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DNA微阵列检测与信号放大方法的比较

Comparison of detection and signal amplification methods for DNA microarrays.

作者信息

Vora Gary J, Meador Carolyn E, Anderson George P, Taitt Chris Rowe

机构信息

Center for Bio/Molecular Science & Engineering, Naval Research Laboratory, Washington, DC 20375, USA.

出版信息

Mol Cell Probes. 2008 Oct-Dec;22(5-6):294-300. doi: 10.1016/j.mcp.2008.07.002. Epub 2008 Jul 16.

Abstract

One of the factors limiting the use of DNA microarray technology for the detection of pathogenic organisms from clinical and environmental matrices has been inadequate assay sensitivity. To assess the effectiveness of post-hybridization secondary detection steps to enhance the sensitivity of DNA microarray-based pathogen detection, we evaluated a panel of 11 commercial and novel hybridization detection and signal amplification methods (direct labeling, indirect aminoallyl labeling, antibody, DNA dendrimers, viral particles, internally fluorescent nanoparticles, tyramide signal amplification, resonance light scattering nanoparticles and quantum dots) using a multiplex PCR and spotted long oligonucleotide microarray for Vibrio cholerae. Quantitative parameters such as sensitivity, signal intensity, background, assay complexity, time and cost were assessed and provide comparative criteria to be considered for DNA microarray experimental design. While the most important parameter is likely to vary based on the assay, when weighted equally, the findings suggest that recognition element- and dye-functionalized viral particles provide the most attractive option for microarray detection and signal amplification.

摘要

限制DNA微阵列技术用于从临床和环境样本中检测致病生物体的因素之一是检测灵敏度不足。为了评估杂交后二次检测步骤提高基于DNA微阵列的病原体检测灵敏度的有效性,我们使用多重PCR和霍乱弧菌斑点长寡核苷酸微阵列,评估了11种商业和新型杂交检测及信号放大方法(直接标记、间接氨基烯丙基标记、抗体、DNA树枝状大分子、病毒颗粒、内部荧光纳米颗粒、酪胺信号放大、共振光散射纳米颗粒和量子点)。评估了灵敏度、信号强度、背景、检测复杂性、时间和成本等定量参数,并为DNA微阵列实验设计提供了可考虑的比较标准。虽然最重要的参数可能因检测方法而异,但在同等加权时,研究结果表明,识别元件和染料功能化的病毒颗粒为微阵列检测和信号放大提供了最具吸引力的选择。

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