油菜菌核病菌对速克灵的抗药性风险研究

在室内条件下通过菌丝生长速率法测定了分离自安徽省10个县市的油菜菌核病菌（Sclerotinia scleroti-orum）对速克灵的敏感性。结果表明,速克灵对各供试菌株的EC50值分布范围为0.0899-0.4966μg/mL,平均为0.2541μg/mL,且供试菌株在含速克灵质量浓度为10 000μg/mL的PDA平板上菌丝生长几乎完全被抑制。表明各供试菌株对速克灵十分敏感,但其敏感程度地区间存在较大差异。通过室内药剂直接诱变法,获得了抗速克灵突变株。抗性突变株抗性测定结果表明,某些地区的抗性菌株抗性消失,有些地区的抗性菌株抗性继续保持。结果显示安徽省油菜菌核病菌对速克灵具有潜在的抗药性风险。     

拮抗木霉耐多菌灵菌株的筛选

该文进行了耐多菌灵生防木霉菌株的筛选和生防效果的测定研究。为获得对灰葡萄孢霉等病原菌有显著拮抗能力的耐多菌灵木霉菌株,通过含药平板诱导和紫外线诱变,获得5株耐药性菌株,在多菌灵2.0g/L浓度下生长较好,Ec50值提高了40多倍;抗性菌株在含药培养基上连续继代转移培养10次,抗性程度未见下降;经过平板对峙和活体拮抗性测定,确定T42-2为最佳拮抗性耐多菌灵菌株,其对黄瓜灰霉病的防效达92.13%,并且对多菌灵、速克灵和三唑铜存在交互抗性。     

毒死蜱降解木霉菌对几种重要植物病原真菌的生防活性

木霉菌既是广泛应用的防治植物病害的生防菌,又是一类很有应用潜力的环境污染修复菌。针对分离筛选出的6株高效降解毒死蜱的木霉菌株,进行了土传植物真菌病害的生防活性试验。结果表明,在对峙培养条件下,供试木霉菌株对几种病原真菌均具有较为显著的抑制率,发酵滤液对多数病原真菌具有明显的抑菌作用。所有供试木霉菌株能在立枯丝核菌、灰霉、终极腐霉菌落上着生,并逐渐覆盖全部菌落;但不能在茄腐镰孢菌、尖孢镰孢菌、大丽轮枝菌上生长。真菌重寄生现象观察结果表明,供试木霉菌仅对立枯丝核菌具有明显的重寄生现象。研究结果表明,筛选出的高效降解毒死蜱的木霉菌菌株可对多种土传植物病原真菌具有良好的生防潜力。     

我国农作物根际土壤木霉菌资源分布调查

通过对我国18个省市地区的农作物根际土壤进行采样,使用木霉菌选择性培养基(TSM)和马铃薯葡萄糖培养基(PDA),对采样土壤中的木霉菌(Trichoderma spp.)进行分离和纯化,再与同一地区的多种植物病原菌进行平板对峙测试,筛选和保存了1 300余株有拮抗功能的木霉菌株。经形态学和分子生物学(ITSTef1-α)鉴定,这些菌株分属9个木霉菌种。其中哈茨木霉(T.harzianum)和棘孢木霉(T.asperellum)为优势菌种,分别占29.07%和29.91%(总数:393和382株);其次是绿色木霉(T.viride),占筛选总数的14%(总数:185株);而渐绿木霉(T.viridescens)和康宁木霉(T.koningii)分别占7.53%和7.00%(总数:99和92株);深绿木霉(T.atroviride)和钩状木霉(T.harmatum)分别只占5%以上(总数:69和67株);长枝木霉(T.longibrachiatum)和橘绿木霉(T.citrinoviride)的群落在我国农作物根际土壤中的分布最少,分别只占1.5%和0.5%以上(总数:21和7株)。同时,为了解不同地区的木霉菌株对上海地区的草莓灰霉菌(Botrytis cinerea)的拮抗作用的差异性,选用14个不同地区的木霉菌株,通过对峙培养拮抗测定,筛选出6个木霉菌株,进一步做了抑制草莓灰霉病的室内生测试验。结果显示,来源于华东地区的木霉菌株TR78和TR85,在平板对峙试验中对草莓灰霉菌生长的抑菌率分别为85.49%和82.90%,室内生测对灰霉病的防治效果分别为80.19%和80.02%,显著高于(P0.05)其他菌株对灰霉病的防治效果。     

