solution provided by the invention third is that: the monascus purpureus CGMCC No.11319 is in preparing food
Using.
The food is the food of this field routine, is containing monascus purpureus CGMCC No.11319 or its metabolite
Can, preferably dairy products are more preferably cheese.
Technical solution provided by the invention fourth is that: a kind of to be fermented cheese obtained using monascus purpureus, described is purplish red
Aspergillus is monascus purpureus CGMCC No.11319.
The cheese has the distinctive flavour of monascus purpureus cheese and smell, and fermented bean curd aromatic flavour has monascus purpureus
The distinctive tender texture of cheese, shell is good, surface corrugationless, and shell takes on a red color or purple, and inside is in uniform purple or red
Color meets the eating habit of Chinese Consumer's.
Technical solution provided by the invention fifth is that: it is a kind of to be fermented red kojic rice powder obtained using monascus purpureus, it is described
Monascus purpureus is monascus purpureus CGMCC No.11319.
The red kojic rice powder is red to dark violet red, and quality is crisp, no mildew, without obvious macroscopic impurity, is in
Irregular graininess, with the intrinsic Qu Xiang of red yeast rice.
On the basis of common knowledge of the art, above-mentioned each optimum condition, can any combination to get each preferable reality of the present invention
Example.
The reagents and materials used in the present invention are commercially available.
The positive effect of the present invention is that: it is mould that the monascus purpureus CGMCC No.11319 is provided simultaneously with generation tangerine
The content of element is low and generates the very high good characteristic of monascorubin color value, this be at present existing monascus purpureus belong in bacterial strain all
The outstanding advantage not having.It can be used for preparing in the dairy products such as cheese or other food processing technologies, so that obtained
Food is practically free of the green element of tangerine, meets safe food sanitation standard, while colouring bright-coloured, pure color, more preferably deep by vast consumption
Person's likes.
Biomaterial preservation information
Monascus purpureus BD-Y-5 of the invention was deposited in Chinese microorganism strain preservation management on September 23rd, 2015
Committee's common micro-organisms center (CGMCC), preservation address: Yard 1, BeiChen xi Road, Chaoyang District, Beijing City 3, postcode:
100101, deposit number are as follows: CGMCC No.11319, culture title are BD-Y-5, and classification naming is monascus purpureus
(Monascus purpureus)。
Detailed description of the invention
Fig. 1 is the morphological feature of monascus purpureus BD-Y-5.Wherein A indicates monascus purpureus BD-Y-5 in wort agar culture
Colonial morphology on base (MEA);The microscopic features of B~C expression monascus purpureus BD-Y-5.
Fig. 2 is the case where monascus purpureus BD-Y-5 biomass changes with fermentation time.
Specific embodiment
The present invention is further illustrated below by the mode of embodiment, but does not therefore limit the present invention to the reality
It applies among a range.In the following examples, the experimental methods for specific conditions are not specified, according to conventional methods and conditions, or according to quotient
The selection of product specification.
Monascus GL-1 in effect example is red yeast rice (Monascus sp.), which protects on May 8th, 2013
It ensconces China Committee for Culture Collection of Microorganisms's common micro-organisms center (CGMCC), bacterial strain deposit number: CGMCC
No.7603 is announced in CN103444878A.
Monascus purpureus BD-M-1 in effect example is purplish red bent (Monascus purpureus), the bacterial strain in
It is deposited in China Committee for Culture Collection of Microorganisms's common micro-organisms center (CGMCC), bacterial strain preservation on August 28th, 2013
Number: CGMCC No.8120 is announced in CN104585333A.
Monascus purpureus BD-M-2 purplish red bent (Monascus purpureus) in effect example, the bacterial strain is in 2013
On October 16, in is deposited in China Committee for Culture Collection of Microorganisms's common micro-organisms center (CGMCC), and bacterial strain preservation is compiled
Number: CGMCC No.8310 is announced in CN105062894A.
Monascus purpureus BD-M-4 monascus purpureus (Monascus purpureus) in effect example, the bacterial strain in
On October 8th, 2014 is deposited in China Committee for Culture Collection of Microorganisms's common micro-organisms center (CGMCC), bacterial strain preservation
Number: CGMCC No.9712 is announced in CN104962483A.
Monascus purpureus BD-A5, monascus purpureus BD-B5, monascus purpureus BD-C5 and monascus purpureus GL- in comparative example
A5 is obtained by following step:
(1) PDA solid medium: potato leaching powder 6g/L, glucose 20g/L and agar 20g/L is configured.
(2) coating culture: the red kojic rice powder of a small amount of China's MeiZhou,GuangDong is taken uniformly to be sprinkled into the PDA solid of step (1) preparation
Media surface.30 DEG C are cultivated 2 days in constant incubator.
