玫烟色拟青霉最适液体培养条件的研究

通过对不同营养和不同培养条件下玫烟色拟青霉菌丝生物量和产孢量的研究,结果表明:葡萄糖为玫烟色拟青霉液体培养的最适碳源,蛋白胨为该菌生长的最适氮源,C/N为10∶1~20∶1最适于玫烟色拟青霉菌丝生长和产孢;25℃2、4 h全光照条件,对该菌生长和产孢均有利。接种后144~168 h时,菌丝生物量和产孢量均达到高峰,分别为31.72 mg/mL、24.62孢子/mL,为黑暗条件下的1.5倍和18.3倍,因此玫烟色拟青霉液体发酵终点应选择在接种后144~168 h为最好。     

十种虫生真菌液体培养芽生孢子的形态发生

芽生孢子是许多真菌通过出芽方式产生的无性孢子,在液体发酵中主要以这种形式大量繁殖。真菌杀虫剂活性成分分生孢子的大量生产使用液体发酵得到的芽生孢子作为接种物,另外,它也是当今虫生真菌遗传转化的重要受体,因而研究虫生真菌芽生孢子的形态和发生特点具有重要意义。本研究分别对液体发酵中的球孢白僵菌、粉棒束孢、蝉棒束孢、环链棒束孢、玫烟色棒束孢、细脚棒束孢、斜链棒束孢、金龟子绿僵菌、蝗绿僵菌和蜡蚧霉等10种常见虫生真菌芽生孢子的形成过程进行显微观察,了解其分生孢子产生过程的异同。结果表明,芽生孢子的产生方式有两种类型：1）蝉棒束孢在其整个生活史中以菌丝生长为主,芽生孢子产生的数量很少。2）其他各种真菌芽生孢子产生方式相似,在菌丝体形成后就开始大量以菌丝出芽或缢缩产生芽生孢子,接着还可通过芽生孢子的出芽或缢缩断裂产生新的芽生孢子。芽生孢子的产生分为3个时期：初期先由菌丝形成芽生孢子;指数期芽生孢子大量增殖,菌丝和芽生孢子都可产生芽生孢子;后期以芽生孢子产新芽生孢子为主要方式。     

生防真菌分生孢子抗氧化能力与多糖含量的关系

作为重要的丝孢类昆虫病原真菌,球孢白僵菌和玫烟色棒束孢因其易于生产和环境友好等优点而在害虫生防防治中受到广泛青睐。为初步探求孢子耐氧化力及其与孢子多糖含量的关系,球孢白僵菌和玫烟色棒束孢11株菌经胁迫后的残存指数随氧化剂H2O2浓度增加而减小。所有菌株的残存指数均能良好地与Logistic方程拟合,并计算出各菌株在氧化胁迫条件下的半致死浓度。结果显示玫烟色棒束孢孢子的耐氧化力强于球孢白僵菌。两种真菌的分生孢子耐氧力与各自多糖含量呈现良好线性正相关。培养基碳源成分和浓度变化可影响球孢白僵菌孢子耐氧化力,但耐氧化力与多糖含量依旧呈现线性正相关。由此可见,生防真菌分生孢子的耐氧化力的确与多糖积累有关,并在一定程度上受培养条件的调节。研究结果有望为提高生防真菌孢子环境稳定性提供新的策略。     

哈茨木霉的培养及其对烟草疫霉生长的抑制研究*

哈茨木霉是一类重要的植病生防因子。哈茨木霉TH-1分别在PDA培养基、麦芽糖培养基、查氏培养基和琼脂培养基上培养均能产孢,其中PDA培养基为最适培养基。PDA培养基上,菌丝生长适宜温度27.5℃~35℃,最适温度32.5℃,产孢最适温度27.5℃。菌丝生长适宜pH值为3~7,产孢适宜pH值为5~9,生长与产孢最适pH值为5。光照对菌丝生长影响不大但明显影响菌株的产孢数量,光照时间越长产孢量越大。对峙培养试验表明TH-1明显抑制疫霉菌的生长速率,其无菌滤液明显抑制烟草疫霉菌游动孢子的萌发,并抑制游动孢子芽管     