T2-2菌株对多菌灵的降解特性及生物修复试验

摘要：【目的】为获得降解多菌灵的微生物菌株,并用其制备生物修复剂,修复被污染的土壤。【方法】从耐药性木霉菌株诱变选育过程中,得到一株能降解多菌灵的变异菌株T2-2。该菌株在多菌灵浓度100 mg/L无机盐培养基中, 于25℃、200 r/min振荡培养取样,用HPLC-MS检测代谢产物;以玉米秸秆粉为原料经固体发酵制成T2-2生物修复剂;采用土壤人工接种,在T2-2菌剂接种量为107cfu/g干土、多菌灵含量为0.1 mg/g干土时进行灭菌土和自然土壤的修复试验;另外,还做了T2-2菌剂对黄瓜枯萎病的活体防效试验。【结果】处理2 d的培养液,HPLC-MS检测出代谢产物为：2-氨基苯并咪唑,苯并咪唑和2-氨基苯腈,处理5 d的培养液经检测未发现多菌灵和代谢产物;土壤修复试验中,灭菌土壤中的多菌灵接种6 d被完全降解,而自然土壤中的多菌灵被完全降解缩短到4 d。说明秸秆粉作为共代谢底物,促进了T2-2和土著微生物的共代谢降解作用;另外,T2-2菌剂对黄瓜枯萎病的活体防治效果达到81.7%,优于化学农药。【结论】木霉T2-2菌株即可降解土壤中的多菌灵,又可防治植物病害。     

基因组重排技术选育乙醇高产菌株

里氏木霉（Trichoderma reesei）被认为是最合适联合生物加工（consolidated bioprocessing）的微生物之一。原始里氏木霉菌株产乙醇能力太低,需要进一步提高其产酒量。我们通过基因组重排技术提高了里氏木霉菌株产乙醇能力和乙醇耐受力。首先对CICC40360菌株孢子进行NTG诱变得到正向突变菌株,再以此为出发菌株进行基因组重排。进行基因组重排后,重组菌株在含不同乙醇浓度的原生质体再生培养基上进行筛选。突变菌株和原始菌株一起做摇瓶发酵实验进行比较以确定产乙醇能力的提高。经过两轮基因组重排后,筛选获得表现最优异的重组菌S2-254。该菌株能在利用50g/l葡萄糖发酵出6.2g/l乙醇,同时能耐受3.5% （v/v）浓度乙醇。上述结果表明,本实验采用的基因组重排技术能够有效而且快速获得具有目的性状的优良菌株。     

抗油桐枯萎病木霉菌的分离鉴定及抑菌作用研究

油桐是我国重要的木本油料植物,其生产的桐油作为天然的优良干性油在工业上具有广泛用途。但由油桐专化型尖孢镰孢菌Fusarium oxysporum f. sp. fordiis（Fof-1）侵染引起的枯萎病给油桐产业造成了毁灭性灾害,目前尚无有效防治手段。众多实践证明,利用生防菌可以有效防治土传枯萎病。本研究发现,在抗病油桐根围土壤中木霉菌的相对丰度较高,并从中分离获得了16株木霉菌;通过形态学鉴定和ITS-TEF1双基因联合构建系统进化树,鉴定出4种木霉菌：拟康宁木霉Trichoderma koningiopsis（TkonT1）、螺旋木霉T. spirale（TspiT2）、深绿木霉T. atroviride（TatrT3）和哈茨木霉T. harzianum（TharT4）;通过对峙培养试验,发现木霉菌株TkonT1、TharT4和TspiT2具有较好的抑菌效果;进一步显微观察发现菌株TkonT1和TatrT3可缠绕在尖孢镰孢菌菌丝体上或穿入菌丝体内营寄生生长,吸收病菌菌丝体养分进而导致病菌菌丝体破裂和细胞原生质消解。结果表明,从抗病油桐根围土壤中获得的拮抗木霉菌株可用于油桐枯萎病的生物防治。     