(3) after white fluffy mycelia grows, picking a little mycelia scribing line switching on another PDA solid medium after
Continuous culture, 30 DEG C are cultivated 1 week in constant incubator.Step (2) and step (3) 3 times are continuously repeated, the purple of uniform character is obtained
Monascus is respectively designated as monascus purpureus BD-A5, monascus purpureus BD-B5, monascus purpureus BD-C5 and monascus purpureus GL-A5.It will
Monascus purpureus BD-A5, monascus purpureus BD-B5, monascus purpureus BD-C5 and monascus purpureus GL-A5 bacterial strain are stored in the test tube slant PDA
It is placed on culture medium in 4 DEG C of refrigerators.
The acquisition of 1 monascus purpureus BD-Y-5 bacterial strain of embodiment
Purification procedures are as follows:
(1) PDA solid medium: potato leaching powder 6g/L, glucose 20g/L and agar 20g/L is configured.
(2) coating culture: the red kojic rice powder of a small amount of China's MeiZhou,GuangDong is taken uniformly to be sprinkled into the PDA solid of step (1) preparation
Media surface.30 DEG C are cultivated 2 days in constant incubator.
(3) after white fluffy mycelia grows, picking a little mycelia scribing line switching on another PDA solid medium after
Continuous culture, 30 DEG C are cultivated 1 week in constant incubator.Step (2) and step (3) 3 times are continuously repeated, the purple of uniform character is obtained
Monascus is named as BD-Y-5.
(4) monascus purpureus BD-Y-5 bacterial strain is stored on PDA solid medium and is placed in 4 DEG C of refrigerators.
Monascus purpureus BD-Y-5 is commonly micro- in China Committee for Culture Collection of Microorganisms on September 23rd, 2015
Bio-Centers (CGMCC) preservation obtains deposit number are as follows: CGMCC No.11319, culture title are BD-Y-5, classification naming
It is monascus purpureus (Monascus purpureus).
The cultural character of 2 monascus purpureus BD-Y-5 of embodiment
(1), monascus purpureus BD-Y-5 is very fast in MEA cultured on solid medium, cultivates 10 days under 25 DEG C of dark conditions, bacterium
It falls diameter and reaches 45~50mm.Aerial hyphae is luxuriant, edge white, and middle part is orange;The bacterium colony back side dissolves in culture in dark orange
In base.Micro- sem observation shows, monascus purpureus BD-M-4 generates a large amount of conidiums, and conidiophore specialization is unobvious, it is straight or
Slightly bent, conidium is spherical, and colourless, wall is slightly coarse, and base portion is truncate, concatenates, and 5.5-10.4 μm.Cleistothecium shallowly arrives brown, more
Number is immature, has no ascospore, meets the feature of monascus purpureus category (referring to Figure 1A~C).
(2), it is found by culture, BD-Y-5 bacterial strain can be grown under the conditions of 20~42 DEG C, proper growth temperature
Degree is 25~32 DEG C, and optimum temperature is 30 DEG C;Suitable pH is 3.5~6.0, optimal pH 5.5.Suitable growth medium can
To be PDB fluid nutrient medium, YES fluid nutrient medium or MEA fluid nutrient medium.Wherein, in MEA fluid nutrient medium and PDB liquid
It on body culture medium, cultivates 10 days under the conditions of 30 DEG C, is continuously cultivated through 15 generations, cultural characteristic, morphological feature etc. become without obvious
Change, the biological character of the bacterium is basicly stable.
Wherein, PDB culture medium includes 30g/L glucose and 10g/L potato leaching powder.YES culture medium includes 5g/L yeast
Soak powder, 30g/L glucose, 6g/L potassium dihydrogen phosphate, 4g/L sodium dihydrogen phosphate and 1g/L ammonium hydroxide.MEA culture medium includes
25g/L malt extract and 3g/L soy peptone.
The physiological property of 3 monascus purpureus BD-Y-5 of embodiment
The constituent of PDA solid medium are as follows: 6g/L potato leaching powder, 20g/L glucose and 20g/L agar.
The constituent of PDB fluid nutrient medium are as follows: 6g/L potato leaching powder and 20g/L glucose.
The monascus purpureus BD-Y-5 that 4 DEG C save aseptically is transferred in PDA solid medium, 30 DEG C of activation trainings
Be inoculated in PDA solid medium after supporting 4 days 30 DEG C activation culture 5 days to get first order seed.
250mL triangular flask be packed into 50mL PDB fluid nutrient medium, access diameter be 1cm first order seed bacteria cake, 30 DEG C
Shaking table, 180r/min revolving speed cultivate 4 days to get second order fermentation seed.
It is packed into 100mL PDB fluid nutrient medium in 500mL triangular flask, second order fermentation kind is accessed with the ratio of 5% (v/v)
Son, 30 DEG C of shaking tables, 180r/min revolving speed are cultivated 10 days.