虫生真菌玫烟色棒束孢Pf9606抗逆性的研究

采用凹玻片悬滴法测定了玫烟色棒束孢在高温、紫外照射、紫外保护剂和杀菌剂等逆境胁迫下分生孢子的存活率。结果表明:玫烟色棒束孢Pf9606分生孢子在36～45 ℃高温下连续处理24 h后,该菌孢子几乎不能存活;36～45 ℃短时高温处理后,随温度的升高和处理时间的延长,孢子存活率明显降低;随紫外照射时间的延长,玫烟色棒束孢孢子存活率明显降低,当紫外照射50 s时,孢子存活率为55.33%,当照射时间延长为180 s时,孢子不能存活;不同浓度的抗坏血酸和高浓度的荧光素钠可提高玫烟色棒束孢抗紫外照射能力,抗坏血酸的理想浓度为0.2 mg/mL,荧光素钠的理想浓度为0.9 mg/mL,而不同浓度的刚果红和氧化锌对玫烟色棒束孢没有保护作用;玫烟色棒束孢与杀菌剂72%农用硫酸链霉素、70%代森联和58%甲霜灵锰锌混用后,对该菌孢子存活影响较小,不同浓度下孢子存活率均达85%以上,而常规浓度的氟吗·锰锌对玫烟色棒束孢孢子存活有较强的抑制作用。     

紫外线照射对玫烟色拟青霉产孢子能力的影响

目的:探讨紫外线照射对玫烟色拟青霉产孢子能力的影响.方法:利用20W紫外 灯对玫烟色拟青霉的原生质体悬浮液进行了不同照射时间、对孢子悬浮液进行了不同照射距 离和时间组合的紫外线照射处理.结果:紫外灯下30cm照射原生质体90 s及紫外灯下20cm照射孢子20min两个处理中,菌落直径最大菌株的菌丝生长速度显著高于出 发菌株,产孢量也分别是出发菌株的1.4及1.6倍.结论:适宜的紫外线照射处理可以提高玫烟色拟青霉的产孢子能力.     

玫烟色棒束孢侵染小菜蛾的透射电镜观察

利用透射电镜观察了玫烟色棒束孢Isaria fumosorosea(=Paecilomyces fumosoroseus)对小菜蛾Plutella xylostella(L.)的侵染过程及菌体在虫体内的增殖方式。以浓度为1×107孢子/mL的孢子悬浮液接种小菜蛾4龄幼虫,在透射电镜下对虫体各部位的观察结果表明:接种后1h玫烟色棒束孢菌株EBCL03011的分生孢子开始萌芽,至4h可观察到附着孢的形成和穿透,接种后24h已普遍侵入体腔。玫烟色棒束孢在寄主表皮和体腔内,以菌丝段出芽生殖、菌丝分隔及菌丝段分隔3种方式大量增殖,主要以颗粒状的菌丝段在寄主体腔内扩散,菌丝段在穿透表皮和体腔内增殖过程中伴随着机械压力和酶的活动。     

两种表面活性剂对玫烟色棒束孢PF904菌株侵染小菜蛾幼虫的影响

【目的】在前期筛选试验的基础上,比较表面活性剂对玫烟色棒束孢Isaria fumosoroseus PF904菌株侵染小菜蛾Plutella xylostella 3龄幼虫的增效作用,获得可提高玫烟色棒束孢PF904防治效果的助剂。【方法】通过扫描电镜观察和室内致病力试验,测定喷施分别添加表面活性剂聚二甲基硅氧烷(OFX-0193)（终浓度125 mg/L）和二异丁基萘磺酸钠(Nekal)(终浓度250 mg/L）的玫烟色棒束孢PF904孢子悬浮液后玫烟色棒束孢PF904在小菜蛾3龄幼虫体表的孢子附着量及对小菜蛾3龄幼虫的侵染速率和致病力。【结果】添加250 mg/L Nekal和125 mg/L OFX-0193可显著提高玫烟色棒束孢PF904孢子悬浮液在小菜蛾3龄幼虫体表各结构区的孢子附着量,其中添加250 mg/L Nekal的玫烟色棒束孢PF904孢子悬浮液在小菜蛾3龄幼虫体表刺状突起结构区、平缓结构区和嵴状突起结构区的孢子附着量分别为对照(添加清水的孢子悬浮液)的2.19, 1.78和1.94倍,说明Nekal提高了玫烟色棒束孢PF904的孢子附着率;添加250 mg/L Nekal和125 mg/L OFX-0193均显著缩短了玫烟色棒束孢PF904孢子萌发时间,促进附着孢的形成,提高了玫烟色棒束孢PF904的侵染速率。室内致病力测定结果表明,玫烟色棒束孢PF904孢子悬浮液中添加250 mg/L Nekal和125 mg/L OFX-0193可显著提高玫烟色棒束孢PF904孢子悬浮液对小菜蛾3龄幼虫的致病力,其中添加250 mg/L Nekal的玫烟色棒束孢PF904孢子悬浮液对小菜蛾3龄幼虫的校正死亡率达79.2%,致死中时(LT₅₀)降低为2.71 d,说明Nekal的增效作用显著。【结论】250 mg/L Nekal为玫烟色棒束孢PF904的适宜的助剂和添加浓度,可显著提高其对小菜蛾幼虫的防治效果。     

