JPS60149379A - Production of basidiomycetous fruiting body - Google Patents

Production of basidiomycetous fruiting body

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Publication number
JPS60149379A
JPS60149379A JP449684A JP449684A JPS60149379A JP S60149379 A JPS60149379 A JP S60149379A JP 449684 A JP449684 A JP 449684A JP 449684 A JP449684 A JP 449684A JP S60149379 A JPS60149379 A JP S60149379A
Authority
JP
Japan
Prior art keywords
basidiomycetous
basidiomycete
fruiting body
anthranilic acid
fruiting bodies
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Pending
Application number
JP449684A
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Japanese (ja)
Inventor
Sawao Murao
村尾 澤夫
Hideo Hayashi
英雄 林
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Individual
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Individual
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Application filed by Individual filed Critical Individual
Priority to JP449684A priority Critical patent/JPS60149379A/en
Publication of JPS60149379A publication Critical patent/JPS60149379A/en
Pending legal-status Critical Current

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Abstract

PURPOSE:To obtain a basidiomycetous fruiting body, e.g. an edible mushroom, at a low cost without a change from a dark to a lighted places nor temperature change, by cultivating a basidiomycetous mold starter in a nutrient culture medium containing anthranilic acid, p-aminobenzoic acid, etc. to induce the basidiomycetous fruiting body. CONSTITUTION:A basidiomycetous mold starter is inoculated into a nutrient culture medium containing at least one of anthranilic acid, p-aminobenzoic acid or a metal salt or a mixture thereof and further maltose, polypeptone, a salt such as KH2PO4 or thiamin hydrochloride, etc. and cultivated therein to induce a basidiomycetous fruiting body and give the aimed mushroom. Examples of the basidiomycete to be used include edible mushrooms such as Lentinus edodes (SHIITAKE mushroom), Flammulina velutipes, Panus ostreatus, Pholiota nameko, Auricularia auricula, Lyophyllum aggregatum, etc. and Polyporus orcularius, Polyporaceae versicolor, Elfvinga applanata, etc.

Description

【発明の詳細な説明】 本発明は担子菌子実体の製造法に関する。更に詳しくは
、担子菌種菌をアントラニル酸(別名〇−アミノ安息香
酸)、p−アミノ安息香酸又はそれらのカリウム、ナト
リウム又はカルシウム塩の少なくとも1種又はこれらの
混合物を添加した栄養培地に培養し、担子菌子実体を誘
発せしめることを特徴とする担子菌の製造法に関する。DETAILED DESCRIPTION OF THE INVENTION The present invention relates to a method for producing basidiomycete fruiting bodies. More specifically, the basidiomycete inoculum is cultured in a nutrient medium supplemented with at least one of anthranilic acid (also known as 〇-aminobenzoic acid), p-aminobenzoic acid, or their potassium, sodium, or calcium salts, or a mixture thereof. , relates to a method for producing basidiomycetes, which is characterized by inducing basidiomycete fruiting bodies.

担子菌子実体は、例えば椎茸、エノキ茸、ヒラ茸、ナメ
コ、キクラゲ、松茸などのように食用キノコとして古く
から賞味されているだけでなく、近年種々の有用な生理
活性物質並びに医薬の供給源として特に注目されるよう
になってきた。Basidiomycete fruiting bodies have not only been enjoyed as edible mushrooms for a long time, such as shiitake mushrooms, enoki mushrooms, hiratake mushrooms, nameko mushrooms, wood ear fungi, and matsutake mushrooms, but also in recent years have been used as sources of various useful physiologically active substances and medicines. It has started to attract particular attention.

担子菌子実体の形成には十分な栄養素の供給のみならず
、十分な照明、適当な温度変化等の環境的刺激が必須な
ものとされている。しかしながら担子菌子実体の製造に
おいて、培養途中に暗所から光照射への切り換え操作成
いは培養温度を途中から低下させる等の温度処理等の処
置はそれだけ手間を要し、しかもコスト高を招く要因と
なっていた。For the formation of basidiomycete fruiting bodies, not only the supply of sufficient nutrients but also environmental stimuli such as sufficient lighting and appropriate temperature changes are considered essential. However, in the production of basidiomycete fruiting bodies, temperature treatments such as switching from dark to light irradiation or lowering the culture temperature midway through cultivation are time-consuming and are factors that increase costs. It became.