According to the research method of Shao Wei et al., (Shao Wei, Wang Dong, Tang Ming wait " monascus purpureus produces property of protease research "
The brewing of [J] China, 2006,5:34-37.), measure mycelia weight (i.e. biomass), indicate its upgrowth situation.It can from Fig. 2
Out, monascus purpureus BD-Y-5 is in 3 days that culture starts, and thallus largely generates, and thallus reaches maximum value 5.4g/ within the 4th day or so
L, and thalli growth is in the stabilization sub stage, and then the biomass of thallus is slowly reduced, and meets the growth characteristics of monascus purpureus.
The physiological property of 4 monascus purpureus BD-Y-5 of embodiment
The constituent of PDA solid medium are as follows: 10g/L potato leaching powder, 30g/L glucose and 30g/L agar.
The constituent of PDB fluid nutrient medium are as follows: 10g/L potato leaching powder and 30g/L glucose.
The monascus purpureus BD-Y-5 that 4 DEG C save aseptically is transferred in PDA solid medium, 30 DEG C of activation trainings
Be inoculated in PDA solid medium after supporting 4 days 30 DEG C activation culture 5 days to get first order seed.
250mL triangular flask be packed into 50mL PDB fluid nutrient medium, access diameter be 1cm first order seed bacteria cake, 30 DEG C
Shaking table, 180r/min revolving speed cultivate 4 days to get second order fermentation seed.
It is packed into 100mL PDB fluid nutrient medium in 500mL triangular flask, second order fermentation kind is accessed with the ratio of 10% (v/v)
Son, 30 DEG C of shaking tables, 180r/min revolving speed are cultivated 10 days.
According to the measuring method of the honor of Jiangxi perhaps, (detection of Jiangxi honor red yeast rice citrinin and the Jiangnan ferment control technology [D] are big perhaps
Doctoral thesis, 2004.), it is measured using Agilent HPLC 1260.As a result, it has been found that monascus purpureus BD-Y-5 does not produce tangerine
Mycin amount is suitable for preparing cheese.
Illustrated by the data of embodiment 2~4, the monascus purpureus CGMCC No.11319 has microbiology below special
Property:
1, morphologic characteristic
It is very fast in MEA cultured on solid medium, it is cultivated 10 days under 25 DEG C of dark conditions, colony diameter reaches 45~
50mm.Aerial hyphae is luxuriant, edge white, and middle part is orange;The bacterium colony back side dissolves in MEA solid medium in dark orange.It produces
Raw a large amount of conidiums, conidiophore specialization is unobvious, straight or slightly bent, and conidium is spherical, and colourless, wall is slightly coarse, base
Portion is truncate, concatenates, and 5.5-10.4 μm.Cleistothecium shallowly arrives brown, most immature, has no ascospore.
2, the characteristic that culture is learned
It can be grown under the conditions of 20~42 DEG C, proper growth temperature is 25~32 DEG C, and optimum temperature is 30 DEG C;
Suitable pH is 3.5~6.0, optimal pH 5.5.Suitable growth medium can be PDB fluid nutrient medium, the training of YES liquid
Support base or MEA fluid nutrient medium.
3, physiological property
Citrinin is not produced, can produce natural monascorubin, and possesses higher color value.
The rDNA sequence of 5 monascus purpureus BD-Y-5 of embodiment is analyzed
Monascus purpureus BD-Y-5 is subjected to rRNA gene sequencing (being sequenced by Institute of Microorganism, Academia Sinica), sequencing knot
For fruit as shown in SEQ No.1 in sequence table, which contains the 18S rRNA segment of monascus purpureus BD-Y-5, ITS1,5.8S
The complete sequence and 28S region sequence segment of rRNA, ITS2.By the sequence and document and public database DDBJ, EMBL, GenBank
It is found Deng being compared through BLAST, homology 99%.Therefore, monascus purpureus BD-Y-5 belongs to monascus purpureus (Monascus
purpureus)。
6 monascus purpureus BD-Y-5 of embodiment prepares red kojic rice powder
Ingredient: long-grained nonglutinous rice 10kg, glucose 40g, potato leaching powder 12g and agar 20g.
The constituent of PDA solid medium are as follows: 6g/L potato leaching powder, 20g/L glucose and 20g/L agar.
The constituent of PDB fluid nutrient medium are as follows: 6g/L potato leaching powder and 20g/L glucose.
Preparation step:
(1) activation and processing of strain: the monascus purpureus BD-M-4 that 4 DEG C save aseptically is transferred and is consolidated in PDA
In body culture medium, 30 DEG C be inoculated in after activation culture 4 days in PDA solid medium 30 DEG C activation culture 5 days to get level-one kind
Son.
250mL triangular flask be packed into 50mL PDB fluid nutrient medium, access diameter be 1cm first order seed bacteria cake, 30 DEG C
Shaking table, 180r/min revolving speed cultivate 4 days to get second order fermentation seed.
