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Quantitative screening of single copies of human papilloma viral DNA without amplification

机译:无需扩增即可定量筛选人乳头瘤病毒DNA的单拷贝

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摘要

We describe a novel quantitative viral screening method based on single-molecule detection that does not require amplification. DNA of human papilloma virus (HPV), the major etiological agent of cervical cancer, served as the screening target in this study. Eight 100-nucleotide single-stranded DNA probes were designed complementary to the E6-E7 gene of HPV-16 DNA. The probes were covalently stained with Alexa Fluor 532 and hybridized to the target in solution. The individual hybridized molecules were imaged with an intensified charge-coupled device (ICCD) in two ways. In the single-color mode, target molecules were detected via fluorescence from hybridized probes only. This system could detect HPV-16 DNA in the presence of human genomic DNA down to 0.7 copy/ cell and had a linear dynamic range of over 6 orders of magnitude. In the dual-color mode, we employed fluorescence resonance energy transfer and added YOYO-3 dye as the acceptor. The two colors from Alexa Fluor 532 and YOYO-3 were dispersed by a transmission grating located in front of the ICCD. With this reinforced criterion for identifying the hybridized molecules, zero false-positive count was achieved. We also showed that DNA extracts from Pap test specimens did not interfere with the measurements.
机译:我们描述了一种基于单分子检测的新型定量病毒筛选方法,该方法不需要扩增。宫颈癌的主要病因是人乳头瘤病毒(HPV)的DNA,是本研究的筛选目标。设计了八个与HPV-16 DNA的E6-E7基因互补的100个核苷酸的单链DNA探针。探针用Alexa Fluor 532共价染色,并与溶液中的靶标杂交。单个杂交分子用增强电荷耦合器件(ICCD)两种方式成像。在单色模式下,仅通过杂交探针的荧光检测靶分子。该系统可以在存在人类基因组DNA的情况下(低至0.7个拷贝/细胞)检测HPV-16 DNA,并具有超过6个数量级的线性动态范围。在双色模式下,我们采用了荧光共振能量转移并添加了YOYO-3染料作为受体。 Alexa Fluor 532和YOYO-3的两种颜色由位于ICCD前面的透射光栅分散。利用这种用于鉴定杂交分子的增强标准,实现了零假阳性计数。我们还表明,从巴氏测试标本中提取的DNA不会干扰测量。

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