そこで本発明者らは担子菌子実体の製造に際して暗所か
ら明所への変化、或いは温度変化を施すことなく暗所の
みで且つ一定の温度のままで担子菌種菌を培養すること
により、培地上に担子菌子実体を形成せしめることを可
能とするところの担子菌子実体誘発物質を自然界の微生
物生産物にめた。Therefore, the present inventors cultivated the basidiomycete inoculum only in the dark and at a constant temperature without changing from dark to light or changing the temperature when producing basidiomycete fruiting bodies. A natural microbial product was used as a basidiomycete fruiting body inducer, which makes it possible to form basidiomycete fruiting bodies on top of the basidiomycete.

そしてたまたま放線菌群に属する一菌株TA−7株のブ
ロス中に該担子菌子実体誘発物質を見出すことができた
のであるが、このTA−7株のブロス中の担子菌子実体
誘発物質を積製し、同定したところ、該担子菌子実体誘
発物質がアントラニル酸であることが判−朋したのであ
る。そして更にその関連物質であるp−アミノ安息香酸
にも同様な担子菌子実体誘発作用の存在することを知り
本発明を完成したものである。即ち本発明は担子菌種菌
をアントラニル酸、p−アミノ安息香酸又はそれらの金
属塩又はこれらの混合物を添加した栄養培地で培養し、
担子菌子実体を誘発せしめることを特徴とする担子菌子
実体の製造法である。By chance, we were able to find the basidiomycete fruiting body inducer in the broth of TA-7, a strain belonging to the actinobacteria group. Upon identification, it was determined that the basidiomycete fruiting body inducing substance was anthranilic acid. Furthermore, the present invention was completed after discovering that p-aminobenzoic acid, a related substance, has a similar effect on inducing fruiting bodies of basidiomycetes. That is, the present invention cultivates a basidiomycete inoculum in a nutrient medium supplemented with anthranilic acid, p-aminobenzoic acid, a metal salt thereof, or a mixture thereof,
This is a method for producing a basidiomycete fruiting body, which is characterized by inducing a basidiomycete fruiting body.

本発明で担子菌と称するのは椎茸、エノキタケ、ヒラタ
ケ、ナメコ、キクラゲ、シメン等の食用キノコに限定さ
れず、アミスギタケ、カワラタケ、サルノコシカケ等の
広く担子菌一般をいう。In the present invention, the term "basidiomycetes" is not limited to edible mushrooms such as shiitake, enokitake, oyster mushroom, nameko, wood ear fungus, and cymen, but broadly refers to basidiomycetes in general, such as amis gitake, versicolor, and sarunokoshika.

本発明における担子菌子実体製造用培地は、澱粉、マル
ト−ス、グルコース、シュークロース等の糖質、ペプト
ン、アミノ酸、大豆蛋白、魚粕、硫安等の有機及び無機
窒素源、サイアミン、酵母エキス、C3L、核酸関連物
質等の微量栄養素を適宜組み合わせたもの、又は、これ
らを木屑、オカ屑、米糠、紙屑等と適宜組み合わせたも
の、もしくは、じゃがいも煮汁培地等にアントラニル酸
等の担子菌子実体誘発物質を適量添加する。The medium for producing basidiomycete fruiting bodies in the present invention includes carbohydrates such as starch, maltose, glucose, and sucrose, peptone, amino acids, soybean protein, fish meal, organic and inorganic nitrogen sources such as ammonium sulfate, thiamine, yeast extract, Appropriate combinations of micronutrients such as C3L, nucleic acid-related substances, etc., or appropriate combinations of these with wood chips, oak waste, rice bran, paper waste, etc., or basidiomycete fruiting body inducers such as anthranilic acid in potato broth medium, etc. Add appropriate amount.