It is packed into 100mL PDB fluid nutrient medium in 500mL triangular flask, second order fermentation kind is accessed with the ratio of 10% (v/v)
Son, 30 DEG C of shaking tables, 180r/min revolving speed are cultivated 10 days, its pH value are adjusted to 3.0, obtains the strain of processing.
(2) long-grained nonglutinous rice is impregnated 12 hours in clear water, makes feed moisture content 50%, obtain soaked long-grained nonglutinous rice;
(3) soaked long-grained nonglutinous rice is put into high-pressure steam sterilizing pan, 121 DEG C of steamed rice 20min obtain steamed long-grained nonglutinous rice meal, make Xian
Rice maturation is without the white heart, and uniformity is without agglomeration;
(4) steamed long-grained nonglutinous rice meal is poured out, spreading for cooling is simultaneously sieved, and is inoculated in 38 DEG C.Every 10kg long-grained nonglutinous rice is inoculated with 0.04g step
(1) strain of resulting processing, is mixed thoroughly, is put into constant temperature and humidity incubator, 30 DEG C of constant temperature, the culture of constant relative humidity 80% 6
It, during which turned over bent and moisturizing, rate of water make-up 10% every 4 hours, and the percentage is mass percent, when culture was to the 5th day
Stop moisturizing.Drying is taken out to grind to get red kojic rice powder.
Obtained red kojic rice powder is red to dark violet red, and quality is crisp, no mildew, the obvious macroscopic impurity of nothing,
In irregular graininess, with the intrinsic Qu Xiang of red yeast rice.
7 monascus purpureus BD-Y-5 of embodiment prepares cheese
Ingredient: fresh cow milk 100L (being purchased from bright milk industry), MA14 (being purchased from Danisco (China) Co., Ltd product) hair
Ferment agent 3g, calf stomach renin (being purchased from Chr. Hansen A/S) 1g, salt 0.75kg, glucose 40g and potato leaching powder 6g.
(1) after taking 100L fresh cow milk filtering and impurity removing matter, 72 DEG C of sterilizing 30s are subsequently cooled to 30 DEG C, must handle cream.To institute
State inoculating starter MA14, inoculum concentration 3g/100L in processing cream, under 30 DEG C of constant temperature culture to pH6.5 when 1g calf stomach is added
Renin, curdled milk 30min obtain curdled milk;
(2) step (1) resulting curd cutting is stirred into 10min discharging whey at bulk;After whey to be discharged into curdled milk
1.5% salt is added, the percentage is the mass percent that the salt accounts for the curdled milk, enters rectangular mould after mixing evenly
Tool;
(3) curdled milk enters mold forming and obtains ziega and periodically overturn, and frequency is to overturn 1 time every 2 hours, continues 24 hours,
Whey is discharged further;
(4) the monascus purpureus fermentation liquid that thickness is about 1mm is uniformly sprayed toward the ziega surface that step (3) obtain, be packed into
Mature container, constant incubator is mature, the temperature of the maturation are as follows: and 25 DEG C of initial stage, relative humidity 90%, 10 DEG C of the middle and later periods;Institute
State the mature time are as follows: initial stage 2 weeks, the middle and later periods 2 weeks.
The monascus purpureus fermentation liquid is made by following methods: monascus purpureus BD-Y-5 is inoculated in PDB fluid nutrient medium
In 30 DEG C cultivate 2 days, the formula of the PDB fluid nutrient medium are as follows: glucose 40g/L, potato leaching powder 6g/L, surplus are water.
Obtained monascus purpureus cheese has the distinctive flavour of monascus purpureus cheese and smell, and fermenting aroma is strong, tool
There is a distinctive tender texture of monascus purpureus cheese, shell is good, surface corrugationless, and shell takes on a red color or purple, and inside is in uniform
Purple or red, be suitble to Chinese Consumer's eating habit.
8 monascus purpureus BD-Y-5 of embodiment prepares cheese
Ingredient: fresh sheep cream 100L (being purchased from bright milk industry), MA14 (being purchased from Danisco (China) Co., Ltd product) hair
Ferment agent 3g, microbial rennet (being purchased from Chr. Hansen A/S) 1g, salt 0.5kg, glucose 40g and potato leaching powder 6g.
