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首页> 外文期刊>Clinical Chemistry: Journal of the American Association for Clinical Chemists >Quantitative polymerase chain reaction-based homogeneous assay with fluorogenic probes to measure c-erbB-2 oncogene amplification
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Quantitative polymerase chain reaction-based homogeneous assay with fluorogenic probes to measure c-erbB-2 oncogene amplification

机译:基于荧光定量探针的基于聚合酶链反应的均相测定以测量c-erbB-2癌基因扩增

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We describe a PCR-based assay for determining c- erb B-2 oncogene amplification in breast cancer in which we use the TaqManTM system. Two fluorogenic probes anneal to the target between primers for c- erb B-2 and β-globin genes and contain both a reporter dye (6-carboxy-fluorescein) and a quencher dye (6-carboxy-tetramethyl-rhodamine). During the extension phase of the PCR cycle, the 5′→3′ exonuclease activity of Taq polymerase cleaves the hybridized fluorogenic probe, resulting in an increase of fluorescence emission of the reporter dye that is quantitative for the amount of PCR product and, under appropriate conditions, for the amount of template. Assay performance showed adequate precision and a lower detection limit and good correlation with the results obtained in the same samples by a competitive PCR assay (n = 25, r = 0.94, P 0.01). This homogeneous assay is time-saving, avoids usually cumbersome postamplification procedures (that can be additional sources of inaccuracy and contamination), and seems suitable for determination of c- erb B-2 oncogene amplification in tumor specimens.
机译:我们描述了一种基于PCR的测定方法,用于确定使用TaqManTM系统的乳腺癌中c-erb B-2癌基因的扩增。两个荧光探针与C-erb B-2和β-珠蛋白基因的引物之间的靶标退火,并且既包含报告染料(6-羧基荧光素)又包含淬灭染料(6-羧基-四甲基罗丹明)。在PCR循环的延伸阶段,Taq聚合酶的5'→3'核酸外切酶活性裂解了杂交的荧光探针,导致报告染料的荧光发射增加,该染料的定量对于PCR产物的量是适当的,并且在适当的条件下条件,用于模板的数量。测定性能显示出足够的精密度和较低的检出限,并且与竞争性PCR测定法在相同样品中获得的结果具有良好的相关性(n = 25,r = 0.94,P <0.01)。这种均相测定节省了时间,避免了通常繁琐的扩增后步骤(这可能是不准确和污染的其他来源),并且似乎适合于测定肿瘤标本中的c-erb B-2癌基因扩增。

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