KR101018145B1 - Method for making of nutrient broth for cultivating Oyster mushrooms and nutrient broth for cultivating Oyster mushrooms made thereby - Google Patents

Abstract

The present invention relates to a method for producing a medium for growing oyster mushroom and a medium for cultivating oyster mushroom prepared by using the same. More specifically, the pH of the medium is mixed with a predetermined amount of calcium hydroxide instead of high temperature heat treatment for sterilizing the medium for oyster mushroom production. Method of producing a medium for sterile cultivation of sterile mushrooms, which can produce mushrooms with excellent marketability while saving energy because it can omit the most important sterilization process for the prevention of secondary pollution in mushroom cultivation by maintaining the alkali condition. It relates to a prepared oyster mushroom medium.

Sterilized medium, calcium hydroxide, pH, spawn, medium raw material, oyster mushroom

Description

Method for making oyster mushroom cultivation medium and medium for cultivating oyster mushroom using the same {Method for making of nutrient broth for cultivating Oyster mushrooms and nutrient broth for cultivating Oyster mushrooms made hence}

The present invention relates to a method for producing a medium for growing oyster mushrooms and a medium for cultivating oyster mushrooms prepared by using the same, and more specifically, maintaining a alkaline amount by mixing a certain amount of calcium hydroxide in a dry medium mixed with the main medium of oyster mushroom production. The present invention relates to a method for producing a non-sterilized oyster mushroom cultivation medium that can produce oyster mushrooms having excellent merchandise even without high temperature heating sterilization by preventing secondary bactericidal effects of microorganisms and sterilization effect, and a medium for cultivating oyster mushrooms prepared using the same. .

Oyster mushroom has been widely edible to mankind since ancient times by its unique flavor and high nutritional value, and in modern times it is regarded as the third food given to mankind. In the past, it has been known to be effective in simply anti-cancer effect and strengthening immunity of human body, but the discovery of special ingredients in oyster mushroom and the physiological function of these ingredients have been revealed, as well as Western countries as well as Japan, China and many other countries around the world. As a result, the government has established a policy of preserving and nurturing the genetic characteristics of oyster mushrooms, and the demand for oyster mushroom cultivation medium is greatly increased as the cultivation area of oyster mushrooms increases. Therefore, the development of mass production technology that can reduce the cost of growing oyster mushroom is required throughout the world, and the situation is being developed.

In order to cultivate oyster mushrooms, holes were drilled in oak and cottonwood trees and inoculated and inoculated with mycelium in the holes, but the medium itself was hardened (hardened), resulting in prolonged sticking period and difficulty in maintaining proper humidity. There was a problem that the length of time required for production. In order to solve this problem, recently, a medium is prepared by using a blend of crests, rice bran, waste noodles, sawdust, and the like.

Conventional methods for producing such a medium include, first, a blending step of blending various raw materials constituting the medium and mixing water;

Secondly, depositing the blended mixture at a constant height and adjusting the amount of moisture to be contained;

Thirdly, sterilizing with a high temperature heat for a certain time to destroy the bacteria in the mixture of the second step;

Fourth, through the fermentation step of fermenting the sterilized mixture in the same place as the general fermentation plant to prepare a medium.

The medium prepared as described above is a granular work laid down by a predetermined amount on the upper woven in three to four stages, and then flattened to flatten the medium to a certain thickness, and then seeded with seedlings to grow mushrooms. will be.

However, the production method of the mushroom cultivation medium as described above has a disadvantage in that the manufacturing process is complicated and takes a long time, and in addition, in order to destroy the germs of the medium, the high-temperature sterilization process must be performed. This raises the cost of production and lowers the competitiveness.

In order to solve this problem, it is possible to purchase and use sealed media such as polypropylene (PP) stem after sterilization in the media manufacturing plant, but discard the media in which the secondary infection caused by contact with the atmosphere during transportation is occurred. Or, there is a problem that needs to be used again by high temperature heating sterilization.

Therefore, it is necessary to simplify the manufacturing process of the cultivation medium for oyster mushroom, and to develop a method for producing a mushroom cultivation medium that can effectively kill various bacteria and prevent contamination even without high temperature heat sterilization treatment.