(1) after taking the fresh sheep cream filtering and impurity removing matter of 100L, 72 DEG C of sterilizing 15s are subsequently cooled to 28 DEG C, must handle cream.To institute
State inoculating starter MA14, inoculum concentration 3g/100L in processing cream, under 28 DEG C of constant temperature culture to pH6.5 when 1g microorganism is added
Renin, curdled milk 30min obtain curdled milk;
(2) step (1) resulting curd cutting is stirred into 10min discharging whey at bulk;After whey to be discharged into curdled milk
1% salt is added, the percentage is the mass percent that the salt accounts for the curdled milk, enters square dies after mixing evenly;
(3) curdled milk enters mold forming and obtains ziega and periodically overturn, and frequency is to overturn 1 time every 2 hours, continues 24 hours,
Whey is discharged further;
(4) the monascus purpureus fermentation liquid that thickness is about 1.5mm is uniformly sprayed toward the ziega surface that step (3) obtain, filled
Enter mature container, constant incubator is mature, the temperature of the maturation are as follows: 20 DEG C of initial stage, relative humidity 95%, 8 DEG C of the middle and later periods;Institute
State the mature time are as follows: initial stage 2 weeks, the middle and later periods 2 weeks.
The monascus purpureus fermentation liquid is made by following methods: monascus purpureus BD-Y-5 is inoculated in PDB fluid nutrient medium
In 30 DEG C cultivate 2 days, the formula of the PDB fluid nutrient medium are as follows: the formula of the monascus purpureus culture medium are as follows: glucose 40g/
L, potato leaching powder 6g/L.
9 monascus purpureus BD-Y-5 of embodiment prepares cheese
Ingredient: fresh horse cream 100L (being purchased from bright milk industry), MA14 (being purchased from Danisco (China) Co., Ltd product) hair
Ferment agent 3g, calf stomach renin (being purchased from Chr. Hansen A/S) 1g, salt 1.5kg, glucose 40g and potato leaching powder 6g.
(1) after taking the fresh horse cream filtering and impurity removing matter of 100L, 72 DEG C of sterilizing 30s are subsequently cooled to 32 DEG C, must handle cream.To institute
State inoculating starter MA14, inoculum concentration 3g/100L in processing cream, under 32 DEG C of constant temperature culture to pH6.5 when 1g calf stomach is added
Renin, curdled milk 30min obtain curdled milk;
(2) step (1) resulting curd cutting is stirred into 10min discharging whey at bulk;After whey to be discharged into curdled milk
1.25% salt is added, the percentage is the mass percent that the salt accounts for the curdled milk, enters rectangular mould after mixing evenly
Tool;
(3) curdled milk enters mold forming and obtains ziega and periodically overturn, and frequency is to overturn 1 time every 2 hours, continues 24 hours,
Whey is discharged further;
(4) the monascus purpureus fermentation liquid that thickness is about 1mm is uniformly sprayed toward the ziega surface that step (3) obtain, be packed into
Mature container, constant incubator is mature, the temperature of the maturation are as follows: and 22 DEG C of initial stage, relative humidity 85%, 12 DEG C of the middle and later periods;Institute
State the mature time are as follows: initial stage 2 weeks, the middle and later periods 2 weeks.
The monascus purpureus fermentation liquid is made by following methods: monascus purpureus BD-Y-5 is inoculated in PDB fluid nutrient medium
In 30 DEG C cultivate 2 days, the formula of the PDB fluid nutrient medium are as follows: glucose 40g/L, potato leaching powder 6g/L.
10 monascus purpureus BD-Y-5 of embodiment prepares cheese
Ingredient: fresh camel cream 100L (being purchased from bright milk industry), MA14 (being purchased from Danisco (China) Co., Ltd product) hair
Ferment agent 3g, calf stomach renin (being purchased from Chr. Hansen A/S) 1g, salt 0.5kg, glucose 40g and potato leaching powder 6g.
(1) after taking the newborn filtering and impurity removing matter of the fresh camel of 100L, 72 DEG C of sterilizing 30s are subsequently cooled to 30 DEG C, must handle cream.To institute
State inoculating starter MA14, inoculum concentration 3g/100L in processing cream, under 30 DEG C of constant temperature culture to pH6.5 when 1g calf stomach is added
Renin, curdled milk 30min obtain curdled milk;
(2) step (1) resulting curd cutting is stirred into 10min discharging whey at bulk;After whey to be discharged into curdled milk
1% salt is added, the percentage is the mass percent that the salt accounts for the curdled milk, enters square dies after mixing evenly;
(3) curdled milk enters mold forming and obtains ziega and periodically overturn, and frequency is to overturn 1 time every 2 hours, continues 24 hours,
Whey is discharged further;
(4) the monascus purpureus fermentation liquid that thickness is about 1mm is uniformly sprayed toward the ziega surface that step (3) obtain, be packed into
Mature container, constant incubator is mature, the temperature of the maturation are as follows: and 25 DEG C of initial stage, relative humidity 90%, 10 DEG C of the middle and later periods;Institute
State the mature time are as follows: initial stage 2 weeks, the middle and later periods 2 weeks.
The monascus purpureus fermentation liquid is made by following methods: monascus purpureus BD-Y-5 is inoculated in PDB fluid nutrient medium
In 30 DEG C cultivate 2 days, the formula of the PDB fluid nutrient medium are as follows: glucose 40g/L, potato leaching powder 6g/L.