耐低水活度高毒力虫生真菌菌株选育

以球孢白僵菌Beauveria bassiana和玫烟色拟青霉Paecilomyces fumosoroseus为研究对象,利用紫外线诱变芽生孢子和低水活度条件胁迫筛选,选育出突变株Bb07240、Pf01120和Pf01160,它们在低水活度（或相对湿度）下的生长和萌发均明显优于其相应的初始菌株。生物测定表明,突变株对桃蚜的毒力明显高于其初始菌株。     

温湿度对玫烟色棒束孢IF‐1106菌株孢子萌发及对烟粉虱致病力的影响(英文)

B型烟粉虱Bemisia tabaci Gennadius是一种重要的世界性农业害虫。玫烟色棒束孢Isaria fumosorosea是防治烟粉虱的一种重要的虫生真菌。对不同温度(20、23、26、29、32℃)、不同湿度(53%、65%、75%、85%、95%)下玫烟色棒束孢IF‐1106菌株分生孢子萌发及其对烟粉虱的致病力进行了测定。结果表明:温度对孢子的萌发有显著影响,26℃时孢子萌发率最高。当相对湿度低于75%时,孢子不萌发或萌发率较低;当相对湿度为85%–95%时,孢子萌发率显著升高。26℃时,烟粉虱2龄若虫的累计死亡率最高。随着相对湿度增大,病菌的致病力增强。当相对湿度为53%–95%时,烟粉虱2龄若虫累计死亡率从54.55%增加到88.89%。玫烟色棒束孢的致病力与孢子萌发率呈正相关,但温度比相对湿度对其影响更明显。结果表明,玫烟色棒束孢IF‐1106菌株侵染烟粉虱的最佳条件是温度26℃和相对湿度大于85%。     

Effect of Additives on the Production, Viability and Virulence of Blastospores of Metarhizium anisopliae

Studies on the blastospore production of Metarhizium anisopliae var. anisopliae were conducted in Adamek's medium used as a standard, enriched with lecithin, collagen, lactic acid or polyethylene glycol 200 (PEG 200) to increase spore yield and suppress mycelial pellet formation. The addition of 5% lecithin resulted in a significant 10-fold increase in spore yield up to 1.9 108 blastospores/ml compared with 1.9 107 spores/ml in the standard medium. Collagen (3%) increased the number of blastospores 3.7-fold, and lactic acid (1.5%) two-fold. A reduction of mycelial pellet formation in favour of spore production was noted with each additive. The viability of blastospores at 40IC from media with lecithin, collagen and lactic acid suspended in 25% Ringer's solution was comparable to that of spores produced in the standard medium. Striking differences were noticed in the viability of spores produced with 5% PEG 200 in standard medium. The half-life of blastospores produced in standard medium suspended in sunflower oil was 33.6 h and that of 5% PEG 200 spores only 25.2 h. In bioassays, the virulence of spores produced in standard medium to which 3% lecithin, 3% collagen, 1.5% lactic acid or 5% PEG 200 had been added was tested against third-instar nymphs of Locusta migratoria migratorioides (R. & F.). The median lethal time and the mortality of L. migratoria achieved with blastospores produced with 3% lecithin (5.7 days, 99%) was comparable to that of blastospores from standard medium (5.1 days, 98%). The virulence of blastospores from all other media with additives was significantly reduced.     

