气升式液体培养假褐云斑鹅膏菌丝及毒素检测分析

采集并组织分离到假褐云斑鹅膏Amanita pseudoporphyria的纯培养菌丝。培养发现其在琼脂培养基上生长形态与一般蕈菌有差别。摇瓶液体培养条件下,假褐云斑鹅膏菌丝体干重为0.626g/L,在气升式反应器内假褐云斑鹅膏菌丝体干重可达到1.629g/L。反应器培养的菌丝体毒素的HPLC分析表明菌丝体内含有鹅膏毒肽,而不含有鬼笔毒肽。结果表明可以通过液体培养鹅膏菌丝体来生产鹅膏毒素。     

7种鹅膏菌属真菌肽类毒素的HPLC分析

利用HPLC法对长白山地区分布的7种鹅膏属真菌成熟子实体中的α鹅膏毒肽(αamanitin)、β鹅膏毒肽(βamanitin)和鬼笔毒肽(phalloidin)的含量进行了测定。结果表明:芥橙黄鹅膏(Amanitasubjunquillea)和橙黄鹅膏(Amanitaaff.citrina)中均含有3种毒素,其中芥橙黄鹅膏的α鹅膏毒肽含量为2395.91μg/g、β鹅膏毒肽含量为1653.75μg/g和鬼笔毒肽含量为405.26μg/g;橙黄鹅膏的分别为1121μg/g、4244μg/g和9442μg/g。芥橙黄鹅膏白色变种(Amanitasubjunquilleavar.abla)中含有β鹅膏毒肽,其含量为614.00μg/g。其他5种鹅膏中均未检测到上述3种毒素。     

长白山鹅膏菌肽类毒素的HPLC分析

采用HPLC法对长白山地区分布的10种鹅膏菌中的α-鹅膏毒肽（α-amanitin)、β鹅膏毒肽（β-amanitin)和鬼笔毒肽（phalloidin)3种毒素的含量进行了测定。结果表明：白鹅膏（A.verna)和磷柄白鹅膏（A.virsa)中含有α-amanitin和β－amanitin两种毒素,二者β－amanitin的含量分别为1861．85μg/g和2477.02μg/g,均高于欧洲产毒鹅膏（A.phalloides)中的含量（1607μg/g）而接近灰花纹鹅膏Amanita fuliginea中的量（2633.80μg/g)。毒鹅膏A.phalloides中含有3种毒素,并且菌蕾中的含量高于成熟子实体,尤其菌蕾中Phalloidin的含量（1113.35μg/g)是灰花纹鹅膏成熟子实体中（432．5μg/g）的3倍。     

我国鹅膏菌新发现种——致命鹅膏(Amanita exitialis)的肽类毒素分析

采用高效液相色谱（HPLC）技术对在广州发现的鹅膏菌新种——致命鹅膏(Amanita exitialis)不同组织部位的肽类毒素(鹅膏毒肽和鬼笔毒肽)的含量进行了分析,结果表明,致命鹅膏是一种剧毒蘑菇,其毒素含量相当高,子实体中组织部位不同,毒素含量以及鹅膏毒肽和鬼笔毒肽在其中的分布也不一样,菌盖中的毒素含量最高,达8152.6μg/g干重,菌柄的毒素含量次之,为3742.3μg/g干重,菌托中的毒素含量最低,只有1142.5μg/g干重;在菌盖、菌柄和菌托中都以鹅膏毒肽为主,尤其以αamanitin的相对含量最高,但从菌盖至菌柄到菌托,鬼笔毒肽尤其是Phallacidin的相对含量依次增加。     

