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Bacillus strains used for biological control of fusarium head blight: Identification, growth studies, and lipopeptide production.

机译:用于控制镰刀菌枯萎病的芽孢杆菌菌株:鉴定,生长研究和脂肽生产。

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摘要

For the last several years, our laboratory has been working with four endospore-forming bacterial strains (designated as 1B-A, 1B-C, 1B-E, and 1D-3) isolated from South Dakota wheat foliage and residue that can antagonize Fusarium graminearum in laboratory plate assays and in greenhouse and field plot trials. We have attempted to identify these bacterial strains by different techniques, with different identification methods resulting in different genus affiliations for the strains. Sequence analysis showed that all four strains had identical sequences in the first 500 base pairs of their 16S rDNA genes, and all were most closely related to Bacillus amyloliquefaciens with less but significant relatedness to Bacillus atrophaeus . In the work presented here, colony morphology, microscopic appearance, and phenotypic traits were evaluated and used to arrive at suggested identities for the strains. Strains 1B-A and 1B-C had similar colony morphology, with a shiny and undulate appearance, whereas colonies of strain 1B-E were shiny but not wrinkled, and colonies of strain 1D-3 were a dull color with dotted appearance instead of wrinkles. Results of phenotypic tests suggested that all four strains were most closely related to Bacillus firmus. These attempts to identify the four strains strongly suggest that they are tied to a phylogenetically and phenetically coherent B. subtilis group (group II). However, the four strains may all belong to a previously uncharacterized taxon with relatedness to B. amyloliquefaciens and B. atrophaeus, taxa that were split out of the old Bacillus subtilis taxon. There is a good amount known about the antibiotics produced by members of the B. subtilis group (group II). Among the many antibiotics produced by B. subtilis and its relatives are cyclic lipopeptides such as iturin and surfactin. We have cultured these bacterial strains in potato dextrose broth (PDB), a complex medium containing glucose, which may suppress iturin production to some degree. We have also cultured the Bacillus sp. in a defined broth medium lacking glucose, containing mannitol, glutamic acid and inorganic salts. Bacterial cell numbers in this original formulation were lower than desirable for application of cells to wheat plants, so a modification of the original medium was used increasing the mannitol by 2.3 times, and increasing the glutamic acid by 2.1 times. After 10 days of growth in the modified broth medium with increased carbon and nitrogen sources, bacterial strain 1B-A grew to over 10 times the optical density it achieved in the initial medium formulation. Plate count data also showed better growth of 1B-A in the modified defined medium having elevated carbon and nitrogen. Higher numbers of cells in the modified defined growth medium should allow better coverage of bacterial cells sprayed onto wheat surfaces when these bacteria are used in biocontrol trials. In addition, plate assays were done to see whether pure iturin would