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首页> 外文期刊>Research in Microbiology >Long-term persistence and bacterial transformation potential of transplastomic plant DNA in soil.
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Long-term persistence and bacterial transformation potential of transplastomic plant DNA in soil.

机译:转质体植物DNA在土壤中的长期持久性和细菌转化潜力。

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摘要

The long-term physical persistence and biological activity of transplastomic plant DNA (transgenes contained in the chloroplast genome) either purified and added to soil or naturally released by decaying tobacco leaves in soil was determined. Soil microcosms were amended with transplastomic tobacco leaves or purified plant DNA and incubated for up to 4 years. Total DNA was extracted from soil and the number of transgenes (aadA, which confers resistance to both spectinomycin and streptomycin) was quantified by quantitative PCR. The biological activity of these transgenes was assessed by transformation in the bacterial strain Acinetobacter sp. BD413(pBAB2) in vitro. While the proportion of transgenes recovered increased with the increasing amount of transplastomic DNA added, plant DNA was rapidly degraded over time. The number of transgenes recovered decreased about 10,000 fold within 2 weeks. Data reveal, however, that a small fraction of the plant DNA escaped degradation. Transgene sequences were still detected after 4 years and transformation assays showed that extracted DNA remained biologically active and could still transform competent cells of Acinetobacter sp. BD413(pBAB2). The approach presented here quantified the number of transgenes (based on quantitative PCR of 50% of the gene) released and persisting in the environment over time and provided new insights into the fate of transgenic plant DNA in soil.
机译:确定了纯化并添加到土壤中或通过腐烂的烟叶在土壤中自然释放的转质体植物DNA(叶绿体基因组中包含的转基因)的长期物理持久性和生物活性。用转基因烟草叶或纯化的植物DNA修改土壤微观世界,并孵育长达4年。从土壤中提取总DNA,并通过定量PCR定量转基因(aadA,赋予对壮观霉素和链霉素的抗性)的数量。这些转基因的生物活性通过在细菌菌株不动杆菌属中的转化来评估。 BD413(pBAB2)体外。尽管回收的转基因比例随添加的转基因组DNA的增加而增加,但植物DNA随时间迅速降解。在2周内,回收的转基因数量减少了约10,000倍。但是,数据表明,植物DNA的一小部分没有降解。 4年后仍检测到转基因序列,转化试验表明提取的DNA仍具有生物活性,并且仍可以转化不动杆菌属的感受态细胞。 BD413(pBAB2)。本文介绍的方法定量了随时间推移释放并持续存在于环境中的转基因数量(基于50%的基因的定量PCR),并提供了对土壤中转基因植物DNA命运的新见解。

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