11 monascus purpureus BD-Y-5 of embodiment fermentation
Seed culture: the monascus purpureus BD-Y-5 that 4 DEG C save is to slowly warm up to 15 DEG C, after aseptically will heat up
Bacterial strain is crossed on PDA solid medium, 30 DEG C activation culture 4 days, obtain seed liquor.
PDA solid medium are as follows: 6g/L potato leaching powder, 20g/L glucose and 20g/L agar.
Fermented and cultured: being inoculated in PDB fluid nutrient medium for seed liquor with 5%, 42 DEG C shake culture 3 days, revolving speed is
220rpm, the percentage are percent by volume.
PDB fluid nutrient medium are as follows: 6g/L potato leaching powder and 20g/L glucose.
12 monascus purpureus BD-Y-5 of embodiment fermentation
Seed culture: the monascus purpureus BD-Y-5 that 4 DEG C save is to slowly warm up to 25 DEG C, after aseptically will heat up
Bacterial strain is crossed on YES solid medium, 30 DEG C activation culture 7 days, obtain seed liquor.
YES solid medium are as follows: 5g/L yeast extract, 30g/L glucose, 6g/L potassium dihydrogen phosphate, 4g/L biphosphate
Sodium, 1g/L ammonium hydroxide and 20g/L agar.
Fermented and cultured: being inoculated in YES fluid nutrient medium for seed liquor with 5%, 20 DEG C shake culture 10 days, revolving speed is
120rpm, the percentage are percent by volume.
YES fluid nutrient medium are as follows: 5g/L yeast extract, 30g/L glucose, 6g/L potassium dihydrogen phosphate, 4g/L biphosphate
Sodium and 1g/L ammonium hydroxide.
13 monascus purpureus BD-Y-5 of embodiment fermentation
Seed culture: the monascus purpureus BD-Y-5 that 4 DEG C save is to slowly warm up to 15 DEG C, aseptically will heat up
Bacterial strain is crossed on YES solid medium afterwards, 32 DEG C activation culture 6 days, obtain seed liquor.
YES solid medium are as follows: 4g/L yeast extract, 20g/L glucose, 5g/L potassium dihydrogen phosphate, 3g/L biphosphate
Sodium, 0.5g/L ammonium hydroxide and 15g/L agar.
Fermented and cultured: being inoculated in YES fluid nutrient medium for seed liquor with 10%, 25 DEG C shake culture 5 days, revolving speed is
220rpm, the percentage are percent by volume.
YES fluid nutrient medium are as follows: 4g/L yeast extract, 20g/L glucose, 5g/L potassium dihydrogen phosphate, 3g/L biphosphate
Sodium and 0.5g/L ammonium hydroxide.
14 monascus purpureus BD-Y-5 of embodiment fermentation
Seed culture: the monascus purpureus BD-Y-5 that 4 DEG C save is to slowly warm up to 15 DEG C, after aseptically will heat up
Bacterial strain is crossed on YES solid medium, 25 DEG C activation culture 8 days, obtain seed liquor.
YES solid medium are as follows: 6g/L yeast extract, 40g/L glucose, 7g/L potassium dihydrogen phosphate, 5g/L biphosphate
Sodium, 1.5g/L ammonium hydroxide and 25g/L agar.
Fermented and cultured: being inoculated in YES fluid nutrient medium for seed liquor with 10%, 30 DEG C shake culture 5 days, revolving speed is
180rpm, the percentage are percent by volume.
YES fluid nutrient medium are as follows: 6g/L yeast extract, 40g/L glucose, 7g/L potassium dihydrogen phosphate, 5g/L biphosphate
Sodium and 1.5g/L ammonium hydroxide.
15 monascus purpureus BD-Y-5 of embodiment fermentation
Seed culture: the monascus purpureus BD-Y-5 that 4 DEG C save is to slowly warm up to 20 DEG C, after aseptically will heat up
Bacterial strain is crossed on MEA solid medium, 35 DEG C activation culture 5 days, obtain seed liquor.
MEA solid medium are as follows: 25g/L malt extract, 3g/L soy peptone and 15g/L agar.
Fermented and cultured: being inoculated in MEA fluid nutrient medium for seed liquor with 5%, 30 DEG C shake culture 10 days, revolving speed is
180rpm, the percentage are percent by volume.
MEA fluid nutrient medium are as follows: 25g/L malt extract and 3g/L soy peptone.
16 monascus purpureus BD-Y-5 of embodiment fermentation
Seed culture: the monascus purpureus BD-Y-5 that 4 DEG C save is to slowly warm up to 20 DEG C, after aseptically will heat up
Bacterial strain is crossed on MEA solid medium, 15 DEG C activation culture 10 days, obtain seed liquor.
