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Chemiluminescent bead-based hybridization assay for the detection of genomic DNA from E. coli in purified plasmid samples

机译:基于化学发光珠的杂交检测,可从纯化的质粒样品中检测大肠杆菌的基因组DNA

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摘要

A bead-based hybridization assay was developed for detection of traces of E. coli genomic DNA (gDNA) present in purified plasmid DNA (pDNA) samples. Standards of gDNA and pDNA samples were sheared by sonication and adsorbed onto aminopropyl controlled pore glass (CPG) particles (130 μm). A preliminary study was conducted to optimize the amount of DNA adsorbed on the particles. Results indicated that maximum attachment efficiency was obtained by adsorbing DNA for 2 h in 0.2 × SSC, pH 5.7. The DNA-bound particles were hybridized overnight with a 181-bp digoxigenin-labeled probe, specific for gDNA. Following a chemiluminescent detection protocol, signal intensities of the standards were plotted as a function of initial gDNA concentration. The calculated detection limit (LOD) was 1.4 pM of gDNA. The assay was able to detect gDNA in pure plasmid preparations at the 1% level even in the presence of 1,000-fold excess of noncomplementary target. Hybridization results were compared with a quantitative real-time PCR assay. Both methods afforded similar accurate results at the 95% confidence level.
机译:开发了一种基于珠的杂交测定法,用于检测纯化的质粒DNA(pDNA)样品中存在的痕量大肠杆菌基因组DNA(gDNA)。 gDNA和pDNA样品的标准品通过超声剪切并吸附到氨丙基可控孔玻璃(CPG)颗粒(130μm)上。进行了初步研究,以优化吸附在颗粒上的DNA量。结果表明,通过在0.2×SSC,pH 5.7中吸附DNA 2 h可获得最大的附着效率。将与DNA结合的颗粒与对gDNA特异的181-bp地高辛配基标记的探针杂交过夜。按照化学发光检测方案,将标准品的信号强度绘制为初始gDNA浓度的函数。计算的检测限(LOD)为1.4 pM gDNA。该测定法即使在存在1,000倍过量的非互补靶标的情况下也能够以1%的水平检测纯质粒制剂中的gDNA。将杂交结果与实时定量PCR分析进行比较。两种方法在95%的置信度下都提供了相似的准确结果。

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  • 来源
    《Analytical and Bioanalytical Chemistry》 |2008年第6期|2179-2187|共9页
  • 作者单位

    Institute for Biotechnology and Bioengineering Centre for Biological and Chemical Engineering Instituto Superior Técnico Av. Rovisco Pais 1049-001 Lisbon Portugal;

    Institute for Biotechnology and Bioengineering Centre for Biological and Chemical Engineering Instituto Superior Técnico Av. Rovisco Pais 1049-001 Lisbon Portugal;

    Institute for Biotechnology and Bioengineering Centre for Biological and Chemical Engineering Instituto Superior Técnico Av. Rovisco Pais 1049-001 Lisbon Portugal;

    Institute for Biotechnology and Bioengineering Centre for Biological and Chemical Engineering Instituto Superior Técnico Av. Rovisco Pais 1049-001 Lisbon Portugal;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    Genomic DNA; CPG microparticles; Hybridization; Chemiluminescence; Plasmid;

    机译:基因组DNA;CPG微粒;杂交;化学发光;质粒;

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