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1.
从大连海域20~30 m深处生长的海绵中分离到一株有很高抗菌活性的链霉菌D164。根据培养和显微形态、生理生化数据、16S rRNA基因序列数据分析,菌株D164鉴定为娄彻氏链霉菌(Streptomyces rochei)。对菌株D164发酵产物进行抗农业病原菌、杀虫和除草活性检测,结果表明,菌株D164发酵产物具有很高的抗农业病原菌活性,同时又具有很高的杀虫和除草活性,其活性化合物值得进一步研究。  相似文献   

2.
内生拮抗放线菌FRo2的鉴定及抑菌活性物质的分离   总被引:1,自引:1,他引:0  
【目的】鉴定从东乡野生稻根部分离得到的对多种农作物病原真菌具有拮抗活性的内生放线菌株FRo2,并对其抑菌活性物质进行分离。【方法】根据FRo2形态特征观察、生理生化特性、细胞壁组分和16S rRNA基因序列对其进行鉴定。采用管碟法和菌丝生长速率法测定了该菌株的抗菌活性,活性追踪法结合正相硅胶柱层析及凝胶(Sephadex LH-20)柱层析等技术对抑菌组分进行分离,并通过NMR对抑菌活性物质进行解析。【结果】菌株FRo2属于链霉菌属,与娄彻氏链霉菌(Streptomyces rochei)极为相似。该菌株发酵液对小麦赤霉菌、立枯丝核菌等7种主要农作物致病菌具有较好的抑制活性;从菌株FRo2发酵液中分离得到抑菌活性化合物AW2,结构鉴定为邻苯二甲酸二丁酯。【结论】研究阐明了内生放线菌FRo2抑菌活性物质,也为该菌今后的农业生防应用提供物质基础。  相似文献   

3.
采用硅胶柱色谱和半制备反相高效液相色谱分离方法,对南海海洋放线菌Streptomyces lusitanus SCSIOLR32的次级代谢产物进行了研究,分离得到四个酰胺类化合物,经MS1、H和13 C NMR波谱分析鉴定为二甲基甲苯2,4-二氨基甲酸甲酯(1),甲苯2,4-二氨基甲酸乙酯(2),甲苯2,6-二氨基甲酸甲酯(3)和甲苯2,6-二氨基甲酸乙酯(4)。运用X-单晶衍射确定了1的结构式。其中化合物2和4是首次从自然界中分离得到。采用16S分子生物学方法鉴定该菌株为链霉菌属放线菌。  相似文献   

4.
番茄灰霉病生防链霉菌筛选及鉴定   总被引:1,自引:0,他引:1  
【背景】由灰葡萄孢侵染所致的番茄灰霉病是一类重要的真菌病害,生物防治具有环境友好、病原菌不易产生抗药性等特点,是果蔬灰霉病绿色防控的有效措施。【目的】筛选对番茄灰霉病具有防病作用且能促进番茄种子发芽的广谱拮抗性链霉菌,并明确该菌株种级分类地位。【方法】采用琼脂块法筛选拮抗番茄灰霉病菌的链霉菌菌株,采用对峙培养法和生长速率法检测菌株T22抑菌谱,通过产胞外酶活性检测、离体叶片防效和种子发芽试验明确该菌株的防病促生相关特性,根据形态学特征、生理生化特性和分子生物学方法对该菌株进行种类鉴定。【结果】从分离的56株放线菌中筛选到14株对番茄灰霉病菌具有拮抗效果的放线菌菌株,其中链霉菌T22对番茄灰霉病菌抑制作用最强,且具有较广抑菌谱,同时菌株T22具有产生纤维素酶和几丁质酶的能力。菌株T22无菌发酵滤液对番茄灰霉病菌、桃褐腐病菌、黄瓜枯萎病菌抑菌率分别为84.6%、81.5%和79.1%;其无菌发酵滤液原液对番茄灰霉病离体防效为55.1%;100倍稀释液处理番茄种子,胚轴、胚根和种子活力指数分别增加15.1%、29.7%和43.9%。根据形态学特征、生理生化特性和多基因聚类分析将链霉菌T22鉴定为白黑链霉菌(Streptomycesalboniger)。【结论】白黑链霉菌T22具有较强的抗真菌、产胞外酶、防病和促生活性,在番茄灰霉病生物防治中具有较好的开发应用潜力。  相似文献   