MEA solid medium are as follows: 20g/L malt extract, 2g/L soy peptone and 12g/L agar.
Fermented and cultured: being inoculated in MEA fluid nutrient medium for seed liquor with 8%, 42 DEG C shake culture 3 days, revolving speed is
120rpm, the percentage are percent by volume.
MEA fluid nutrient medium are as follows: 20g/L malt extract and 2g/L soy peptone.
17 monascus purpureus BD-Y-5 of embodiment fermentation
Seed culture: the monascus purpureus BD-Y-5 that 4 DEG C save is to slowly warm up to 20 DEG C, after aseptically will heat up
Bacterial strain is crossed on MEA solid medium, 15 DEG C activation culture 10 days, obtain seed liquor.
MEA solid medium are as follows: 40g/L malt extract, 4g/L soy peptone and 20g/L agar.
Fermented and cultured: being inoculated in MEA fluid nutrient medium for seed liquor with 10%, 42 DEG C shake culture 3 days, revolving speed is
150rpm, the percentage are percent by volume.MEA fluid nutrient medium are as follows: 40g/L malt extract and 4g/L soy peptone.
Effect example 1
By monascus purpureus BD-Y-5, monascus purpureus BD-A5, monascus purpureus BD-B5, monascus purpureus BD-C5, purple aspergillus GL-
The step of A5, monascus GL-1, monascus purpureus BD-M-1, monascus purpureus BD-M-2 and monascus purpureus BD-M-4 are according to embodiment 3
The step of being activated, being cultivated measures mycelia weight, and the results are shown in Table 1.
The result of table 1 illustrates that the biomass of other bacterial strains is compared compared with, the maximum biomass of monascus purpureus BD-Y-5 compared with
Greatly, there is significant difference with other bacterial strains, there is apparent growth vigor under 30 DEG C of environment.
The different monascus purpureus bacterial strain of table 1 is when fermenting 10 days the case where biomass
Effect example 2
By monascus purpureus BD-Y-5, monascus purpureus BD-A5, monascus purpureus BD-B5, monascus purpureus BD-C5, monascus purpureus
GL-A5, monascus GL-1, monascus purpureus BD-M-1, monascus purpureus BD-M-2 and monascus purpureus BD-M-4 according to embodiment 4 step
Suddenly the step of being activated, being cultivated measures citrinin content, and the results are shown in Table 2.
The different monascus purpureus bacterial strain of table 2 is when fermenting 10 days the case where citrinin content
Table 2 illustrates, is free of citrinin in the bacterium solution that monascus purpureus BD-Y-5 fermentation generates, purple in addition to purplish red song M-1 bacterial strain
The fermentation liquid of monascus BD-Y-5 bacterial strain is substantially less than other comparison bacterial strains, illustrates that BD-Y-5 bacterial strain is capable of being applied to for safety
In the processing technology for preparing the food such as dairy products, red kojic rice powder.
Effect example 3
By monascus purpureus BD-Y-5, monascus purpureus BD-A5, monascus purpureus BD-B5, monascus purpureus BD-C5, monascus purpureus
GL-A5, monascus GL-1, monascus purpureus BD-M-1, monascus purpureus BD-M-2 and monascus purpureus BD-M-4 are with the ratio of 5% (v/v)
Example is inoculated in YES culture medium (including 5g/L yeast extract, 30g/L glucose, 6g/L potassium dihydrogen phosphate, 4g/L sodium dihydrogen phosphate
With 1g/L ammonium hydroxide) in, fermentation liquid is cultivated 5 days to obtain at 28 DEG C, (Jiangxi honor red yeast rice tangerine is mould perhaps according to the measuring method of the honor of Jiangxi perhaps
The detection of element and ferment control technology [D] Southern Yangtze University doctoral thesis, 2004.), take 10mL fermentation liquid with isometric 70%
(v/v) ethyl alcohol extracts 30min, filtering, and filtrate carries out after suitably diluting, scans in 190-700nm wave-length coverage.
The calculation formula of color value: color value (CV)=OD505× extension rate (U/ml).The results are shown in Table 3:
Color value situation of the different monascus purpureus bacterial strain of table 3 when fermenting 5 days
Strain name | Color value (CV) |
Monascus purpureus BD-Y-5 | 7 |
Monascus purpureus BD-A5 | 4 |
Monascus purpureus BD-B5 | 4 |
Monascus purpureus BD-C5 | 5 |
Monascus purpureus GL-A5 | 4.5 |
Monascus GL-1 | 4 |
Monascus purpureus BD-M-1 | 5 |
Monascus purpureus BD-M-2 | 6 |
Monascus purpureus BD-M-4 | 6 |
Table 3 illustrates that the color value that monascus purpureus BD-Y-5 bacterial strain produces monascorubin is high, illustrates the ability for producing monascus purpureus pigment
By force.