種菌の接種法は、通常の方法で良く、接種後20〜30
℃好ましくは25°C前後で10〜40日間暗所にて培
養する。このようにして担子菌子実体が誘発されるか、
更に光照射のもと培養を続けることにより成熟した担子
菌子実体が得られる。The inoculum can be inoculated by the usual method, and 20 to 30 minutes after inoculation.
C., preferably around 25.degree. C., for 10 to 40 days in the dark. In this way, the basidiomycete fruiting body is induced or
Further, by continuing the culture under light irradiation, mature basidiomycete fruiting bodies can be obtained.

本発明で培地に添加するアントラニル酸、p−アミノ安
息香酸又はそれら金属塩は、化学的に合成され容易に入
手が可能である。従ってTA−7菌株をわざわざ培養し
て生産しなくとも入手できる。そして試薬特級のみなら
ず試薬1級及び試薬2級程度の純度のアントラニル酸、
p−アミノ安息香酸又はそれら金属塩又はこれらの混合
物のいずれも、本発明において好適に用いられ得る。Anthranilic acid, p-aminobenzoic acid, or their metal salts added to the culture medium in the present invention are chemically synthesized and easily available. Therefore, the TA-7 strain can be obtained without going to the trouble of culturing and producing it. And anthranilic acid with a purity of not only special reagent grade but also first grade reagent and second grade reagent,
Any of p-aminobenzoic acid or their metal salts or mixtures thereof may be suitably used in the present invention.

次に本発明における担子菌誘発物質であるアントラニル
酸の培地への最適添加量及びアントラニル酸関連化合物
の担子菌子実体誘発能に関する試験例について述べる。Next, a test example regarding the optimal amount of anthranilic acid, which is a basidiomycete-inducing substance, to be added to a medium in the present invention and the ability of anthranilic acid-related compounds to induce basidiomycete fruiting bodies will be described.

試験例1 実施例1に示したものと同し組成の寒天培地を入れたエ
ルシンマイヤーフラスコ10本のそれぞれにアミスギタ
ケ(Favolus arcularius ATCC
24461)を接種し、次いで0.01〜100 ng
/ディスクの各濃度のアントラニル酸をしみ込ませたデ
ィスクをそれぞれのフラスコの周囲に配置し、暗所で2
5°Cで2週間培養した。アミスギタケ子実体誘発能と
アンI−ラニル酸添加量との関係を表−1に示す。Test Example 1 Amysgitake (Favolus arcularius ATCC) was placed in each of 10 Ersinmeyer flasks containing an agar medium with the same composition as that shown in Example 1.
24461) and then 0.01-100 ng
/ Discs impregnated with anthranilic acid at various concentrations were placed around each flask and incubated in the dark for 2 hours.
Cultured at 5°C for 2 weeks. Table 1 shows the relationship between the ability to induce fruit bodies of Amis Gitake and the amount of anI-ranilic acid added.

(以下余白) 表−1 表−1より明らかのようにアントラニル酸の添加量は0
.1〜3 ng/ディスクの範囲(培地中の添加量とし
て、3〜long/−に相当)で子実体誘発能を示すこ
とがわかる。(Left below) Table-1 As is clear from Table-1, the amount of anthranilic acid added is 0.
.. It can be seen that the ability to induce fruiting bodies is shown in the range of 1 to 3 ng/disc (equivalent to 3 to long/- as the amount added in the medium).

試験例2 試験例1におけるディスクにしみ込ませた各種濃度のア
ントラニル酸の代わりにアントラニル酸関連化合物を用
いるほかは試験例1と同様の条件で試験を行った。アン
トラニル酸関連化合物とアミスギタケ子実体誘発能との
関係を表−2に示す。Test Example 2 A test was conducted under the same conditions as Test Example 1, except that an anthranilic acid-related compound was used instead of the anthranilic acid of various concentrations impregnated into the disk in Test Example 1. Table 2 shows the relationship between anthranilic acid-related compounds and the ability to induce fruit bodies of Mysgitake.