The present invention was devised to solve the problems of the conventional method for producing the cultivated mushrooms for Pleurotus erythritis, by mixing a certain amount of calcium hydroxide in a dry medium mixed with the main media raw material of the production of Pleurotus mushrooms to make alkaline conditions 2 Non-sterilized oyster mushroom cultivation medium that can shorten the production time of the medium that can produce healthy mushrooms that are not contaminated without high temperature heating sterilization, and can drastically reduce the production cost such as raw material cost and labor cost. To provide a method for producing and a culture medium for growing oyster mushroom prepared using the same as the problem.

When the appropriate amount of solution in which 100 g of calcium hydroxide [purity 95%] is dissolved in 1 liter of groundwater is dried, the pH of the medium is increased to become strong alkaline. In this chemical reaction, if the temperature of the medium is maintained at 15 ℃ or higher, the reaction with the salted calcium hydroxide solution is promoted, and the pH of the medium is gradually lowered to maintain the pH 7 suitable for the growth of mushroom mycelium. Is the same as

Therefore, the inventors of the present invention, since the physiological characteristics of the oyster mushroom and yellow locust mushroom require more calcium than other mushrooms, the calcium hydroxide that can satisfy this generates heat in the process of dissolution and becomes strong alkaline, thus determining the medium. The structure is crystallized so that the mushroom can be easily used as a nutrient source, and the germs in the medium are also sterilized or weakened, so that the growth is suppressed. The experiment was carried out with the idea that the mushrooms could be grown by the researchers. In addition, since humans require a large amount of calcium in minerals due to their physiological characteristics, it was determined that using oyster mushrooms produced with non-sterile medium treated with calcium hydroxide would be an effective calcium food source, thus completing the present invention.

In order to solve the above problems, the present invention is a method for producing a cultivated oyster mushroom medium prepared by mixing the medium raw material, one kind selected from the group consisting of corn cobs, rice bran, lung noodles or sugar cane watermelon as the medium raw material to the total amount of the medium Alternatively, after mixing two or more mixtures of dry medium 94.5 to 95% by weight and 5 to 5.5% by weight of calcium hydroxide, the mixture is placed in a mixer so that the optimum pH of the medium is 9 to 10, and water is added so that the medium humidity is 60 to 65%. It provides a method for producing a medium for growing oyster mushroom, characterized in that to be mixed uniformly for 30 minutes.

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In addition, the present invention, after mixing the dry medium and calcium hydroxide, the pH is measured, and when the pH is less than 9 after the measurement further comprises the step of further processing calcium hydroxide so that the optimum pH after mixing to 9 It provides a method for producing a culture medium.

In addition, the present invention is prepared by the above production method, and provides a medium for growing oyster mushroom, characterized in that the pH of the medium after the production is 9 to 10.

Method for producing a culture medium for oyster mushroom cultivation according to the present invention is a method for producing an sterile medium prepared by alkali treatment using calcium hydroxide, which can effectively destroy germs by calcium hydroxide without high temperature heating sterilization, and prevent contamination of various germs. Unlike conventional sterilization medium, it is possible to inoculate mycelium immediately without going through sterilization and fermentation process, which significantly shortens the process of growing oyster mushrooms, and indirectly shortens the mushroom production cycle.

In addition, the production method according to the present invention has the effect of reducing the production cost and shortening the mushroom production cycle by shortening the mushroom cultivation process by eliminating the sterilization process and fermentation process to improve productivity.

Hereinafter, the present invention will be described in more detail.

Method for producing a culture medium for oyster mushroom cultivation according to the present invention is put a dry medium 94.5 ~ 95.0% by weight, calcium hydroxide 5 ~ 5.5% by weight in a mixer, adding water so that the medium humidity is 60 ~ 65% for a predetermined time Is made evenly miscible.

When the added amount of calcium hydroxide is less than 5.0% by weight, the pH value of the medium is too low, the rate of mycelial growth is fast, but the growth rate of various bacteria is also fast, and the level of contamination of various bacteria is 50% at the level of mycelial growth of the medium. It was 50%, and there was a problem that the bacteria were contaminated with the whole medium within 10 days, so that it was difficult to obtain the antifouling effect of the bacteria. There is no disadvantage, but the inoculated spawn is killed or weakened, so that the spawn of the spawn is late and the completion date of the mycelia culture is long.