Influence of culture conditions on production and freeze-drying tolerance of Paecilomyces fumosoroseus blastospores

With the goal of developing a defined medium for the production of desiccation-tolerant blastospores of the bioinsecticidal fungus Paecilomyces fumosoroseus, we evaluated the impact of various media components such as amino acids, carbohydrates, trace metals and vitamins on hyphal growth and sporulation of P. fumosoroseus cultures and on the freeze-drying tolerance of blastospores produced under these conditions. A comparison of 13 amino acids as sole nitrogen sources showed that glutamate, aspartate, glycine and arginine supported biomass accumulations (12–16 mg ml⁻¹) and blastospore yields (6–11 × 10⁸ blastospores ml⁻¹) comparable to our standard production medium which contains casamino acids as the nitrogen source. Using glutamate as the sole nitrogen source, tests with various carbohydrates showed that P. fumosoroseus grew best on glucose (18.8 mg biomass ml⁻¹) but produced similar blastospore concentrations (7.3–11.0 × 10⁸) when grown with glucose, glycerol, fructose or sucrose. P. fumosoroseus cultures grown in media with sodium citrate or galactose as the sole carbohydrate produced lower blastospore concentrations but more-desiccation-tolerant spores. Zinc was the only trace metal tested that was required for optimal growth and sporulation. In a defined medium with glutamate as the nitrogen source, vitamins were unnecessary for P. fumosoroseus growth or sporulation. When blastospores were freeze-dried in the absence of a suspension medium, residual glucose (>2.5% w/v) was required for enhanced spore survival. Thus, a defined medium containing basal salts, glucose, glutamate and zinc can be used to produce optimal concentrations of desiccation-tolerant blastospores of P. fumosoroseus. Received 27 October 1998/ Accepted in revised form 06 May 1999     

Influence of formulation additives on the desiccation tolerance and storage stability of blastospores of the entomopathogenic fungus Paecilomyces fumosoroseus (Deuteromycotina: Hyphomycetes)

Blastospores of the entomopathogenic fungus Paecilomyces fumosoroseus were formulated with 10% lactose/1% bovine serum albumin (BSA) or various compositions of Fantesk™, a starch-oil composite prepared by jet-cooking an aqueous dispersion of starch and oil. Storage stability studies with wet blastospore formulations showed that maximum blastospore survival was achieved during low-temperature storage at -20°C with lactose/BSA formulations or starch-oil formulations supplemented with sucrose, zein protein, and whole milk. Under conditions of wet storage at -20°C, the addition of whole milk to starch-oil formulations significantly improved blastospore stability while the addition of sucrose or zein protein had no effect. In freeze-drying studies, no significant differences were seen in blastospore desiccation tolerance or in stability during storage at either 4 or -20°C when blastospores of P. fumosoroseus were formulated with lactose/BSA or starch-oil formulations with sucrose, zein protein, and whole milk. Freeze-dried blastospore formulations stored at 4°C showed no loss in blastospore viability after 3 months storage and blastospore formulations stored at -20°C showed no loss in viability during the entire 12-month study. For freeze-dried, starch-oil formulations, sucrose was shown to improve blastospore survival during the freeze-drying process. The addition of whole milk to starch-oil formulations significantly improved the stability of freeze-dried blastospores stored at 4°C. Compared to unformulated blastospore suspensions that showed blastospore settling after 30 min, suspensions of blastospores formulated with lactose/BSA or starch-oil composites remained stable for up to 2 h after mixing.     

Characterisation of optimum cultural environmental conditions for the production of high numbers of Metarhizium anisopliae blastospores with enhanced ecological fitness

The aim of this study was the production of high numbers of M. anisopliae blastospores with enhanced germination efficiency under conditions of water-stress (ecological fitness). Different nitrogen sources and concentrations were screened for their ability to induce blastospore production while keeping pH and water activity (a_w) at fixed levels (6.8, and 0.98 a_w, respectively). After optimum nitrogen status was determined (cornsteep solid (CS) + yeast extract (YE); or cottonseed flour (CF) + YE), the effect of interaction of nitrogen source, pH (3.5, 5, 6.8, 8, 9 and 10) and solutes for a_w adjustment (KCl, NaCl, PEG 200) on blastospore production, endogenous polyol content (glycerol, erythritol, arabitol and mannitol) and total protein, were determined. For both ionic (NaCl, KCl) and non-ionic solutes (PEG 200), optimum blastospore production (between 4×10⁷ and 2×10⁸ blastospores ml^-1) and growth occurred in the pH range 6.8-8, with the CF + YE nitrogen profile giving higher yields than CS + YE. Optimum conditions for high erythritol and total protein endogenous concentrations (40.37-73.44 and 14.33-18.90 mg g^-1 fresh weight, respectively) occurred between pH 6.8 and 8 by ionic a_w modification (KCl, NaCl) and with the CF + YE nitrogen profile. Germination of blastospores produced under these cultural conditions was between 62 and 89% under conditions of water-stress (0.96 a_w). On the other hand, blastospores with lower amounts of erythritol and total protein content had decreased germination (8-67%). These results could have significant implications for developing a liquid fermentation medium for the production of high numbers of fungal propagules with enhanced efficacy under non-optimum environmental conditions.     