antagonize F. graminearum, and if the defined broth media in solidified form allowed the bacteria to antagonize the fungus. Purified iturin A was found to inhibit F. graminearum at a concentration of 40 mug/ml applied to a paper disk, challenging growth of the fungus on Potato Dextrose Agar. Analysis of extracts of broth cultures in defined media by absorption spectroscopy and HPLC indicated that iturin-like compounds were produced by all four Bacillus strains we have studied. Better understanding of the production of iturin, surfactin and other compounds that might act in concert with them would allow better understanding and use of these and related bacteria as biocontrol agents to control FHB. Bacillus sp. strain 1B-A was cultured in a variety of defined (synthetic) and semi-defined broth media that lack glucose (which can suppress iturin production) to see if types and amounts of antibiotics produced differed in different media. The three broth media that were studied were: (1) a basal defined medium (BDM) containing mannitol, glutamic acid and inorganic salts; (2) a defined medium (DM) similar to BDM but containing increased amounts of mannitol and glutamic acid; and (3) a defined medium with the same composition as (2) but with increased concentrations of calcium and manganese, two elements which are known to be important in regulating different aspects of Bacillus metabolism. Broth cultures of Bacillus strain 1B-A were grown for different time periods in these three media. (Abstract shortened by UMI.)
机译:在过去的几年中,我们的实验室一直在研究从南达科他州小麦叶片中分离出的四种能形成内生孢子的细菌菌株(命名为1B-A,1B-C,1B-E和1D-3)和可以拮抗镰刀菌的残留物。谷氨酰胺在实验室平板测定以及温室和田间试验中的应用。我们试图用不同的技术鉴定这些细菌菌株,用不同的鉴定方法导致这些菌株的属属不同。序列分析表明,这四个菌株在其16S rDNA基因的前500个碱基对中具有相同的序列,并且都与解淀粉芽孢杆菌关系最密切,而与萎缩芽孢杆菌的联系却不那么明显。在本文介绍的工作中,对菌落的形态,显微外观和表型性状进行了评估,并用于确定菌株的建议身份。菌株1B-A和1B-C具有相似的菌落形态,有光泽和起伏的外观,而菌株1B-E的菌落有光泽但没有皱纹,菌株1D-3的菌落是暗淡的颜色,带有点状外观而不是皱纹。表型测试的结果表明,所有四个菌株与芽孢杆菌紧密相关。这些试图鉴定四种菌株的尝试强烈表明,它们与系统发育和表观上一致的枯草芽孢杆菌组(II组)相关。但是,这四个菌株可能都属于以前未鉴定的分类单元,与解淀粉芽孢杆菌和萎缩芽孢杆菌的分类单元相关,它们是从旧枯草芽孢杆菌分类单元中分离出来的。关于枯草芽孢杆菌组(II组)的成员产生的抗生素有很多已知的知识。枯草芽孢杆菌及其亲属产生的许多抗生素中,有环脂肽,如iturin和surfactin。我们已经在马铃薯葡萄糖肉汤(PDB)中培养了这些细菌菌株,马铃薯葡萄糖肉汤是一种含有葡萄糖的复杂培养基,可以在一定程度上抑制尿素的产生。我们还培养了芽孢杆菌。在缺乏葡萄糖的特定肉汤培养基中,含有甘露醇,谷氨酸和无机盐。该原始配方中的细菌细胞数量低于将细胞应用于小麦植株所需的细菌细胞数量,因此使用了对原始培养基的改良,将甘露醇提高了2.3倍,并将谷氨酸提高了2.1倍。在碳和氮源增加的改良肉汤培养基中生长10天后,细菌菌株1B-A的生长密度达到其在初始培养基配方中达到的光密度的10倍以上。板计数数据还显示在具有升高的碳和氮的改良的确定培养基中1B-A的更好生长。当将这些细菌用于生物防治试验时,改良的定义生长培养基中的细胞数量较高,应该可以更好地覆盖喷洒到小麦表面的细菌细胞。另外,进行平板试验以观察纯的伊图灵是否会拮抗禾本科镰刀菌,以及确定的固体培养基培养基是否允许细菌拮抗真菌。已发现纯化的iturin A可以以40杯/毫升的浓度抑制禾本科镰刀菌到纸盘上,挑战真菌在马铃薯葡萄糖琼脂上的生长。通过吸收光谱法和HPLC分析在确定的培养基中的肉汤培养物的提取物表明,我们研究的所有四种芽孢杆菌属菌株都产生了类鸟尿素样化合物。更好地了解iturin,surfactin和其他可能与之协同作用的化合物的产生,将有助于更好地了解和使用这些细菌和相关细菌作为控制FHB的生物控制剂。芽孢杆菌将菌株1B-A在缺少葡萄糖的多种特定(合成)和半特定肉汤培养基中进行培养(可抑制尿ur素的产生),以查看在不同培养基中产生的抗生素的类型和数量是否不同。研究的三种肉汤培养基为:(1)含甘露醇,谷氨酸和无机盐的基础培养基(BDM); (2)与BDM相似但含有增加量的甘露醇和谷氨酸的限定培养基(DM); (3)确定的培养基,其组成与(2)相同,但钙和锰的浓度增加,这两种元素在调节芽孢杆菌代谢的不同方面都很重要。在这三种培养基中,芽孢杆菌菌株1B-A的肉汤培养物生长了不同的时间。 (摘要由UMI缩短。)

著录项

  • 作者

    Baye, Nichole Louise.;

  • 作者单位

    South Dakota State University.;

  • 授予单位 South Dakota State University.;
  • 学科 Biology Microbiology.
  • 学位 M.S.
  • 年度 2007
  • 页码 87 p.
  • 总页数 87
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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