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An evaluation of soil bioaugmentation with microorganisms bearing plasmidpJP4: Plasmid dissemination and impact on remediation.

机译:带有质粒pJP4的微生物对土壤的生物增强作用的评估:质粒的传播及其对修复的影响。

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摘要

The objective of this research was to evaluate the impact of bioaugmentation of soil with microorganisms harboring plasmid pJP4 on remediation, plasmid transfer, and plasmid dispersal. Divided into three sections, this research showed that use of microbial inocula harboring self-transmissible plasmids holds promise as an applicable bioremediation approach.; In the first study, a pJP4 donor that could readily be counter-selected due to a lack of chromosomal genes necessary for 2,4-dichlorophenoxyacetic acid (2,4-D) mineralization was generated to allow detection of transconjugants in soil. Plasmid pJP4 was introduced into Escherichia coli (ATCC 15224), via plate mating with Ralstonia eutropha JMP134 to create such a donor (E. coli D11). Transfer of Plasmid pJP4 to diverse indigenous populations was detected in soils, and under conditions, where it had not been observed previously.; Plexiglass columns were used in the second study to evaluate dissemination of plasmid pJP4 under unsaturated or saturated flow conditions in a 2,4-D contaminated soil. In unsaturated soil, pJP4 was detected in both culturable donor and transconjugant cells extending to 10.5 cm from the inoculated layer. In soil subjected to saturated flow conditions, no transconjugants were detected; however, donors were found throughout the entire length of the column (30.5 cm). Thus, donor transport in conjunction with plasmid transfer to indigenous recipients allowed for significant dissemination of introduced genes through contaminated soil.; The last study was conducted using soil contaminated with 2,4-D alone or co-contaminated with 2,4-D and cadmium (Cd). This study assessed the impact of introduction of the pJP4 genes via cell bioaugmentation (R. eutropha JMP134 donor), or via gene augmentation (E. coli D11 donor). Both introduced donors remained culturable and transferred plasmid pJP4 to diverse indigenous recipients. Cell bioaugmentation resulted in the most rapid 2,4-D degradation; however, upon a second exposure to 2,4-D, gene augmentation of indigenous populations was more successful. The presence of Cd (100 μg g dry soil−1) had a minimal impact on 2,4-D degradation and transconjugant formation. The establishment of an array of stable indigenous plasmid hosts may be particularly useful in sites with potential for re-exposure or extensive, and thus, long term contamination.
机译:这项研究的目的是评估带有质粒pJP4的微生物对土壤的生物强化对修复,质粒转移和质粒分散的影响。分为三个部分,这项研究表明使用带有自我传播质粒的微生物接种物有望作为一种适用的生物修复方法。在第一个研究中,由于缺少2,4-二氯苯氧基乙酸(2,4-D)矿化所必需的染色体基因,因此可以轻易地反选pJP4供体,以检测土壤中的共轭结合物。通过与 Ralstonia eutropha JMP134的平板交配将质粒pJP4导入大肠杆菌(ATCC 15224),以创建这种供体( E。coli D11 )。在土壤中和在以前没有观察到的条件下,检测到质粒pJP4向不同的土著种群的转移。在第二项研究中,使用有机玻璃柱评估了质粒pJP4在不饱和或饱和流动条件下在2,4-D污染土壤中的分布。在不饱和土壤中,在可培养的供体和转结合细胞中都检测到了pJP4,该细胞距接种层10.5 cm。在饱和流动条件下的土壤中,未检测到任何共轭物。但是,在整个柱长(30.5厘米)中都发现了供体。因此,供体的运输结合质粒向土著受体的转移使引入的基因可以通过受污染的土壤大量传播。上一项研究是使用仅被2,4-D污染或与2,4-D和镉(Cd)共同污染的土壤进行的。这项研究评估了通过细胞生物增强( R。eutropha JMP134供体)或通过基因增强( E。coli D11供体)引入pJP4基因的影响。两种引入的供体仍可培养并将质粒pJP4转移至不同的土著受体。细胞的生物强化导致最快速的2,4-D降解。然而,第二次接触2,4-D后,土著居民的基因扩增更为成功。 Cd(100μg干燥土壤 -1 )的存在对2,4-D降解和共轭结合物形成的影响最小。建立稳定的本地质粒宿主阵列可能在有可能再次暴露或长期广泛污染的场所中特别有用。

著录项

  • 作者

    Newby, Deborah Trishelle.;

  • 作者单位

    The University of Arizona.;

  • 授予单位 The University of Arizona.;
  • 学科 Biology Microbiology.; Agriculture Soil Science.; Engineering Environmental.
  • 学位 Ph.D.
  • 年度 2000
  • 页码 155 p.
  • 总页数 155
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 微生物学;土壤学;环境污染及其防治;
  • 关键词

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