高雄山虫草生物学特性及人工驯化条件优化

高雄山虫草Cordyceps tenuipes是一种重要的珍稀野生虫草,无性型为细脚棒束孢Isaria tenuipes。对采集的野生无性型高雄山虫草生物学特性进行了研究,采用小麦和大米为栽培基质,通过添加不同营养成分进行人工驯化和栽培条件优化,对后续提高其孢梗束产量和商业化栽培具有重要意义。试验结果表明,该虫草菌丝在固体和液体培养条件下生长所需的最佳营养组成一致,通过单因素和多因素正交试验得出菌丝在固体和液体条件下生长的最佳培养基配方为蔗糖30g/L、酵母粉15g/L、磷酸二氢钾2g/L、七水硫酸镁2g/L,最佳培养条件为温度25℃,pH 7。以小麦为培养基栽培的孢梗束生物学效率介于(45.750±6.062)%-(67.820±6.018)%,总体优于大米培养基(23.410±5.242)%-(36.880±8.812)%。以添加蚕蛹粉的小麦培养基栽培的孢梗束生物转化率最高,达67.820%,高于已有的报道。通过生物学特性分析和人工驯化条件的优化,为高雄山虫草的规模化人工栽培提供参考。     

Liquid-culture production of blastospores of the bioinsecticidal fungus<Emphasis Type="Italic"> Paecilomyces fumosoroseus</Emphasis> using portable fermentation equipment

The production of fungal spores using on-site, non-sterile, portable fermentation equipment is technically constrained. Very little information is available on the production requirements, such as medium concentration, inoculum stabilization, required fermentation times, and maintenance of axenic growth. In this study, we developed a two-part, liquid concentrate of the production medium that remains stable and soluble at room temperature. We also examined inoculum stability and showed that freeze- or air-dried blastospore preparations were stable for 7 days after rehydration when stored at 4 °C. The use of a low-pH (pH 4), relatively rich complex medium provided a growth environment deleterious to bacterial growth yet conducive to rapid sporulation by Paecilomyces fumosoroseus. High concentrations of blastospores (7.9×10⁸/ml) of P. fumosoroseus were produced in a 40-h fermentation with very low levels of bacterial contamination when the fermentor was charged with a blastospore production medium with a starting pH of 4 and inoculated with blastospore concentrations greater than 1×10⁶ spores/ml. These studies demonstrate that the use of disinfected, portable fermentation equipment has potential for on-site production of high concentrations of blastospores of the bioinsecticidal fungus P. fumosoroseus.     

Media and Fermentation Processes for the Rapid Production of High Concentrations of Stable Blastospores of the Bioinsecticidal Fungus Paecilomyces fumosoroseus

In shake flask and fermentor studies, various media components and culture inocula were tested to improve P. fumosoroseus spore production rates, yield and stability. To evaluate inoculum potential and inoculum scale-up for fermentor studies, conidia and liquid culture-produced spores of various strains of P. fumosoroseus were compared as inoculum. Inoculation of liquid cultures with blastospores at concentrations of at least 1×10⁶ spores mL^-1 resulted in the rapid production of high concentrations of blastospores (∼1×10⁹ spores mL^-1, 48 h fermentation time) for all strains tested. The rapid germination rate of blastospores (90% after 6 h incubation) compared to conidia (>90% after 16 h incubation) and the use of higher inoculum rates reduced the fermentation time from 96 to 48 h for maximal spore yields. A comparison of various complex nitrogen sources showed that liquid media supplemented with acid hydrolyzed casein or yeast extract supported the production of high concentrations of blastospores that were significantly more desiccation-tolerant (79-82% survival after drying) when compared to blastospores produced in media supplemented with other nitrogen sources (12-50% survival after drying). For rapid spore production, requirements for trace metals and vitamin supplementation were dependent on the type of hydrolyzed casein used in the medium. Fermentor studies with two strains of P. fumosoroseus showed that high concentrations (1.3-1.8×10⁹ spores mL^-1) of desiccation-tolerant blastospores could be produced in 48-h fermentations. These studies have demonstrated that the infective spores of various strains of the fungal bioinsecticide Paecilomyces fumosoroseus can be rapidly produced using deep-tank, liquid culture fermentation techniques.     