工厂化生产海鲜菇菌包污染霉菌的鉴定及防治

对工厂化生产中海鲜菇菌包污染霉菌进行分离,根据霉菌的形态特征、培养性状及ITS序列分析,鉴定其为哈茨木霉、拟康氏木霉、脉孢霉、长枝木霉、黑曲霉、产红青霉和产黄青霉;在此基础上探讨了常用抑菌剂对霉菌的防治效果及对海鲜菇菌丝生长的影响。结果表明,质量浓度100 mg/L克霉灵对哈茨木霉、黑曲霉、产红青霉、产黄青霉、拟康氏木霉有强抑制作用,质量浓度100 mg/L多菌灵对长枝木霉、产红青霉、产黄青霉、拟康氏木霉有强抑制作用,二者对海鲜菇菌丝生长的抑制都比较弱。可为海鲜菇工厂化生产中污染霉菌的综合防治提供参考。     

柱晶白霉素产生菌的选育：耐磷高产突变株的分离

柱晶白霉素产生菌──北里链霉菌（Ｓｔｒｅｐｏｍｙｃｅｓ．Ｋｉｔａｓａｔｏｎｅｓｉｓ）,通过紫外线处理和高浓度磷酸盐平板上选择分离到突变株ＵＤＰ１－２,在正常发酵培养基条件下摇瓶发酵柱晶白霉素超产可达１８．６％。而且变株的菌落形态与亲本菌株差异较大。     

新疆野果林木霉分离鉴定、抑菌作用及固态发酵配方优化

【背景】新疆野苹果病害发生严重,而木霉(Trichoderma spp.)是重要的植物病害生防菌,因此可利用其对新疆野苹果病害进行防治。【目的】分离鉴定新疆野果林木霉菌株,分析其对新疆野苹果2种病原菌的抑菌能力,为新疆野苹果专用木霉菌肥的制备提供菌种资源。【方法】利用平板稀释法对新疆野果林4种草本植物根围木霉菌进行分离,通过形态学与分子生物学方法进行菌种鉴定,平板对峙试验检测其抑菌能力并优化木霉菌株的固态发酵配方。【结果】共分离得到2种木霉菌共42株,分别为34株棘孢木霉(T. asperellum)和8株深绿木霉(T. atroviride);棘孢木霉TasT01对苹果炭疽病菌(Colletotrichum gloeosporioides,Cgl)和苹果斑点落叶病病原菌(Alternaria alternariaf.sp.mali,Aal)的抑菌率分别为58.60%和57.14%;深绿木霉TatT35对Cgl和Aal的抑菌率分别为43.86%和36.90%。进一步显微镜观察发现,TasT01可通过菌丝缠绕的方式抑制2种病原菌的生长。TatT35菌株固态发酵配方为稻壳90%、麦麸10%...     

Isolation and characterization of solvent-tolerant Pseudomonas putida strain T-57, and its application to biotransformation of toluene to cresol in a two-phase (organic-aqueous) system

Pseudomonas putida T-57 was isolated from an activated sludge sample after enrichment on mineral salts basal medium with toluene as a sole source of carbon. P. putida T-57 utilizes n-butanol, toluene, styrene, m-xylene, ethylbenzene, n-hexane, and propylbenzene as growth substrates. The strain was able to grow on toluene when liquid toluene was added to mineral salts basal medium at 10-90% (v/v), and was tolerant to organic solvents whose log P(ow) (1-octanol/water partition coefficient) was higher than 2.5. Enzymatic and genetic analysis revealed that P. putida T-57 used the toluene dioxygenase pathway to catabolize toluene. A cis-toluene dihydrodiol dehydrogenase gene (todD) mutant of T-57 was constructed using a gene replacement technique. The todD mutant accumulated o-cresol (maximum 1.7 g/L in the aqueous phase) when cultivated in minimal salts basal medium supplemented with 3% (v/v) toluene and 7% (v/v) 1-octanol. Thus, T-57 is thought to be a good candidate host strain for bioconversion of hydrophobic substrates in two-phase (organic-aqueous) systems.     