但し子実体誘発能の有る場合を(+)とし、無い場合を
(−)で表示した。However, cases with the ability to induce fruiting bodies are indicated as (+), and cases without are indicated as (-).

(以下余白) 表−2 表−2より明らかのようにアントラニル酸、アントラニ
ル酸のナトリウム塩、又はそのカリウム塩の他にも関連
化合物のp−アミノ安息香酸又はp−アミノ安息香酸の
ナトリウム塩、又はそのカリウム塩(1〜3 ng/デ
ィスクの投与量)にアミスギタケ子実体誘発能が見られ
たが、m−アミノ安息香酸、アントラニル酸メチル及び
N−メチルアントラニル酸のいずれにも子実体誘発能は
存在しなかった(0.01〜100 ng/ディスクの
投与量)。(Space below) Table 2 As is clear from Table 2, in addition to anthranilic acid, the sodium salt of anthranilic acid, or its potassium salt, p-aminobenzoic acid or the sodium salt of p-aminobenzoic acid of related compounds, or its potassium salt (dose of 1 to 3 ng/disc) was found to have the ability to induce fruiting bodies of Mysgitake, but neither m-aminobenzoic acid, methyl anthranilate, nor N-methylanthranilate had the ability to induce fruiting bodies. was absent (doses of 0.01-100 ng/disc).

そして又代謝経路においてアントラニル酸と関連性のあ
るトリプトファン及びキヌレニンも、更には、p−アミ
ノ安息香酸基を含んでいる葉酸も0.01〜100 n
g/ディスクの投与においてアミスキタケ子実体誘発能
を有していないことが示される。Tryptophan and kynurenine, which are related to anthranilic acid in the metabolic pathway, as well as folic acid, which contains a p-aminobenzoic acid group, have a concentration of 0.01 to 100 n.
It is shown that it does not have the ability to induce Amisukitake fruiting bodies when administered at 100 g/disk.

試験例1及び2においては担子菌としてアミスギタケを
使用したが、エノキダケ、ヒラタケ、椎茸等のキノコで
も同様な結果が得られた。In Test Examples 1 and 2, Amis Gitake was used as the basidiomycete, but similar results were obtained with mushrooms such as Enoki mushroom, Oyster mushroom, and Shiitake.

本発明による担子菌子実体の製造方法は極めて?に量の
アントラニル酸、それのナトリウム塩、カリウム塩又は
カルシウム塩、p−アミノ安息香酸、これのナトリウム
塩、カリウム塩又はカルシウム塩を添加した培養培地に
種菌を接種し、且つ暗所において一定温度で培養するの
みで子実体が誘発されるのであり、これはこれまでのキ
ノコ栽培技術では想像することさえできない画期的なこ
とである。Is the method for producing basidiomycete fruiting bodies according to the present invention extremely? The inoculum was inoculated into a culture medium to which anthranilic acid, its sodium salt, potassium salt, or calcium salt, p-aminobenzoic acid, its sodium salt, potassium salt, or calcium salt was added, and the culture medium was kept at a constant temperature in the dark. Fruiting bodies can be induced simply by culturing the mushrooms, which is an epoch-making phenomenon that could not even be imagined using conventional mushroom cultivation techniques.

以下に実施例にて本発明を具体的に説明する。The present invention will be specifically explained below with reference to Examples.

実施例1 マルトース20g1ボリベプI・ン1 g 、KH2P
O40,3g、MgSO4・71120’0.3g、 
CaCl2・2H200,1g。Example 1 Maltose 20g 1 Volibep I・N 1g, KH2P
O40.3g, MgSO4・71120'0.3g,
CaCl2.2H200, 1g.