The mixture of the dry medium and calcium hydroxide is added to a mixer, and the mixing time is preferably 15 to 30 minutes. This is to ensure that the pH of the medium immediately after the calcium hydroxide treatment is about 11 when measured with a pH meter, and the optimum pH of the mushroom is 9 to 10 while adding water so that the medium humidity becomes 60 to 65%. In particular, it is more preferable that the pH value is 9 preferably.

According to the present invention, the pH of the medium immediately after calcium hydroxide treatment is about 11, and the mixing time is 15 minutes or more, the pH of the calcium hydroxide treatment medium is lowered to about 10, and the pH after mixing for about 30 minutes is lowered to about 9, so that the optimum pH suitable for mushroom growth. It will have a value.

If the pH after mixing is 9 or less, it can be adjusted to pH 9 or more by further treatment with calcium hydroxide.

The pH of the medium prepared by the method for preparing the oyster mushroom cultivation medium according to the present invention is preferably 9 to 10, and more preferably, calcium hydroxide is treated so that the optimum pH of the medium is 9. In this case, as an example of the calcium hydroxide treatment, a calcium hydroxide solution may be prepared by dissolving calcium hydroxide in groundwater, followed by mixing with a suitable amount of the calcium hydroxide solution. As an example, 100 g of calcium hydroxide [purity 95%] is dissolved in 1 liter of groundwater to prepare a calcium hydroxide solution, and the calcium hydroxide solution is mixed while being administered so that an appropriate pH is 9 or more.

Here, the concentration of the calcium hydroxide solution can be used to be prepared by adjusting appropriately during the manufacturing process, it does not necessarily have to use calcium hydroxide solution, it may be mixed by directly administering calcium hydroxide.

Tobacco used in the method for preparing the oyster mushroom cultivation medium according to the present invention uses one or two or more kinds selected from the group consisting of corncob, rice bran, waste noodles or sugarcane watermelon. Preferably, it is good to use a mixture of two or more kinds, and may be used by further mixing other nutrient sources as needed.

Hereinafter, a preferred embodiment of the present invention having the above-described technical configuration will be described. However, the present invention is not limited to the following examples.

Example 1

4 to 6.0% by weight of calcium hydroxide [Ca (OH) ₂ ] was added to the mixer, and the medium was mixed uniformly for 30 minutes while adding water so that the medium humidity was 60 to 65%. In order to check the pH of the culture medium was measured three times with a pH meter (Fisher scientific, accumet model 50), inoculated oyster mushroom spawn in the prepared medium and compared the contamination rate of each sterilized medium by pH It is shown in Table 1 below. At this time, toast was used corncob.

As shown in Table 1, in the case of the medium having a pH of 11 or more, there was no hybridization in a strong alkaline state, but the inoculated spawn was killed or weakened, and thus the spawning of the spawn was delayed, which took about 35 days. In the medium of pH 9-10, there was no incidence of mycelia, and mycelial culture was faster than that of pH 11, so the completion of mycelial culture was advanced 2-3 days. In the medium below pH 8, the rate of mycelial growth was high, but the growth rate of various bacteria was also fast. When the mycelial growth rate was 50%, the contamination level of the bacteria was 50%, and it spreaded to the whole medium within 10 days. .

Referring to FIG. 1, FIG. 1 is a photograph showing arrangements of mycelia and contaminants of various mycelia after pH treatment of calcium hydroxide prepared in Example 1, but no occurrence of bacteria in medium (A) having a pH of 11. It can be seen that the mycelia were killed about 40%, in the medium (B) with a pH of 10, no germs were generated, and the mycelia were 100% active. It progressed faster than B and 100% completed, and the medium (D) having a pH of 8 or less showed that 100% of inoculated mycelia were killed from contaminated bacteria.

In other words, when the medium was prepared so that the calcium hydroxide was mixed in the medium, and the pH was adjusted to 9 to 10, various bacteria in the medium were killed, and the humidity and temperature of the medium were maintained at the proper level, which resulted in the best condition for the growth of Pleurotus eryngii. . It was found that calcium was used as a nutrient source for mycelial growth, and the strength of the mycelia became stronger, showing an advantage in competition with the remaining germs, thereby inhibiting the growth of the germs.

2 is a view showing the growth of fruiting bodies (B, C) from the C state of FIG. Giving.