Isolation and characteristics of methanosaeta in paddy field soils

The population of filamentous acetate-utilizing methanogens in paddy field soils was 2.0 x 10(4) MPN/g dry soil in the submerged condition. They were able to form colonies in a deep agar medium, but not in a roll tube. Filamentous acetate-utilizing methanogens isolated from Kanagi, Japan (strain K-5) and Tsukuba, Japan (strain T-3) were divided into two types based on length of filaments. One type, strain K-5, formed a short chain which was dispersed easily by weak shaking. The other type, strain T-3, formed a long chain, which formed cotton-like flocs and was not dispersed by weak shaking. They had sheaths composed of a pair of adjacent membranes on the outside of the cell membranes. The 16S rRNA gene similarities of strain T-3 and K-5 to Methanosaeta concilii strain Opfikon were 100% and 99.5% respectively. Filamentous acetate-utilizing methanogens were also isolated from paddy field soils in various other regions of Japan. Our results suggest that Methanosaeta is universal in paddy soils and that it plays an important role in methane production from acetate.     

一株球孢白僵菌转基因工程菌在继代培养中的变异

基因工程是解决昆虫病原真菌致死慢、致死率低的有效途径,但在传代培养过程中,被转入的基因是否会丢失以及转基因工程株是否会像野生型菌株那样频繁地发生变异,引起产孢减少和毒力减退等生产性状的退化？针对这些问题,研究一株球孢白僵菌Beauveria bassiana转外源蝎毒基因工程菌株在继代培养过程中的的变异现象,发现工程株也和野生型菌种一样会发生菌落局变,但所插入的蝎毒基因并未丢失。与野生型出发菌株及其单孢分离株相比,工程株的角变率居高不下而产孢量及对松毛虫的毒力显著降低。然而,从该工程株筛选出的一株单孢分离     

The overexpression of one single cbh gene making Trichoderma asperellum T-1 a better cellulase producer

Trichoderma asperellum T-1, a traditional bio-control strain, is previously found to be potentially useful in the degradation of natural waste lignocellulose as it can ferment the natural materials without pretreatment. Many problems caused by substrate pretreatment can be therefore avoided. In this study, we intended to engineer a new strain to enhance its lignocellulose degradation ability by modifying the genome of T. asperellum T-1. A genetic transformation system mediated by Agrobacterium tumefaciens AGL-1 (ATMT) was constructed on T. asperellum T-1. On this basis, the overexpressed strain was produced by transforming a recombinant cellobiosidase gene (cbh) under the control of inducible promoter of endo-1, 4-β-xylanase gene, into wild-type T. asperellum T-1. After resistance screening, multiple transmission, growth comparison, and enzyme activity determination, four transformants (M1, M2, M5, and M6) were obtained. Filter paper cellulase activity of these transformants reached, respectively, 36.2%, 30.6%, 32.9%, and 42.7% higher than the wild-type strain. Most importantly, the CMCase, β-glucosidase and xylanase activity were also increased, although only one cbh gene was overexpressed. This work indicated that the enhancement of cellulase production ability of T. asperellum T-1 can be promisingly feasible by genetic modification. And the xylanase gene’s promoter can be effectively used in genetic modification to promote T. asperellum T-1 to be more effectively used in lignocellulose degradation.     