Zn5O+ ・7 H2O0,3n+g、FeSO4−
7H2O0,15mg、CuSO4・5 H2O0,1
nv、MnSO4・5H200,1nw、(N114 
)6 Mo7024 ・t1200.02mg、チアミ
ン塩酸塩0.1■、アントラニル酸(和光純薬製、試薬
特級)3/’gを1000mの水に溶解したもの(pH
5,2,)’ 5(1ml!を200me容エルレンマ
イヤーフラスコに分注シ、加熱殺菌後、アミスギタケ(
Favolus arculariusAT、CC24
461)を接種して暗所で25℃で2週間培養したとこ
ろ、フラスコ中に数本の子実体が形成された。一方、ア
ントラニル酸無添加の場合は暗所では子実体は形成され
ず、明所に移してから2日目に原基が形成され、更に3
日目に子実体が得られた。Zn5O+ ・7 H2O0,3n+g, FeSO4−
7H2O0,15mg, CuSO4・5 H2O0,1
nv, MnSO4・5H200,1nw, (N114
)6 Mo7024・t1200.02mg, thiamine hydrochloride 0.1■, anthranilic acid (Wako Pure Chemical Industries, Ltd., reagent special grade) 3/'g dissolved in 1000m water (pH
5,2,)' 5 (1ml!) was dispensed into a 200me Erlenmeyer flask, and after heat sterilization, Amis Gitake (
Favolus arcularius AT, CC24
461) and cultured in the dark at 25°C for 2 weeks, several fruiting bodies were formed in the flask. On the other hand, in the case where anthranilic acid is not added, fruiting bodies are not formed in the dark, but primordia are formed on the second day after being transferred to the light, and then 3
Fruiting bodies were obtained on day one.

実施例2 アントラニル酸にかえてp−アミノ安息香酸を10pr
g添加する以外には実施例1と同じ組成の培地50me
を200+++(!容エルレンマイヤーフラスコに分注
し、加熱殺菌後、アミスギタケ(Favolus ar
cula−rius ATCC24461)を接種して
暗所で25°Cで15日間培養したところ、フラスコ中
に多数の子実体が形成された。一方、p−アミノ安息香
酸無添加の場合には暗所では子実体は誘発されず、明所
に移してから2日目に原基が形成され、更に3日経過後
子実体が形成された。Example 2 10 pr of p-aminobenzoic acid instead of anthranilic acid
50me of medium having the same composition as in Example 1 except that g was added.
was dispensed into Erlenmeyer flasks with a capacity of 200 + + + (!), and after heat sterilization, the Favolus
cula-rius ATCC24461) and cultured in the dark at 25°C for 15 days, numerous fruiting bodies were formed in the flask. On the other hand, when p-aminobenzoic acid was not added, fruiting bodies were not induced in the dark, primordia were formed on the second day after transfer to the light, and fruiting bodies were formed after a further 3 days.

実施例3 ジャガイモ煮汁培地(新鮮ジャガイモ300gを30分
間加熱抽出してlooomEの煮汁を得、マルト−スを
10g加えたもの)にアントラニル酸3pgを加えiM
したのち、 10〇−容エルレンマイヤーフラスコに分
注し、 120℃で15分間殺菌し冷却後、エノキタケ
(Flammulina velutipes IFO
7045)を接種し、暗所で25℃で38日間培養した
ところ、フラスコ中に多数の子実体が誘発された。一方
アントラニル酸無添加の培地では38日間培養しても子
実体は形成されなかった。子実体を形成せしめるには1
4日間暗所で25°Cにて培養後、明所に移し、しかも
17℃に温度を低下せしめて11日間培養することによ
り子実体原基が形成され、更に培養を続けて13日経過
後に子実体が形成された。Example 3 3 pg of anthranilic acid was added to a potato broth medium (300 g of fresh potatoes were heat-extracted for 30 minutes to obtain a broth of looomE, and 10 g of maltose was added).
After that, it was dispensed into a 100-capacity Erlenmeyer flask, sterilized at 120°C for 15 minutes, and after cooling, it was mixed with enokitake (Flammulina velutipes IFO).
7045) and cultured in the dark at 25°C for 38 days, a large number of fruiting bodies were induced in the flask. On the other hand, no fruiting bodies were formed even after 38 days of culture in a medium without anthranilic acid. To form fruiting bodies 1
After culturing at 25°C in the dark for 4 days, the fruiting body primordium was formed by culturing in the light and lowering the temperature to 17°C for 11 days, and after 13 days of continued culture. Fruiting bodies were formed.