我国28种鹅膏菌主要肽类毒素的检测分析*

利用高效液相色谱(HPLC)技术对产于我国的28种鹅膏菌的主要肽类毒素(鹅膏毒肽和鬼笔毒肽)进行了检测分析,并和采于欧洲(德国)的毒鹅膏Amanita phalloides作对照,结果表明,3种东亚所特有的鹅膏菌(灰花纹鹅膏、致命鹅膏和黄盖鹅膏白色变种)和欧洲毒鹅膏所含毒素种类多、含量高,其子实体菌盖部位主要毒素总量分别达到12583.7μg/g、8152.6μg/g、1058.2μg/g、7456.2μg/g干重子实体,这4种鹅膏菌可称之为剧毒鹅膏菌。其它25种鹅膏菌中有10种检测出含有微量鹅膏毒肽,含量在19.5μg/g-151.2μg/g之间。在4种剧毒鹅膏菌中,子实体组织部位不同,毒素含量以及鹅膏毒肽和鬼笔毒肽在其中的分布也不一样,菌盖中的毒素含量最高,菌柄的毒素含量次之,菌托中的毒素含量最低;对于灰花纹鹅膏、致命鹅膏和黄盖鹅膏白色变种,无论在菌盖、菌柄和菌托中,鹅膏毒肽类毒素的含量都高于鬼笔毒肽类毒素,尤其以α-amanitin的相对含量最高;而在欧洲毒鹅膏中,菌盖、菌柄和菌托中都以鬼笔毒肽为主,尤其以phallacidin的相对含量最高,并且从菌盖至菌柄到菌托,鬼笔毒肽的相对含量依次增加。     

三种鹅膏菌培养条件及所产肽类毒素的比较研究

以外生菌根菌鹅膏菌属三个种Amanita muscaria,A.pseudoporphyria和A.fritillaria为研究材料,以生长速率为评价指标,对其最适生长温度、pH值、光照、培养基、C及N源的利用等基本培养条件及所产肽类毒素进行了比较研究。研究结果表明,三种菌株最适生长温度有差异,A.pseudoporphyria和A.fritillaria的最适温度为28℃,A.muscaria的最适温度为22℃;A.muscaria菌丝体生长的pH值范围为5-7,另外两个菌株的pH值范围为3-6;24h光照、12h光暗交替和24h黑暗对鹅膏菌的生长速率影响不大;SPDM培养基和MMN培养基都适合三种菌株的生长,但对于A.muscaria来说PDM培养基更适合其生长。鹅膏菌能够利用比较广泛的C、N源,但三个种在利用的C、N源种类上有一定的差别。通过抑芽法实验和HPLC分析分别表明三种鹅膏菌所含肽类毒素在种类和含量上有所不同,但都对绿豆发芽有一定的抑制作用。A.pseudoporphyria和A.fritillaria菌丝体中α-amanitin的含量分别为35.56μg/gDCW(drycellweight细胞干重)和26.02μg/gDCW,不含有phalloidin和β-amanitin;A.muscaria菌丝体中没有检测到α-amanitin、β-amanitin和phalloidin。结果表明供试的三种鹅膏菌在基本培养条件及所产肽类毒素方面存在种水平上的差异。     

我国28种鹅膏菌主要肽类毒素的检测分析

利用高效液相色谱(HPLC)技术对产于我国的28种鹅膏菌的主要肽类毒素(鹅膏毒肽和鬼笔毒肽)进行了检测分析,并和采于欧洲(德国)的毒鹅膏。Amanita phalloides作对照,结果表明,3种东亚所特有的鹅膏菌(灰花纹鹅膏、致命鹅膏和黄盖鹅膏白色变种)和欧洲毒鹅膏所含毒素种类多、含量高,其子实体菌盖部位主要毒素总量分别达到12583．7μg／g、8152．6μg／g、1058．2μg／g、7456．2μg／g干重子实体,这4种鹅膏菌可称之为剧毒鹅膏菌。其它25种鹅膏菌中有10种检测出含有微量鹅膏毒肽,含量在19．5μg／g—151．2μg/g之间。在4种剧毒鹅膏菌中,子实体组织部位不同,毒素含量以及鹅膏毒肽和鬼笔毒肽在其中的分布也不一样,菌盖中的毒素含量最高,菌柄的毒素含量次之,菌托中的毒素含量最低;对于灰花纹鹅膏、致命鹅膏和黄盖鹅膏白色变种,无论在菌盖、菌柄和菌托中,鹅膏毒肽类毒素的含量都高于鬼笔毒肽类毒素,尤其以α-amanitin的相对含量最高;而在欧洲毒鹅膏中,菌盖、菌柄和菌托中都以鬼笔毒肽为主,尤其以phallacidin的相对含量最高,并且从菌盖至菌柄到菌托,鬼笔毒肽的相对含量依次增加。     