Phenotypic features of trehalase mutants in Saccharomyces cerevisiae

In the yeast Saccharomyces cerevisiae, some studies have shown that trehalose and its hydrolysis may play an important physiological role during the life cycle of the cell. Recently, other studies demonstrated a close correlation between trehalose levels and tolerance to heat stress, suggesting that trehalose may be a protectant which contributes to thermotolerance. We had reported lack of correlation between trehalose accumulation and increase in thermotolerance under certain conditions, suggesting that trehalose may not mediate thermotolerance [Nwaka, S., et al. (1994) FEBS Lett. 344, 225–228]. Using mutants of the trehalase genes, NTH1 and YBR0106, we have demonstrated the necessity of these genes in recovery of yeast cells after heat shock, suggesting a role of these genes in thermotolerance (Nwaka, S., Kopp, M., and Holzer, H., submitted for publication). In the present paper, we have analysed the expression of the trehalase genes under heat stress conditions and present genetic evidence for the ‘poor-heat-shock-recovery’ phenotype associated with NTH1 and YBR0106 mutants. Furthermore, we show a growth defect of neutral and acid trehalase-deficient mutants during transition from glucose to glycerol, which is probably related to the ‘poor-heat-shock-recovery’ phenomenon.     

地衣芽孢杆菌BF-002高产芽孢的氮源流加工艺研究*

目的: 提高地衣芽孢杆菌BF-002的芽孢产量,实现氮源流加过程的自动化控制,降低生产成本,为其他芽孢杆菌提高芽孢产率的研究提供一种思路。方法: 通过摇瓶做单因素实验,筛选最佳温度和碳氮源,在此基础上进行5 L发酵罐实验。初始添加不同浓度的氮源,探索芽孢形成与氮源的关系。提出相对氨基氮的概念,通过恒速补料、间歇补料和基于尾气CO₂浓度反馈流加三个策略控制相对氨基氮浓度水平。采用Python语言编写计算机控制程序,实现基于尾气CO₂浓度反馈流加策略的自动化控制。结果: 摇瓶筛选最佳温度及碳氮源分别为:37℃、葡萄糖、鱼粉蛋白胨、豆粕。上罐结果表明,相对氨基氮浓度越低芽孢率越高,采用基于尾气CO₂浓度反馈流加能将相对氨基氮控制在8.42 mg/OD₆₀₀水平,芽孢量可达4.25×10⁹ cfu/mL。利用计算机程序自动控制低价氮源氯化铵的流加,可以使芽孢量达到1.87×10¹⁰ cfu/mL,是前期最优批次的4.4倍,同时降低原料成本。结论: 将相对氨基氮浓度控制在适宜水平可以得到芽孢量较高的培养液,自动流加氯化铵策略能降低生产成本并实现自动化控制,为研究芽孢杆菌产孢提供一种思路。     

古尼虫草胞内多糖高产培养基优化研究

以古尼虫草Cordyceps gunnii胞内多糖产量为目标,利用单因素法筛选古尼虫草产胞内多糖的最适碳源、氮源和无机盐,运用正交试验筛选最佳培养基组合,用最佳培养基研究古尼虫草产胞内多糖的发酵动力学。结果表明：古尼虫草产胞内多糖最佳培养基为葡萄糖35g/L、蛋白胨15g/L、硫酸锌1g/L、KH₂PO₄ 1g/L、K₂HPO₄ 0.5g/L,用最佳培养基获得胞内多糖（5.169±0.274）g/L,产量是优化前的1.81倍;动力学研究表明,144h是古尼虫草胞内多糖最佳培养时间,此时产量最高为（6.794±0.221）g/L,是目前报道古尼虫草胞内多糖的最高产量。