実施例4 サッカロースLog 、ポリペプトン2g、KH2PO
40,5g、MgSO4・711200.5g、 Ca
Cl2−211200.’1g。Example 4 Sucrose Log, polypeptone 2g, KH2PO
40.5g, MgSO4・711200.5g, Ca
Cl2-211200. '1g.

チアミン塩酸塩0.1■、ZnSO4・5 )120 
0.3■、FeSO4・7 N200.15mg、Cu
SO4・51120 0.1mg、MnSO4・5 N
20 0.1m1r、、(N114 )6 Mo702
4 ・H2!00.02mg及びp−アミノ安息香酸N
a塩10pgを水100〇−に熔解したもの20m1を
50mn容エルレンマイヤーフラスコに分注し、加熱殺
菌後ヒラタケ(Pleuro−tus anserin
’a IFO7051)を接種して、27℃で暗所で3
5日間培養したところ、フラスコ中に多数の子実体が誘
発された。一方、p−アミノ安息香酸無添加の場合には
子実体が誘発されず、子実体を形成させるには、暗所で
14日間培養後、17℃の明所に移し、11日間培養を
続ける処置が必要であった。Thiamine hydrochloride 0.1■, ZnSO4.5) 120
0.3■, FeSO4・7 N200.15mg, Cu
SO4・51120 0.1mg, MnSO4・5N
20 0.1m1r, (N114)6 Mo702
4 ・H2!00.02mg and p-aminobenzoic acid N
Dissolve 10 pg of a-salt in 1,000 ml of water, dispense 20 ml into a 50-mn Erlenmeyer flask, and heat-sterilize it.
'a IFO7051) and incubated in the dark at 27℃ for 3
After culturing for 5 days, many fruiting bodies were induced in the flask. On the other hand, when p-aminobenzoic acid is not added, fruiting bodies are not induced, and in order to form fruiting bodies, after culturing in the dark for 14 days, transfer to a light place at 17°C and continue culturing for 11 days. was necessary.

実施例5 実施例1における培地組成のうちアントラニル酸3pg
にかえてアントラニル酸とp−アミノ安息香酸の混合物
(比率1 : 2)lhgを使用する以外は同じ組成の
培地を使用し、その50−を20〇−容エルレンマイヤ
ーフラスコに分注し、加熱殺菌後、アミスギタケ(Fa
volus arcularius ATCC2446
1)を接種して暗所で25°Cで15日間培養したとこ
ろ子実体が多数フラスコ中に誘発された。一方アントラ
ニル酸とp−アミノ安息香酸の混合物無添加の培養にお
いては20日間培養しても子実体は誘発されなかった。Example 5 Of the medium composition in Example 1, 3 pg of anthranilic acid
A medium with the same composition was used, except that a mixture of anthranilic acid and p-aminobenzoic acid (ratio 1:2) was used instead, and 50-mL of the medium was dispensed into a 200-volume Erlenmeyer flask. After heat sterilization, Amis gitake (Fa
volus arcularius ATCC2446
1) and cultured in the dark at 25°C for 15 days, many fruiting bodies were induced in the flask. On the other hand, in the culture without the addition of the mixture of anthranilic acid and p-aminobenzoic acid, fruiting bodies were not induced even after 20 days of culture.

実施例6 実施例1における培地組成のうち、アントラニル酸3p
gにかえてアントラニル酸カリウム3pgを使用する以
外は同じ組成の培地を使用し、その50−を200−容
エルレンマイヤーフラスコに分注し、加熱殺菌後、アミ
スギタケ(Favolus arculariusAT
CC24461)を接種して暗所で25℃で14日間培
養したところ、フラスコ中にアミスギタケ子実体が多数
誘発された。一方アントラニル酸カリウム無添加の場合
は20日間培養してもアミスギタケ子実体は誘発されず
、子実体を誘発させるためには6日間暗所で培養し、次
いで明所に移し5日間培養する必要があった。Example 6 Among the medium compositions in Example 1, anthranilic acid 3p
A medium with the same composition was used, except that 3 pg of potassium anthranilate was used instead of 3 pg of potassium anthranilate, and 50 g of the culture medium was dispensed into a 200-capacity Erlenmeyer flask, and after heat sterilization, the culture medium was incubated with Favolus arcularius AT.
CC24461) and cultured in the dark at 25°C for 14 days, a large number of Mysgitake fruiting bodies were induced in the flask. On the other hand, when potassium anthranilate is not added, Amis Gitake fruiting bodies are not induced even after 20 days of culture; in order to induce fruiting bodies, it is necessary to culture in the dark for 6 days, then transfer to a light place and culture for 5 days. there were.