云南楚雄致命鹅膏中环肽毒素的检测与分析

采用反相高效液相色谱法对采自云南楚雄双柏县的致命鹅膏在3个不同生长期中不同部位的6种环肽毒素含量进行了检测和分析。结果表明,致命鹅膏含有α-, β-鹅膏毒肽、羧基三羟鬼笔毒肽和羧基二羟鬼笔毒肽,未检出γ-鹅膏毒肽和二羟鬼笔毒肽。生长期毒素总量最高（9.3mg/g）、从成熟期（7.5mg/g）到衰老期（6.5mg/g）逐渐降低,但鬼笔毒肽的相对含量随着年龄增长而逐渐增加,鹅膏毒肽与鬼笔毒肽比值从生长期、成熟期到衰老期分别为2.6、1.4和0.9。在3个不同发育阶段中,4种毒素含量从菌盖、菌柄到菌托逐渐降低,而鬼笔毒肽的相对含量逐渐增加。α-鹅膏毒肽和β-鹅膏毒肽在生长期菌盖中含量最高,分别为7.4mg/g和3.1mg/g,而羧基三羟鬼笔毒肽和羧基二羟鬼笔毒肽在衰老期的菌盖中含量最高,分别为2.8mg/g和2.1mg/g。     

长白山鹅膏菌肽类毒素的HPLC分析

采用HPLC法对长白山地区分布的10种鹅膏菌中的-鹅膏毒肽(-amanitin)、鹅膏毒肽(-amanitin)和鬼笔毒肽(phalloidin)3种毒素的含量进行了测定。结果表明:白鹅膏(A.verna)和鳞柄白鹅膏(A.virsa)中含有-amanitin和-amanitin两种毒素,二者-amanitin的含量分别为 1861.85g/g和2477.02g/g,均高于欧洲产毒鹅膏(A.phalloides)中的含量(1607g/g)而接近灰花纹鹅膏Amanita fuliginea中的量(2633.80g/g)。毒鹅膏A.phalloides中含有3种毒素,并且菌蕾中的含量高于成熟子实体,尤其菌蕾中Phalloidin的含量(1113.35g/g)是灰花纹鹅膏成熟子实体中(432.5g/g)的3倍。     

长白山鹅膏菌肽类毒素的HPLC分析*

采用HPLC法对长白山地区分布的10种鹅膏菌中的-鹅膏毒肽(-amanitin)、鹅膏毒肽(-amanitin)和鬼笔毒肽(phalloidin)3种毒素的含量进行了测定。结果表明:白鹅膏(A.verna)和鳞柄白鹅膏(A.virsa)中含有-amanitin和-amanitin两种毒素,二者-amanitin的含量分别为 1861.85g/g和2477.02g/g,均高于欧洲产毒鹅膏(A.phalloides)中的含量(1607g/g)而接近灰花纹鹅膏Amanita fuliginea中的量(2633.80g/g)。毒鹅膏A.phalloides中含有3种毒素,并且菌蕾中的含量高于成熟子实体,尤其菌蕾中Phalloidin的含量(1113.35g/g)是灰花纹鹅膏成熟子实体中(432.5g/g)的3倍。     

Scale-up of a liquid static culture process for hyperproduction of ganoderic acid by the medicinal mushroom Ganoderma lucidum

Scale-up of a liquid static culture process was studied for hyperproduction of ganoderic acid (GA) by a famous Chinese traditional medicinal mushroom, Ganoderma lucidum. Initial volumetric oxygen transfer coefficient (K(L)a) and area of liquid surface per liquid volume (A(s)) were identified as key factors affecting cell growth and GA accumulation in liquid static cultures of G. lucidum, on the basis of which a multilayer static bioreactor was designed. At a low initial K(L)a level of 2.1 h(-1), a thick layer of white mycelia was formed on the liquid surface, and an optimal production of total GA (i.e., GA production in the liquid and on the liquid surface) was obtained. Both the formation of white mycelia and production of GA on the liquid surface were enhanced with an increase of A(s) within the range as investigated (0.24-1.53 cm(2)/mL). At an A(s) value of 0.90 cm(2)/mL, the total GA production reached maximum. A successful scale-up from a 20-mL static T-flask to a 7.5-L three-layer static bioreactor was achieved based on initial K(L)a. The maximum biomass (20.8 +/- 0.1 g DW/L), GA content (4.96 +/- 0.13 mg/100 mg DW), and total GA production (976 +/- 35 mg/L) were attained in static bioreactors. Not only GA content but also its production obtained in this work were the highest ever reported.     