5.
利用稀释涂布法从番茄根际土壤中分离放线菌,并以番茄灰霉菌为靶标,利用对峙培养法和牛津杯法筛选拮抗放线菌,得到一株具有较强抑菌活性的放线菌LA-5.通过培养特征、生理生化特性及基于16S rDNA 序列系统进化分析,将菌株LA-5初步鉴定为链霉菌.复筛结果显示,LA-5发酵滤液对番茄灰霉菌孢子萌发及菌丝生长均有明显的抑制作用,其中100倍发酵滤液对孢子萌发抑制率和菌丝生长抑制率均在50%以上;受抑制菌落呈白色,气生菌丝萎缩稀疏,菌丝纤细、分支明显减少.离体防效试验显示,菌株LA-5发酵原液对番茄灰霉病防效可达83.4%.该菌株有望开发为防治番茄灰霉病的生防菌株.  相似文献   

6.
从新疆甜瓜根际土壤中分离到1株甜瓜细菌性斑点病拮抗放线菌P-13, 根据其形态学、生理特征和16S rRNA序列分析, 鉴定该菌株为娄彻氏链霉菌(Streptomyces rochei)。琼脂扩散法生物活性研究表明, 其发酵液对细菌性果腐病菌(Acidovorax avenae subsp. citrull)BFB、细菌性角斑病菌(Pseudomonas syringae pv. Lachrymans)P4的抑菌圈直径分别为19 mm和17 mm以上; 发酵液中抑菌物质主要为胞外代谢物, 不溶于石油醚, 乙醚, 乙酸乙酯等有机溶剂。在100°C处理10 min、pH 6处理6 h或紫外线照射7 h, 该物质抑菌活性不变。纸层析结果表明, 该物质主要为碱性水溶性物质。  相似文献   

7.
土壤放线菌P3-2的分类鉴定及抗菌活性研究   总被引:1,自引:0,他引:1  
对从贵州土壤微生物中筛选到的放线菌菌株P3-2进行了分类学和抗菌活性的研究。采用多相分类法,对该菌株的形态特征、培养特征、生理生化特性以及16S rDNA基因序列进行了研究。结果表明,放线菌P3-2菌株属于链霉菌属;16SrDNA序列长度为1 456 bp,序列分析和系统进化树分析表明其序列与Streptomyces recifenis ST100的同源性最高,为99.4%。但与S.recifenis ST100相比较,P3-2菌株的培养特征和生理生化特性中多项指标都存在着不同,初步确定菌株P3-2为链霉菌属中S.recifenis ST100的一个亚种,暂定名为Streptomyces sp.P3-2。P3-2菌株的10倍稀释发酵液对油菜菌核病菌、黄瓜灰霉病菌、小麦赤霉病菌、水稻纹枯病菌及半夏立枯病菌的抑制率高达99%,对烟灰霉病菌、玉米小斑病菌等9种病原真菌均有不同程度的抑制作用,对金黄色葡萄球菌、蜡状芽孢杆菌和枯草芽孢杆菌有一定的抑制作用。  相似文献   

8.
对青海干旱生境土壤链霉菌Streptomyces pactum KIB-HL8液体发酵,应用硅胶柱色谱和高效液相色谱等方法进行分离和纯化,得到5个化合物,并用MS、NMR等方法对其结构进行解析,分别鉴定为N-乙酰酪胺(1)、N-乙酰色胺(2)、吡咯-2-甲酰胺(3)、Inthomycin C(4)和Inthomycin B(5)。对其抗真菌、细菌活性进行筛选,发现化合物4对金黄色葡萄球菌有抑制活性,化合物1和2对番茄灰霉病菌有抑制活性,化合物3对番茄早疫病菌有较强的抑制活性。  相似文献   

9.
从南海海洋沉积物中分离得到1株海洋放线菌,鉴定为链霉菌Streptomyces sp. SCSIO 1672。通过优化发酵条件,采用海虾生物致死活性和高效液相色谱追踪,利用有机溶剂萃取、正相硅胶、反相硅胶等各种色谱层析方法分离出活性化合物,通过波谱数据解析出海洋放线菌SCSIO 1672次级代谢产物中的该活性化合物为水杨酸。  相似文献   

10.
【目的】筛选并鉴定西藏林芝八一镇土壤中产生抗肿瘤活性物质的放线菌。【方法】用平板稀释法分离放线菌, 用MTT法和纸碟法对放线菌发酵产物进行体外抗肿瘤与抑菌活性检测, 并用多相分类技术对抗肿瘤活性菌株进行鉴定。【结果】共分离出29株放线菌, 得到6个抑制体外肿瘤细胞增殖的活性菌株(20.7%), 同时它们也具有抑菌活性, 其中4株菌的检测样品对Hela细胞的抑制率达80%以上。多相分类研究表明, 6个活性菌株分别隶属于链霉菌属(Streptomyces)的3个已知物种的变种。【结论】林芝八一镇土壤放线菌中蕴藏抗肿瘤活性链霉菌, 是一个潜在的抗肿瘤药用微生物资源。  相似文献   