実施例7 実施例1で使用した培地組成のうちアントラニル酸3p
gにかえてアントラニル酸カルシウム3 )sgを使用
する以外は同じ組成の培地を使用し、その50−を20
0m1!容エルレンマイヤーフラスコに分注し、加熱殺
菌後、アミスギタケ(Favolus arcula−
rius ATCC24461)を接種し、暗所で25
°Cで14日間培養したところフラスコ中にアミスギタ
ケ子実体が多数誘発された。一方アントラニル酸カルシ
ウム無添加の培地では20日間培養してもアミスギタケ
子実体は誘発されなかった。Example 7 Among the medium compositions used in Example 1, anthranilic acid 3p
Calcium anthranilate 3) sg was used instead of sg, but a medium with the same composition was used, and the 50-sg was replaced with 20-sg.
0m1! Pour into Erlenmeyer flasks, heat sterilize, and add Favolus arcula.
rius ATCC24461) and inoculated in the dark for 25 minutes.
When cultured at °C for 14 days, many fruiting bodies of Mysgitake were induced in the flask. On the other hand, in the medium containing no calcium anthranilate, fruiting bodies of Mysgitake were not induced even after 20 days of culture.

実施例8 実施例3のジャガイモ煮汁10100O!中に添加した
アン1−ラニル酸3 Jjgにかえてアントラニル酸と
p−アミノ安息香酸の混合物(混合比率1:1)10J
’gを添加し、その20meを100−容エルレンマイ
ヤーフラスコに分注し、加熱殺菌後、エノキタケ(Fl
ammulina velutipes IFO704
5)を接種し、暗所で27℃で38日間培養したところ
、フラスコ中に多数のエノキタケ子実体が誘発された。Example 8 Potato broth of Example 3 10100O! 10 J of a mixture of anthranilic acid and p-aminobenzoic acid (mixing ratio 1:1) in place of 3 Jjg of anthranilic acid added in the mixture.
20me was added to a 100-capacity Erlenmeyer flask, and after heat sterilization, enokitake (Fl.
ammulina velutipes IFO704
5) and cultured in the dark at 27°C for 38 days, a large number of Enokitake fruiting bodies were induced in the flask.

一方アントラニル酸とp−アミノ安息香酸の混合物を無
添加の場合50日間培養してもエノキタケ子実体は誘発
されなかった。On the other hand, when the mixture of anthranilic acid and p-aminobenzoic acid was not added, enokitake fruiting bodies were not induced even when cultured for 50 days.

【図面の簡単な説明】[Brief explanation of drawings]