蘑菇菌丝体代谢产物对果蝇的致死效应

以果蝇为靶标 ,对 15种蘑菇液体培养产物的毒性进行了检测 ,发现硫磺菌红色变种Laetiporussulphureusvar miniatus和硫磺菌原变种Laetiporussulphureusvar sulphureus液体培养中产生的代谢产物对果蝇具有致死活性。气升式生物反应器 (Airlift/ff)培养条件下 ,硫磺菌红色变种和原变种培养体系的 pH值均连续下降 ,最终都降至 2 2左右。研究发现致死活性产物被分泌到细胞外 ,离子交换树脂柱层析的线性洗脱分离结果表明活性代谢产物呈酸性 ,进一步分析表明草酸是活性代谢物之一 ,而树脂静止交换表明另外一种未知色素也具有致死活性     

假蜜环菌发酵工艺的优化研究

目前,国内普遍采用亮菌固体发酵工艺生产亮菌制剂。采用小型发酵罐液体深层发酵和液体静置发酵对亮菌发酵工艺进行优化研究。液体深层发酵采用28℃,200 r/min,通气量1∶1 v/v·m,培养7 d,亮菌干重为16.55g/L,其中菌丝体中多糖含量为5.42%,蛋白含量为1.75%;液体静置发酵采用500 mL三角瓶,28℃,150 r/min,摇瓶3 d后静置发酵14 d,亮菌干重可达10.69 g/L,发酵液中多糖含量为1.016 g/L,蛋白含量为0.320 g/L。对液体静置发酵进一步研究发现其发酵液中亮菌甲素含量可达3.118 mg/L。由此可见,两种发酵方式在保证生物量和活性成分的前提下,缩短了发酵周期,均优于传统的固体发酵工艺,值得工业生产借鉴。     

Production of Trichoderma micropropagules as a biocontrol agent in static liquid culture conditions by using an integrated bioreactor system

ABSTRACT

In this study, we optimised the conditions for the production of micropropagules of Trichoderma harzianum EGE-K38 in static liquid culture in Modified Czapec Medium (MCM) containing 8?g/L glucose in an integrated tray bioreactor system designed by our research group. Incubation temperature, air flow rate, inoculum spore concentration, inoculation size, medium volume and the use of spores or agar plugs containing mycelia as inoculum were individually studied as one factor at a time. The maximum micropropagule count was 5.2?±?0.2?×?10^9?cfu/mL and dry cell weight was 17?±?2?g/L. For the subsequent drying processes, the maximum drying yield percentage ((viable micropropagule counts after drying/viable cells before drying)*100) after drying of micropropagules was 23.30% (cfu/cfu). Results obtained from our integrated tray bioreactor system showed that static liquid culture fermentation offers potential for industrial scale fungal BCAs production.     

The effect of Zn on the Zn accumulation and biosynthesis of amino acids in mycelia of Cordyceps sinensis

Zinc is an essential trace element in the human body and it participates in various pathways of metabolism. Cordyceps sinensis is a wellknown traditional Chinese medicine that contains cordycepin, cordycepic polysaccharides, proteins, vitamins, trace elements, and many other biological active materials. In this study, we cultured C. sinensis in liquid medium containing Zn ions and then analyzed the biomass, the ratios of total Zn accumulation, and the organic Zn content in the mycelia. The results showed that when the media contain 150 mg/L Zn, the biomass of mycelia of C. sinensis reached 10.7 g/L and the Zn content present in the mycelia reached 4875.1 microg/g. The percentage of Zn accumulated in the mycelia was 34.05% of the total Zn in the media, of which the organic Zn accounted for 76.33%. The results also revealed that the content of total amino acid (TAA) and essential amino acid (EAA) in the mycelia were increased substantially TAA and EAA in the Zn-treated mycelia were 11.1% and 15.2% higher, respectively, than that in the mycelia without Zn treatment. These results will be useful for elucidation of the physiological mechanism of Zn effects on the biological metabolism in the mycelia of C. sinensis.     

