Bizouarn Francisco
Gene Expression Division, Bio-Rad Laboratories, 2000 Alfred Nobel Dr., Hercules, CA, 94547, USA,
Methods Mol Biol. 2014;1160:189-214. doi: 10.1007/978-1-4939-0733-5_16.
Molecular diagnostics and disease-specific tailored treatments are now being introduced to patients at many hospitals and clinics throughout the world (Strain and Richman, Curr Opin HIV AIDS 8:106-110, 2013) and becoming prevalent in the nonscientific literature. Instead of generically using a "one treatment fits all" approach that may have varying levels of effectiveness to different patients, patient-specific molecular profiling based on the genetic makeup of the disease and/or a more accurate pathogen titer could provide more effective treatments with fewer unwanted side effects. One commonly known example of this scenario is epidermal growth factor receptor (EGFR). EGFR is upregulated in many cancers, including many lung and colorectal cancers. Commonly used treatments for these include the receptor blockers cetuximab or panitumumab and tyrosine kinase inhibitors erlotinib or gefitinib. These agents are effective at reducing out-of-control cell cycling and tumor proliferation, but only if downstream signaling kinases and phosphatases are not mutated. Known oncogenes such as BRAF V600E and KRAS G12/13 that are constitutively activated render these treatments ineffective. The use of known ineffective drugs and treatments can thus be avoided reducing time to more effective treatments, reducing cost, and increasing patient well-being. Although digital PCR is for all practical purposes a "new" technology, there is already tremendous interest in its potential for the clinical diagnostics arena. Specificity of the information acquired, accuracy of results, time to results, and cost per sample analyzed are making dPCR an attractive tool for this field. Three areas where dPCR will have a noticeable impact are pathogen/viral detection and quantitation, copy number variations, and rare mutation detection and abundance, but it will inevitably expand from these as the technology becomes more and more prevalent. This chapter discusses digital PCR assay optimization and validation, pathogen/viral detection and quantitation, copy number variation, and rare mutation abundance assays. The sample methods described below utilize the QX100/QX200 methodologies, but with the exception of reaction sub-partitioning (dependent on the instrumentation used) most other parameters remain the same.
目前,分子诊断和针对特定疾病的个性化治疗正在世界各地的许多医院和诊所应用于患者(斯特林和里奇曼,《当前艾滋病病毒与艾滋病观点》8:106 - 110,2013年),并在非科学文献中变得普遍。不再采用可能对不同患者有不同效果水平的“一刀切”治疗方法,基于疾病基因构成和/或更准确病原体滴度的患者特异性分子分析可以提供更有效的治疗,且副作用更少。这种情况一个广为人知的例子是表皮生长因子受体(EGFR)。EGFR在许多癌症中上调,包括许多肺癌和结直肠癌。针对这些癌症常用的治疗方法包括受体阻滞剂西妥昔单抗或帕尼单抗以及酪氨酸激酶抑制剂厄洛替尼或吉非替尼。这些药物在减少失控的细胞周期和肿瘤增殖方面有效,但前提是下游信号激酶和磷酸酶没有突变。诸如BRAF V600E和KRAS G12/13等已知的癌基因如果持续激活会使这些治疗无效。因此,可以避免使用已知无效的药物和治疗方法,从而缩短获得更有效治疗的时间、降低成本并提高患者的健康水平。尽管数字PCR实际上是一项“新技术”,但它在临床诊断领域的潜力已经引起了极大的关注。所获取信息的特异性、结果的准确性、获得结果的时间以及每个分析样本的成本,使得数字PCR成为该领域一个有吸引力的工具。数字PCR将产生显著影响的三个领域是病原体/病毒检测和定量、拷贝数变异以及罕见突变检测和丰度,但随着该技术越来越普及,其应用范围不可避免地会从这些领域扩展。本章讨论数字PCR检测的优化和验证、病原体/病毒检测和定量、拷贝数变异以及罕见突变丰度检测。以下所述的样本方法采用了QX100/QX200方法,但除了反应子分区(取决于所使用的仪器)外,大多数其他参数保持不变。