第1図′a)はエノキタケ子実体の従来の製造法の概略
を示すものであり、第1図(b)はアミスギタケ子実体
の従来の製造法の概略を示すものである。第2図(a)
は本発明のエノキタケ子実体の製造法の概略を示すもの
であり、第2図(b)は本発明のアミスギタケ子実体の
製造法の概略を示すものである。 特許出願人 村尾澤夫C9 第 1 (a) (b) 接種 光照射 子実体原基 成熟子実体 3 野 ト 子実体原基 成熟子実体 9 (− 第2図 (a) 接 種 成熟子実体 (b) 接 種 成熟子実体 25°C,lh’f所 手続補正書(方式) %式% 1、事件の表示 昭和59年 特許願第4496号 2、発明の名称 担子菌子実体の製造法 3、補正をする者 事件との関係 特許出願人 住所 大阪府堺市堀上縁町2丁8−12昭和59年4月
24日 5、補正の対象 「図 面」 6、補正の内容FIG. 1'a) shows an outline of the conventional method for producing the fruiting body of Enokitake mushroom, and FIG. 1(b) shows an outline of the conventional method for producing the fruiting body of Enokitake mushroom. Figure 2(a)
FIG. 2(b) schematically shows the method for producing the fruiting body of Enokitake mushroom of the present invention, and FIG. Patent applicant Sawao Murao C9 No. 1 (a) (b) Inoculation Light-irradiated fruiting body primordium Mature fruiting body 3 Noto fruiting body primordium Mature fruiting body 9 (- Fig. 2 (a) Inoculation Mature fruiting body (b) ) Inoculation Mature fruiting body 25°C, lh'f Office procedure amendment (method) % formula % 1. Indication of the case 1982 Patent Application No. 4496 2. Name of the invention Process for producing Basidiomycete fruiting body 3. Amendment Relation to the case of a person who does

Claims (1)

【特許請求の範囲】 ■ 担子菌種菌をアントラニル酸、p−アミノ安息香酸
又はそれら金属塩の少なくとも1種又はこれらの混合物
を添加した栄養培地で培養し、担子菌子実体を誘発せし
めることを特徴とする担子菌子実体の製造法。 2 担子菌種菌の培養が11η所のみの培養であること
を特徴とする特許請求の範囲第1項記載の担子菌子実体
の製造法。 3 担子菌種菌の培養が一定温度での培養であることを
特徴とする特許請求の範囲第1項又は第2項記載の担子
菌子実体の製造法。[Claims] ■ A basidiomycete inoculum is cultured in a nutrient medium supplemented with at least one of anthranilic acid, p-aminobenzoic acid, or a metal salt thereof, or a mixture thereof, to induce basidiomycete fruiting bodies. A method for producing basidiomycete fruiting bodies. 2. The method for producing a basidiomycete fruiting body according to claim 1, wherein the basidiomycete inoculum is cultured only at 11η sites. 3. The method for producing a basidiomycete fruiting body according to claim 1 or 2, wherein the basidiomycete inoculum is cultured at a constant temperature.
JP449684A 1984-01-12 1984-01-12 Production of basidiomycetous fruiting body Pending JPS60149379A (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
JP449684A JPS60149379A (en) 1984-01-12 1984-01-12 Production of basidiomycetous fruiting body

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
JP449684A JPS60149379A (en) 1984-01-12 1984-01-12 Production of basidiomycetous fruiting body

Publications (1)

Publication Number Publication Date
JPS60149379A true JPS60149379A (en) 1985-08-06

Family

ID=11585676

Family Applications (1)

Application Number Title Priority Date Filing Date
JP449684A Pending JPS60149379A (en) 1984-01-12 1984-01-12 Production of basidiomycetous fruiting body

Country Status (1)

Country Link
JP (1) JPS60149379A (en)

Cited By (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US7354590B2 (en) * 2003-04-09 2008-04-08 Jarrow Formulas, Inc. Methods of producing edible fungi containing activated folates and nutritional supplements containing activated folates
CN115039639A (en) * 2022-08-17 2022-09-13 云南菌视界生物科技有限公司 Tremella liquid strain short-period production method and application of tremella liquid strain

Cited By (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US7354590B2 (en) * 2003-04-09 2008-04-08 Jarrow Formulas, Inc. Methods of producing edible fungi containing activated folates and nutritional supplements containing activated folates
US7682606B2 (en) 2003-04-09 2010-03-23 Jarrow Formulas, Inc. Methods of producing edible fungi containing activated folates and nutritional supplements containing activated folates
CN115039639A (en) * 2022-08-17 2022-09-13 云南菌视界生物科技有限公司 Tremella liquid strain short-period production method and application of tremella liquid strain
CN115039639B (en) * 2022-08-17 2022-11-22 云南菌视界生物科技有限公司 Tremella liquid strain short-period production method and application of tremella liquid strain

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