From field sampling to pneumatic bioreactor mycelia production of the ectomycorrhizal mushroom Laccaria trichodermophora

In order to increase survival rates of greenhouse seedlings destined for restoration and conservation programs, successful mycorrhization of the seedlings is necessary. To reforest forest ecosystems, host trees must be inoculated with ectomycorrhizal fungi and, in order to guarantee a sufficient supply of ectomycorrhizal inoculum, it is necessary to develop technologies for the mass production of ectomycorrhizal fungi mycelia. We selected the ectomycorrhizal fungus Laccaria trichodermophora, due to its ecological traits and feasible mycelia production in asymbiotic conditions. Here, we report the field sampling of genetic resources, as well as the highly productive nutritional media and cultivation parameters in solid cultures. Furthermore, in order to achieve high mycelial production, we used strain screening and evaluated pH, carbon source concentration, and culture conditions of submerged cultures in normal and baffled shake flasks. The higher productivity culture conditions in shake flasks were selected for evaluation in a pneumatic bioreactor, using modified BAF media with a 10 g/L glucose, pH 5.5, 25 °C, and a volumetric oxygen transfer coefficient (K_La) of 36 h⁻¹. Under those conditions less biomass (12–37 %) was produced in the pneumatic bioreactor compared with the baffled shake flasks. This approach shows that L. trichodermophora can generate a large biomass concentration and constitute the biotechnological foundation of its mycelia mass production.     

灵芝菌诱变育种与深层培养的研究

采用紫外线对灵芝菌进行了诱变处理,选育到一株高产菌株ＵＶ－６０Ｓ,其菌体干重达１３．１ｇ／Ｌ,粗多糖含量为６４０ｍｇ／Ｌ,分别比原菌株提高了２１．３％和３０．６％;并研究了培养基组成和培养条件对菌体生长的影响,优化了深层培养的工艺条件,使菌体产量与胞外多糖含量比优化前分别提高了１５．３％和１８．８％。     

Studies on Cell Suspension Culture and Fermentation Culture in Arnebia euchroma

This paper reports some characteristics of cell suspension and fermentation culture in Arnebia euchroma (Royle) Johnst. The yield of suspension culture reached 22.0g dry wt/L per month when inoculum quantity was 2.50 g dry wt/L. Time-course study showed that cell growith lagged in 0–3 days and enhanced greatly in 3–12 days, and almost ceased after 12 days of culture, pH value changed during the culture period and peaked on the 12th day after inoculation. When cells were cultured in liquid production medium, the contents of shikonin derivatives increased quickly and reached to the maximum about the 25th day. The cell yield of 9.47 and 9.34 g dry wt/L per month was obtained in fermentation culture. Timecourse of cell growth in fermentation culture was similar to that in suspension culture. The total content of shikonin derivatives in fermentation culture was 14.26% dry weight from 10 L bioreactor. The yield of shikonin derivatives was 1.93 g/L.     

Artemisinin Production by Adventitious Shoots of Artemisia annua in a Novel Mist Bioreactor

A novel ultrasonic inner-loop bioreactor was used for artemisinin production by adventitious shoots in a multiplate culture of Artemisia annua L. The bioreactor was designed to allow the nutrient mist to uprise along a concentric draught-cylinder until it overflows from the top opening and the side-holes of the central tube downward and out of the annulus, so that the nutrient mist can be fulfilled in the bioreactor within 2 ~ 3 minutes. Under the misting cycles of every 3-minute misting in every 90 minute interval, artemisinin production reached totally 46.9 mg DW/L of culture medium at an airflow rate of 0.5 L/min for 25 d of culture in batches. The product amounted 2.9 and 3.2 folds of those obtained from culturing in solid medium and in shaking flasks respectively.