11.
茄子青枯病拮抗放线菌XL-6的筛选、鉴定及发酵条件优化   总被引:1,自引:0,他引:1  
【背景】茄子青枯病是一种毁灭性的土传病害,生产上化学农药无法对其有效防治。拮抗放线菌具有环保、无残留的优点,并已在植物多种病害上成功应用,这为茄子青枯病的生物防治提供了思路。【目的】从健康茄子根际分离获得对茄子青枯菌有显著拮抗作用的放线菌菌株。【方法】采用稀释涂布法分离放线菌;采用双层琼脂法、琼脂扩散法和平板对峙法筛选拮抗菌株;对目标菌株XL-6的形态、培养特征、生理生化特征及16S rRNA基因序列进行综合分析;通过单因素试验和正交设计试验优化目标菌株培养基组分及发酵条件。【结果】筛选得到一株对青枯菌有强抑制作用的放线菌菌株XL-6,它对其他3种病原菌均具有一定的抑制作用。菌株XL-6的形态和培养特征、生理生化特征与娄彻氏链霉菌相符,而且16S rRNA基因序列分析表明该菌株与娄彻氏链霉菌亲缘关系较近。该菌株最优发酵配方和培养条件分别为:玉米粉30.0 g/L、酵母粉5.0 g/L、K_2HPO_4 2.0 g/L、MgCl_2 2.0 g/L和NaCl 1.0 g/L;初始pH 7.0、培养基装瓶量70 mL/250 mL、摇床转速180 r/min、接种量6%,在28°C条件下培养6 d。【结论】菌株XL-6经鉴定为娄彻氏链霉菌,优化其发酵条件后对青枯菌具有更强的拮抗效果。  相似文献   

12.
Chen HB  Ma L  Han JC  Liu HP  Yan YP 《应用生态学报》2011,22(9):2419-2423
An endophytic actinomycete strain Fq24 was isolated from healthy tomato plants. The acaricidal substances in the metabolites from Fq24 were collected and identified by the methods of extraction, column chromatography, and gas chromatography-mass spectrometry (GC-MS), and their bioactivities against Tetranychus cinnabarinus were measured with slide-dip and leaf-residue methods. Among the extracts, petroleum ether extract had high bioactivity in contact toxicity and oviposition deterrent against T. cinnabarinus. Its lethal concentration of 50% (LC50) was 52.57 mg x L(-1), and its oviposition deterrent concentration of 50% (ODC50) was 43.18 mg x L(-1). The identification with GC-MS showed that the main chemical component of fraction S11 was methyl hexadecanoate, whose molecular formula was C17H34O2, being one of the substances with acaricidal activity in the metabolites from Fq24. The 24 h corrected mortality rate of female mite at 5 mg x mL(-1) of methyl hexadecanoate was 78.3%, and the oviposition deterrent rate was 81.6%.  相似文献   

13.
One major field of interest in bioinorganic chemistry is the design and synthesis of inorganic compounds with low molecular mass, showing structural, spectroscopic, and reactivity properties that mimic enzymes, such as purple acid phosphatases (PAPs). In this study, the unsymmetrical heptadentate ligand 2-[(4,7-diisopropyl-1,4,7-triazacyclonon-1-yl)methyl]-6-{[(2-hydroxybenzyl)(pyridin-2-ylmethyl)-amino]methyl}-4-methylphenol (H(2) L) and its first mixed-valence complex [Fe(III) Zn(II) (L)(μ-OAc)(2) ]ClO(4) (1) were synthesized. Physical and chemical measurements (crystal structure, conductometry, IR and UV/VIS spectroscopy, and electrochemistry) were performed for 1, and these properties are compared with those presented by the kbPAPs active sites. Potentiometric titration studies of 1 have confirmed its acid/base properties that are crucial for the understanding of the phosphodiester and DNA catalytic cleavage in future studies.  相似文献   

14.
【目的】建立并优化链霉菌Fostriecin产生菌Streptomyces pulveraceus的遗传转化系统。【方法】以整合型质粒pSET152为出发质粒,通过供体菌E.coli ET12567/pUZ8002与受体菌Streptomyces pulveraceus进行接合转移。【结果】确定了链霉菌Streptomyces pulveraceus的最佳接合转移条件:培养基为终浓度含15%甘氨酸的MS培养基;孢子热激条件为50°C 10 min;阿伯拉霉素覆盖的时间为18 h,终浓度为20 mg/L。同时,把组成型启动子ermE+与绿色荧光蛋白基因(gfp)克隆到pSET152载体上,通过接合转移整合到该链霉菌中,gfp获得表达。【结论】建立Fostriecin产生菌的遗传转化系统,并发现甘氨酸能显著提高链霉菌的接合转移效率。  相似文献   