Isolation and characterization of solvent-tolerant Pseudomonas putida strain T-57, and its application to biotransformation of toluene to cresol in a two-phase (organic-aqueous) system

Pseudomonas putida T-57 was isolated from an activated sludge sample after enrichment on mineral salts basal medium with toluene as a sole source of carbon. P. putida T-57 utilizes n-butanol, toluene, styrene, m-xylene, ethylbenzene, n-hexane, and propylbenzene as growth substrates. The strain was able to grow on toluene when liquid toluene was added to mineral salts basal medium at 10–90% (v/v), and was tolerant to organic solvents whose log  P _ow (1-octanol/water partition coefficient) was higher than 2.5. Enzymatic and genetic analysis revealed that P. putida T-57 used the toluene dioxygenase pathway to catabolize toluene. A cis-toluene dihydrodiol dehydrogenase gene (todD) mutant of T-57 was constructed using a gene replacement technique. The todD mutant accumulated o-cresol (maximum 1.7 g/L in the aqueous phase) when cultivated in minimal salts basal medium supplemented with 3% (v/v) toluene and 7% (v/v) 1-octanol. Thus, T-57 is thought to be a good candidate host strain for bioconversion of hydrophobic substrates in two-phase (organic-aqueous) systems.

     

一株产T-2毒素镰孢菌的分离、鉴定及其产毒条件的研究

【目的】从青海大骨节病区小麦麦穗中分离的内生真菌中筛选产T-2毒素的菌株,并研究影响其合成该毒素的条件。【方法】采用种子胚芽抑制试验和抑菌试验从分离所得的菌株中筛选产毒菌株;利用薄层层析和高效液相检测待测菌株产物,复筛出产T-2毒素的菌株。通过显微形态学观察及ITS序列分析对筛选出的菌株5-5m-1进行鉴定。应用单因素筛选方案研究固体培养时间、温度以及液体培养转速、初始p H等对其产T-2毒素的影响,并采用正交试验进一步优化。【结果】菌株5-5m-1的显微形态与梨孢镰孢菌(Fusarium poae)相似;ITS序列分析显示,该菌株与F.poae的相似度也较高。其产T-2毒素的最佳条件为:玉米固体培养基、日温25°C/夜温15°C、光暗交替。【结论】5-5m-1菌株为梨孢镰孢菌,培养条件对其产T-2毒素能力有很大影响。实验结果将为进一步研究T-2毒素产生的机制和防止真菌毒素污染提供参考。     

Pathogen-derived resistance to Citrus tristeza virus (CTV) in transgenic mexican lime (Citrus aurantifolia (Christ.) Swing.) plants expressing its p25 coat protein gene

The p25 coat protein (CP) gene of Citrustristezavirus (CTV) was incorporated to Mexican lime plants and forty-twotransgeniclines were produced, 25 containing the p25 CP gene of thesevere CTV strain T-305 and 17 with that of the mild strain T-317. When plantspropagated from each transgenic line were graft-inoculated with CTV T-305 oraphidinoculated with T-300, two types of response to viral challenge wereobserved: some lines developed CTV symptoms similar to those of non-transgeniccontrols, whereas others exhibited protection against the virus. Thisprotectionconsisted of a proportion of plants, ranging from 10 to 33%, that wereresistantto CTV, and the rest of them that showed a significant delay in virusaccumulation and symptom onset. Protection was efficient against non-homologousCTV strains and was generally accompanied by high accumulation of p25 CP in theprotected lines, which suggest a CP-mediated protection mechanism in mostcases.This is the first report demonstrating pathogen-derived resistance intransgenicplants against a Closterovirus member in its natural host.     

Production and characterization of antibodies against HT-2 toxin and T-2 tetraol tetraacetate.