[Example 2]

According to the results obtained in Example 1, a sterile medium was prepared to inoculate the seedlings of Pleurotus eryngii, and various characteristics of the grown Pleurotus eryngii were investigated.

1. Method of producing alkaline treatment medium

95% by weight of corncob and 5% by weight of calcium hydroxide [Ca (OH) ₂ ] were added to the mixer in a toast to the total amount of the medium, and the medium was uniformly mixed for 30 minutes while adding water so that the medium humidity was 60-65%. In order to confirm the pH of the medium miscification process, the pH was measured three times with a pH meter (Fisher scientific, accumet model 50).

The medium prepared as described above was used for mulching black vinyl (pore diameter 70 ~ 100 mm) to control the uniform generation of mushrooms after spawn spawn.

2. Test strain

Medium strains of wild geology, which are collected from cultivated seedlings No. 1 (summer varieties), low temperature spring No. 1 (spring, boulder, and winter varieties), and Jirisan on a sterile medium, using the seedlings of oyster mushrooms. 1 (summer variety) was inoculated.

3. Inoculation and spawning of spawn

There are three kinds of seeding inoculation methods of sterile medium, mixed inoculation method, interlayer inoculation method, and seeding inoculation on the upper surface of the medium. (OH) ₂ ) was immediately inoculated immediately to the medium prepared by mixing and seeding, 20% of the total medium weight.

After inoculation, the indoor temperature is 23 ℃, the average temperature of the medium is 24 ~ 26 ℃, the medium moisture is 60 ~ 65%, the cultivator's humidity is 55 ~ 60%, the pH of the medium is 6.5 ~ 7.0, and the indoor temperature is 25 ~ 27 ℃, The average temperature of the medium was maintained at 27-29 ℃, and the atmospheric humidity was maintained at 90-95% for mycelial culture. Before starting the spawn, the spawn was removed from the spawn bottle for 3-5 days and placed in a large plastic bag to enable the mycelium to be activated. Stored at 20 ℃ and when used as a spawn was used to cut the mycelia to 20 ~ 30mm size.

In the case of mixed inoculation, 70% of the medium spawn was mixed in the medium, and 30% was granulated and evenly sprayed on the upper side of the medium.

In the interlayer inoculation, 30% of the total medium volume was evenly sprayed on the road surface, and then 30% of the spawn seed was placed thereon, the medium was spread over the seed, and 40% of the spawn was inoculated on the medium.

In the present invention, the layer inoculation method was selected, and the top surface of the seedlings was horizontally selected using a circular digger, and then covered with mulching vinyl to prevent the medium from drying.

When the spawn inoculation is completed, cover the transparent breathing film on the mulching vinyl so that the media hyphae does not dry for 5-7 days and then turn on the humidifier when activated on the top of the granulation so that the growth area of the mycelia becomes 30% of the total. It was rolled up, and the medium and the mulching vinyl were stuck closely together.

In the case of terrestrial seedling cultivation, 0.05% calcium hydroxide solution was sprayed on the surface of the surface on which the medium was to be laminated. Ventilation facilities of ground plate type growers in the house should be maintained so that the culture temperature and humidity conditions were maintained and the concentration of methane gas or carbon dioxide was not increased from the medium. However, when the hyphae are cultured, the humidity should be maintained at 65%. However, if the medium becomes overly moist and the medium is too humid, the culture of the bacteria is delayed, deterioration occurs, and bacterial browning disease occurs when mushrooms are controlled. After the end of the mycelial culture, the bacteria were produced by adjusting the room temperature to 18-22 ° C and atmospheric humidity of 90-95%.

4. Cultivation Conditions and Physiological Characteristics of Pleurotus eryngii Strains

Oyster mushroom spawn for cultivation of oyster mushrooms using a medium made of calcium hydroxide [Ca (OH) 2] treatment, that is, sterile medium, is spring 1 (spring, autumn and winter varieties), suhan 1 (summer varieties), geography The mycelia of the wild fruit No. 1 (summer varieties) mushrooms were isolated, transplanted into a malt agar incubator and incubated at 26 ° C. for 10 days, and the cultivation conditions were shown in Table 2.