It should be understood that those skilled in the art can make the present invention various after having read above content of the invention
Change or modification, these equivalent forms also fall within the scope of the appended claims of the present application.
Claims (20)
1. a kind of monascus purpureus (Monascus purpureus), which is characterized in that it is deposited in Chinese microorganism strain preservation
Administration committee's common micro-organisms center, deposit number are as follows: CGMCC No.11319.
2. a kind of method for preparing monascus purpureus CGMCC No.11319, which is characterized in that it includes the following steps, is cultivating
Purplish red song monascus purpureus CGMCC No.11319 is cultivated in base.
3. method according to claim 2, which is characterized in that the culture medium is PDB fluid nutrient medium, the training of YES liquid
Support base or MEA fluid nutrient medium;The PDB fluid nutrient medium includes 6~10g/L potato leaching powder and 20~40g/L grape
Sugar;The YES fluid nutrient medium includes 4~6g/L yeast extract, 20~40g/L glucose, 5~7g/L potassium dihydrogen phosphate, 3
~5g/L sodium dihydrogen phosphate and 0.5~1.5g/L ammonium hydroxide;The MEA fluid nutrient medium is soaked including 20~40g/L malt
Cream and 2~4g/L soy peptone;The time of the culture is 3~10 days;The temperature of the culture is 20~42 DEG C;Described
Culture is shake culture, and the revolving speed of the shake culture is 120~220rpm;And/or the inoculum concentration of the culture be 5~
10%, the percentage is percent by volume.
4. method as claimed in claim 3, which is characterized in that the time of the culture is 5~10 days.
5. method as claimed in claim 3, which is characterized in that the temperature of the culture is 25~30 DEG C.
6. method as claimed in claim 3, which is characterized in that the revolving speed of the shake culture is 180~220rpm.
7. method as claimed in claim 3, which is characterized in that the time of the culture is 5~10 days;The temperature of the culture
It is 25~30 DEG C;The revolving speed of the shake culture is 180~220rpm.
8. method according to claim 2, which is characterized in that further include by monascus purpureus CGMCC before the culture
No.11319 is inoculated in the step of seed culture medium carries out seed culture.
9. method according to claim 8, which is characterized in that the time of the seed culture is 5~10 days;The seed training
Feeding temperature is 15~35 DEG C;And/or the culture medium of the seed culture be PDA solid medium, YES solid medium or
MEA solid medium.
10. method as claimed in claim 9, which is characterized in that the time of the seed culture is 6~8 days.
11. method as claimed in claim 10, which is characterized in that the time of the seed culture is 7 days.
12. method as claimed in claim 9, which is characterized in that the temperature of the seed culture is 25~32 DEG C.
13. method as claimed in claim 12, which is characterized in that the temperature of the seed culture is 30 DEG C.
14. method as claimed in claim 9, which is characterized in that the time of the seed culture is 6~8 days;The seed training
Feeding temperature is 25~32 DEG C.
15. method as claimed in claim 9, which is characterized in that the time of the seed culture is 7 days;The seed culture
Temperature be 30 DEG C.
16. method according to claim 8, which is characterized in that the seed culture includes the monascus purpureus bacterium that will be refrigerated
The step of strain slowly heats up.
17. the method described in claim 16, which is characterized in that the temperature of the heating is 15~25 DEG C.
18. purposes of the monascus purpureus CGMCC No.11319 as described in claim 1 in food production.
19. a kind of utilize monascus purpureus fermentation cheese obtained, which is characterized in that the monascus purpureus is monascus purpureus
CGMCC No.11319。
20. a kind of utilize monascus purpureus fermentation red kojic rice powder obtained, which is characterized in that the monascus purpureus is monascus purpureus
CGMCC No.11319。
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CN105112305A (en) * | 2015-09-18 | 2015-12-02 | 福建农林大学 | Red yeast rice rich in Monacolin K and preparation method of red yeast rice |
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CN105112305A (en) * | 2015-09-18 | 2015-12-02 | 福建农林大学 | Red yeast rice rich in Monacolin K and preparation method of red yeast rice |
Non-Patent Citations (3)
Title |
---|
"Production and optimization of monacolin K by citrinin free Monascus pilosus MS 1 in solid state fermentation using non glutinous rice and soybean flours as substrate";Yanli Feng等;《Eur Food Res Technol》;20140603;第239卷(第4期);摘要,第631页右栏最后一行以及第632页左栏12行 * |
"八种稻米基质对红曲重要代谢产物的影响";高红等;《中国食品添加剂》;20150430;第4卷;第137-142页 * |
Yanli Feng等."Production and optimization of monacolin K by citrinin free Monascus pilosus MS 1 in solid state fermentation using non glutinous rice and soybean flours as substrate".《Eur Food Res Technol》.2014,第239卷(第4期),摘要,第631页右栏最后一行以及第632页左栏12行. * |
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