Three new immunogens which were prepared by conjugation of the carboxymethyl oxime (CMO) derivatives of HT-2 toxin, T-2 tetraol (T-2 4ol), and T-2 tetraol tetraacetate (T-2 4Ac) to bovine serum albumin (BSA) were tested for the production of antibodies against the major metabolites of T-2 toxin. Antibodies against HT-2 toxin and T-2 4Ac were obtained from rabbits 5 to 10 weeks after immunizing the animals with CMO-HT-2-BSA and CMO-T-2 4Ac-BSA conjugates. Immunization with CMO-T-2 4ol-BSA resulted in no antibody against T-2 4ol. The antibody produced against HT-2 toxin had great affinity for HT-2 toxin as well as good cross-reactivity with T-2 toxin. The relative cross-reactivities of anti-HT-2 toxin antibody with HT-2 toxin, T-2 toxin, iso-T-2 toxin, acetyl-T-2 toxin, 3'-OH HT-2, 3'-OH T-2, T-2 triol, and 3'-OH acetyl-T-2, were 100, 25, 10, 3.3, 0.25, 0.15, 0.12 and 0.08%, respectively. Antibody against CMO-T-2 4Ac was very specific for T-2 4Ac and had less than 0.1% cross-reactivity with T-2 toxin, HT-2 toxin, acetyl-T-2 toxin, diacetoxyscirpenol, deoxynivalenol, and deoxynivalenol triacetate as compared with T-2 4Ac. The detection limits for HT-2 toxin and T-2 4ol by radioimmunoassay were approximately 0.1 and 0.5 ng per assay, respectively.     

Production and characterization of antibodies against HT-2 toxin and T-2 tetraol tetraacetate

Three new immunogens which were prepared by conjugation of the carboxymethyl oxime (CMO) derivatives of HT-2 toxin, T-2 tetraol (T-2 4ol), and T-2 tetraol tetraacetate (T-2 4Ac) to bovine serum albumin (BSA) were tested for the production of antibodies against the major metabolites of T-2 toxin. Antibodies against HT-2 toxin and T-2 4Ac were obtained from rabbits 5 to 10 weeks after immunizing the animals with CMO-HT-2-BSA and CMO-T-2 4Ac-BSA conjugates. Immunization with CMO-T-2 4ol-BSA resulted in no antibody against T-2 4ol. The antibody produced against HT-2 toxin had great affinity for HT-2 toxin as well as good cross-reactivity with T-2 toxin. The relative cross-reactivities of anti-HT-2 toxin antibody with HT-2 toxin, T-2 toxin, iso-T-2 toxin, acetyl-T-2 toxin, 3'-OH HT-2, 3'-OH T-2, T-2 triol, and 3'-OH acetyl-T-2, were 100, 25, 10, 3.3, 0.25, 0.15, 0.12 and 0.08%, respectively. Antibody against CMO-T-2 4Ac was very specific for T-2 4Ac and had less than 0.1% cross-reactivity with T-2 toxin, HT-2 toxin, acetyl-T-2 toxin, diacetoxyscirpenol, deoxynivalenol, and deoxynivalenol triacetate as compared with T-2 4Ac. The detection limits for HT-2 toxin and T-2 4ol by radioimmunoassay were approximately 0.1 and 0.5 ng per assay, respectively.     

An extremely oligotrophic bacterium, Rhodococcus erythropolis N9T-4, isolated from crude oil

Rhodococcus erythropolis N9T-4, which was isolated from crude oil, showed extremely oligotrophic growth and formed its colonies on a minimal salt medium solidified using agar or silica gel without any additional carbon source. N9T-4 did not grow under CO(2)-limiting conditions but could grow on a medium containing NaHCO(3) under the same conditions, suggesting that the oligotrophic growth of N9T-4 depends on CO(2). Proteomic analysis of N9T-4 revealed that two proteins, with molecular masses of 45 and 55 kDa, were highly induced under the oligotrophic conditions. The primary structures of these proteins exhibited striking similarities to those of methanol: N,N'-dimethyl-4-nitrosoaniline oxidoreductase and an aldehyde dehydrogenase from Rhodococcus sp. These enzyme activities were three times higher under oligotrophic conditions than under n-tetradecane-containing heterotrophic conditions, and gene disruption for the aldehyde dehydrogenase caused a lack of growth on the minimal salt medium. Furthermore, 3-hexulose 6-phosphate synthase and phospho-3-hexuloisomerase activities, which are key enzymes in the ribulose monophosphate pathway in methylotrophic bacteria, were detected specifically in the cell extract of oligotrophically grown N9T-4. These results suggest that CO(2) fixation involves methanol (formaldehyde) metabolism in the oligotrophic growth of R. erythropolis N9T-4.