15.
Simulation of X- and Q-band electron paramagnetic resonance (EPR) spectra of an unsymmetric dinuclear [Mn(2)(II,III)L(mu-OAc)(2)]ClO(4) complex (1), (L is the dianion of 2-{[N,N-bis(2-pyridylmethyl)amino]methyl}-6-{[N-(3,5-di-tert-butyl-2-hydroxybenzyl)-N-(2-pyridylmethyl)amino]methyl}-4-methylphenol) was performed using one consistent set of simulation parameters. Rhombic g-tensors and hyperfine tensors were necessary to obtain satisfactory simulation of the EPR spectra. The anisotropy of the effective hyperfine tensors of each individual (55)Mn ion was further analyzed in terms of intrinsic hyperfine tensors. Detailed analysis shows that the hyperfine anisotropy of the Mn(III) ion is a result of the Jahn-Teller effect and thus an inherent character. In contrast, the anomalous hyperfine anisotropy of the Mn(II) ion is attributed as being transferred from the Mn(III) ion through the spin exchange interaction. The anisotropy parameter for the Mn(II) is deduced as D(II)=-1.26+/-0.2cm(-1). This is the first reported D(II) value for a Mn(II) ion in a weakly exchange coupled mixed-valence Mn(2)(II,III) complex with a bis-mu-acetato-bridge. The [see text] electronic configuration of the Mn(III) ion in 1 is revealed by the negative sign of its intrinsic hyperfine tensor anisotropy, Deltaa(III)=a(z)-a(x,y)=-46cm(-1). Lower spectral resolution of the Q-band EPR spectrum as compared to the X-band EPR spectrum is associated to large line width broadening of the x- and y-components in contrast to the z-component. The origins of the unequal distribution of line width between the z- and x-, y-components are discussed.  相似文献   

16.
海洋芽孢杆菌(Bacillus marinus)B-9987菌株抑制病原真菌机理   总被引:1,自引:0,他引:1  
[目的]探讨海洋芽孢杆菌(Bacillus marinus)B-9987菌株的代谢产物BMME-1,对植物病原真菌茄链格孢菌的抑菌作用机理.[方法]分别使用分光光法、气相色谱-质谱GC-MS联用技术、红外光谱法等,检测了BMME-1处理病原真菌后,菌体渗透性、细胞壁及细胞膜成份的变化.[结果]BMME-1对茄链格孢菌的抑菌中浓度(MIC_(50))为6.2 mg/L,最小杀菌浓度(MFC)为50 mg/L,在MIC_(50)浓度或高于此浓度处理靶标菌,将导致菌体蛋白质、核酸等大分子物质的外流;处理菌株葡聚糖结构β-型糖苷键、碳-氧键(C-O)、碳-氢键(C-H)等基团的特征吸收强度降低,-OH、C=O的伸缩振动吸收强度升高;菌体细胞壁几丁质结构中酰胺I键吸收强度发生变化;与对照菌株的麦角甾醇含量(62.52±3.31%)相比,处理菌株麦角甾醇减少为(56.36±2.52)%,同时出现麦角固醇合成中间产物粪甾醇.[结论]BMME-1对病原真菌的抑制表现为:干扰细胞膜麦角甾醇的合成从而改变了细胞的通透性;对细胞壁葡聚糖结构的影响较大而几丁质次之.  相似文献   

17.
A new substance, molecular formula C8H10O2, was isolated from the unripe fruits of Citrullus colocynthis, SCHRAD. Judging from the results of infrared absorption spectra, properties of the derivatives and the oxidative product of methyl derivative, this substance was pressumed to be p-hydroxybenzyl methyl ether and this assumption was proved beyond doubt by its direct comparison with an authentic synthesized sample.  相似文献   

18.
The purpose of this work was to screen clinical isolates of actinomycetes producing nonpolyenic antifungals. This choice was made to limit the problem of rediscovery of well-known antifungal families, especially polyenic antifungals. One hundred and ten strains were tested, using two diffusion methods and two test media, against three yeast species and three filamentous fungi. Among 54 strains (49%) showing antifungal activity, five strains belonging to the genus Streptomyces were active against all test organisms and appeared promising. These results indicate that clinical and environmental isolates of actinomycetes could be an interesting source of antifungal bioactive substances. The production of nonpolyenic antifungal substances by these five active isolates was investigated using several criteria: antibacterial activity, ergosterol inhibition, and UV-visible spectra of active extracts. One active strain responded to all three selection criteria and produced potentially nonpolyenic antifungal metabolites. This strain was retained for further investigation, in particular, purification, structure elucidation, and mechanism of action of the active product.  相似文献   

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