As a cultivation condition of the cultivated strains of Pleurotus eryngii, the growth temperature of the mycelium is 22 ~ 26 ℃, the temperature of germ development (initial) is 16 ~ 22 ℃, the forming temperature of fruiting body is 8 ~ 16 ℃, the humidity of the medium is 65%, The growth rate was 75-80%, roughness 400-500 lux, carbon dioxide concentration below 1000 ppm. The physiological characteristics of the wild ginseng No. 1 used in this study were compared with the summer varieties of Suhan No. 1 and Spring 1, which can be cultivated in spring, autumn, and winter. Gili Wild Wine No. 1, which was harvested from, was found to be suitable for growing under high temperature conditions in summer.

To date, all oyster mushrooms used for cultivation and production must be sterilized and fermented, but the sterilized medium prepared by the alkali treatment method using calcium hydroxide of the present invention does not undergo a fermentation process unlike conventional sterilization media. Since it can be inoculated immediately with mycelium, it not only drastically shortened the mushroom cultivation process, but also developed a new technology to indirectly shorten the mushroom production cycle and conducted experiments to verify it. That is, the fruit diameter of the mushroom produced by transplanting the cultivars of oyster mushroom into the sterilized medium, the length of the bag, the diameter of the bag, the diameter of one mushroom, the color of the mushroom, the color of the mushroom, the quality of the mushroom and the production of the first class The result of examining the ratio is shown in Table 3.

The quality of the mushrooms is closely related to balance and harmony, that is, the fruiting body (large) diameter, the length of the sacks (large), the size and color of the head (head) and the weight of the mushroom. Therefore, comparing the characteristics of Jiri wild sake No. 1 grown in the same conditions and Suhan No. 1, a cultivar for summer cultivation, and mushrooms, the diameter of the mushroom stalk is about 19 mm thick, the length of the bag is 10.7 mm long, and the diameter of the gat is 6 mm larger and weighed 2 g heavier. However, the difference between the weight and size of the mushrooms is not significant, but it was confirmed that the geography wild wine No. 1 is excellent. The yields of mushrooms were compared to that of the first-class production rate of Jiri Wild Wine No. 1> Suhan No. 1> Spring Chu No. 1, and the superior quality of Jiri Wild No. 1 mushrooms resulted in 34% of the yield. Could confirm.

As can be seen from the above description, the medium prepared by the method for producing mushroom cultivation medium according to the present invention is an alkali treatment by mixing a dry medium and calcium hydroxide made of a medium material at a predetermined ratio, and sterilizing by high temperature heat as in the prior art. It can be seen that it is possible to prevent the removal of germs and secondary contamination without going through the fermentation process and the post fermentation process.As an example, the inoculation of spawn seedlings for oyster mushrooms resulted in a shorter growth period and a shorter production cycle. In addition, it can be seen that the excellent oyster mushroom can be produced in terms of loss of seeds and quality due to contamination of various bacteria.

In the present invention, but was carried out for the oyster mushroom, according to the results of the above experimental example, other kinds of mushroom spawn in addition to the oyster mushroom may also obtain the same effect. In other words, the sterilized medium prepared by the present invention is not limited to oyster mushroom.

1 is a photograph showing the state of contamination of the mycelia and the bacteria of the mycelium for each medium pH after treatment with calcium hydroxide according to the present invention.

Figure 2 is a picture showing the growth of the fruiting body (B, C) from the C state of FIG.

Claims (5)

In the method for producing a oyster mushroom cultivation medium prepared by mixing a medium raw material, 9,5 to 9, which is one or a mixture of two or more selected from the group consisting of corncobs, rice bran, waste cotton or sugarcane watermelon, which are medium raw materials relative to the total amount of the medium. After mixing 95% by weight and 5% to 5.5% by weight of calcium hydroxide, the optimum pH of the medium is placed in a mixer such that the pH is 9 to 10, and the mixture is uniformly mixed for 15 to 30 minutes while adding water so that the medium humidity becomes 60 to 65%. Method for producing a culture medium for oyster mushroom. delete delete According to claim 1, After the mixing, pH measurement, and after the measurement when the pH is less than 9 further processing the calcium hydroxide so that the optimum pH is 9 to 10 after mixing, Oyster mushroom culture medium Manufacturing method. Prepared by the method according to any one of claims 1 or 4, the medium for cultivating oyster mushroom, characterized in that the pH of the medium after the production is 9 to 10.

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