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通过传播分解代谢质粒增强土壤中2,4-二氯苯氧乙酸(2,4-D)的降解

Enhancement of 2,4-dichlorophenoxyacetic acid (2,4-D) degradation in soil by dissemination of catabolic plasmids.

作者信息

Top E M, Van Daele P, De Saeyer N, Forney L J

机构信息

Department of Biochemical and Microbial Technology, Faculty of Agricultural and Applied Biological Sciences, University of Ghent, Belgium.

出版信息

Antonie Van Leeuwenhoek. 1998 Jan;73(1):87-94. doi: 10.1023/a:1000663619522.

Abstract

Few studies have been done to evaluate the transfer of catabolic plasmids from an introduced donor strain to indigenous microbial populations as a means to remediate contaminated soils. In this work we determined the effect of the conjugative transfer of two 2,4-D degradative plasmids to indigenous soil bacterial populations on the rate of 2,4-D degradation in soil. We also assessed the influence of the presence of 2,4-D on the number of transconjugants formed. The two plasmids used, pEMT1k and pEMT3k, encode 2,4-D degradative genes (tfd) that differ in DNA sequence as well as gene organisation, and confer different growth rates to Ralstonia eutropha JMP228 when grown with 2,4-D as a sole carbon source. In an agricultural soil (Ardoyen) treated with 2,4-D (100 ppm) there were ca. 10(7) CFU of transconjugants per gram bearing pEMT1k as well as a high number of pEMT3k bearing transconjugants (ca 10(6) CFU/g). In this soil the formation of a high number of 2,4-D degrading transconjugants resulted in faster degradation of 2,4-D as compared to the uninoculated control soil. In contrast, only transconjugants with pEMT1k were detected (at a level of ca. 10(3) CFU/g soil) in the untreated Ardoyen soil. High numbers of transconjugants that carried pEMT1k were also found in a second experiment done using forest soil (Lembeke) treated with 100 ppm 2,4-D. However, unlike in the Ardoyen soil, no transconjugants with pEMT3k were detected and the transfer of plasmid pEMT1k to indigenous bacteria did not result in a higher rate of decrease of 2,4-D. This may be because 2,4-D was readily metabolised by indigenous bacteria in this soil. The results indicate that bioaugmentation with catabolic plasmids may be a viable means to enhance the bioremediation of soils which lack an adequate intrinsic ability to degrade a given xenobiotic.

摘要

很少有研究评估分解代谢质粒从引入的供体菌株转移到本地微生物群体,以此作为修复受污染土壤的一种手段。在这项研究中,我们测定了两种2,4 -二氯苯氧乙酸(2,4 - D)降解性质粒向本地土壤细菌群体的接合转移对土壤中2,4 - D降解速率的影响。我们还评估了2,4 - D的存在对形成的接合子数量的影响。所使用的两种质粒pEMT1k和pEMT3k编码2,4 - D降解基因(tfd),这些基因在DNA序列以及基因组织上存在差异,并且当以2,4 - D作为唯一碳源生长时,赋予了嗜麦芽窄食单胞菌JMP228不同的生长速率。在一块用2,4 - D(100 ppm)处理过的农业土壤(Ardoyen)中,每克土壤中携带pEMT1k的接合子大约有10⁷CFU,以及大量携带pEMT3k的接合子(大约10⁶CFU/g)。在这种土壤中,大量2,4 - D降解接合子的形成导致2,4 - D的降解速度比未接种的对照土壤更快。相比之下,在未处理的Ardoyen土壤中,仅检测到携带pEMT1k的接合子(土壤中含量约为10³CFU/g)。在另一项使用用100 ppm 2,4 - D处理过的森林土壤(Lembeke)进行的实验中,也发现了大量携带pEMT1k的接合子。然而,与Ardoyen土壤不同的是,未检测到携带pEMT3k的接合子,并且质粒pEMT1k向本地细菌的转移并没有导致2,4 - D的降解速率更高。这可能是因为在这种土壤中,2,4 - D很容易被本地细菌代谢。结果表明,用分解代谢质粒进行生物强化可能是一种可行的手段,可用于增强那些缺乏足够固有能力来降解特定外源化合物的土壤的生物修复。

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