评价AS—LNA—qPCR法检测JAK2V617F突变率的临床应用价值

A novel modification of real-time AS-qPCR by using locked nucleic acid-modified oligonucleotide probe as wild type allele amplification blockers for quantitative detection of the JAK2 V617F mutation

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摘要目的建立一种定量检测外周血细胞酪氨酸激酶2（JAK2）基因V617F突变率的等位基因特异性实时荧光定量PCR（AS＋qPCR）方法。方法在AS—qPCR基础上，引入l条锁核酸（LNA）修饰的寡核苷酸探针，用以选择性抑制AS—qPCR中突变引物对野生等位基因的非特异性扩增，定量检测JAK2V617F突变率，称之为AS—LNA—qPCR法。通过AS—LNA—qPCR法测定样本的循环阈值（ct值），根据AS．LNA—qPCR法检测不同JAK2V617F突变率标准品的ct值，绘制标准曲线，根据标准曲线直接获得检测样本中JAK2V617F突变率。我们对该方法标准品的批内、批问检测结果进行了评价，并对623名表观健康人外周血细胞基因组DNA中JAK2V617F突变进行检测，以探讨其临床应用价值。结果AS—LNA—qPCR法定量检测JAK2V617F突变率的下限可达到0．01％，批内、批问平均变异率分别是6．3％和8．6％。对623名表观健康人外周血细胞基因组DNA中JAK2V617F突变检测显示，其中19名（3％）表现健康人JAK2V617F突变阳性，突变率变化范围为0．01％～5．49％。结论AS—LNA—qPCR方法直接定量检测外周血细胞JAK2V617F突变率，具有检测灵敏度高和重复性好的特性，适合临床上用于对骨髓增殖性疾病诊断、疾病进程评估和疗效的监测。 Objective To develop a novel real-time PCR for sensitively quantitative detection of JAK2 V617F allele burden in peripheral blood. Methods Based on the real-time allele-specific PCR （ AS-qPCR）, the locked nucleic acid （LNA） -modified oligonucleotide probe was used for selectively blocking amplification of wild-type alleles in AS-qPCR, and then a novel AS-LNA-qPC.R method was established. The percentages of sample JAK2 V617F alleles were directly calculated by its threshold cycle （Ct） values according to the standard curve which generated by JAK2 V617F alleles with its Ct values. We validated intra- and inter-assay variability for quantifying JAK2 V617F. We also assayed 623 apparent healthy donors by our method to validate its clinical application value. Results The quantitative lower limit of this method for JAK2 V617F was 0.01% , and the intra- and inter-assay average variability for quantifying percentage of JAK2 V617F in total DNA was 6.3% and 8.6%, respectively. Nineteen JAK2 V617F-positive individuals were identified using AS-LNA-qPCR in blood of 623 apparently healthy donors, and the range of percentages of JAK2 V617F alleles were 0.01% - 5.49%. Conclusion The AS-LNA-qPCR with highly sensitive and reproducible quantification of JAK2 V617F mutant burden can be used clinically for diagnosis as well as evaluation of disease prognosis and efficacy of therapy in patients with myeloproliferative neoplasms.

作者邵冬华梁国威何美琳曹清芸

机构地区航天中心医院检验科

出处《中华血液学杂志》 CAS CSCD 北大核心 2013年第5期421-425,共5页 Chinese Journal of Hematology

关键词基因 JAK2 DNA突变分析骨髓增殖性疾病聚合酶链反应锁核酸 Gene, JAK2 DNA mutation analysis Myeloproliferative neoplasms Polymerasechain reaction Allele-specific PCR Locked nucleic acid

分类号 R4 [医药卫生—临床医学] R5 [医药卫生—内科学]

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评价AS—LNA—qPCR法检测JAK2V617F突变率的临床应用价值

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