Expanded molecular detection of MPL codon p.W515 and p.S505N mutations in myeloproliferative neoplasms.

IF 2.6 4区 医学 Q2 MEDICAL LABORATORY TECHNOLOGY
Journal of Clinical Laboratory Analysis Pub Date : 2023-12-01 Epub Date: 2023-12-07 DOI:10.1002/jcla.24992
Eric W Miller, Celeste M Lamberson, Ratilal R Akabari, Michel R Nasr, Steven M Sperber
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引用次数: 0

Abstract

Background: Patients negative for the JAK2 p.V617F somatic variant are frequently reflexed to testing for MPL exon 10 variants. Detection of these variants via multiplexed allele-specific PCR followed by fragment analysis has been previously published. The present study builds on this concept by improving the detection of the p.W515A variant, adding a second allele-specific primer to detect the p.W515R variant, and incorporating an improved primer for p.S505N detection.

Methods: The W515 amplification employs 5'-labeled allele-specific forward primers to detect p.W515K, p.W515L, p.W515R, and p.W515A. The p.S505N amplification includes an allele-specific reverse primer with a tail extension. Fragments were subject to capillary electrophoresis on an ABI 3500 Genetic Analyzer and analyzed using GeneMapper 6.0 (Thermo Fisher Scientific).

Results: Thirty MPL-negative and 13 MPL-positive samples previously tested by a reference laboratory were tested with the MPL LDT. Results were 100% concordant. The MPL LDT has a limit of detection of at least 5% VAF for the p.W515 variants and 10% VAF for the p.S505N variant.

Conclusion: Current MPL assays are predominantly focused on p.W515L/K and p.S505N mutations. We have engineered an MPL test for detecting p.W515A/L/K/R and p.S505N variants, thereby increasing the diagnostic yield with little additional expense or technician time.

Abstract Image

MPL密码子p.W515和p.S505N突变在骨髓增长性肿瘤中的扩展分子检测。
背景:JAK2 p.V617F体细胞变异体阴性的患者经常对MPL外显子10变异体进行检测。通过多重等位基因特异性PCR检测这些变异,然后进行片段分析已经发表。本研究在此基础上改进了p.W515A变异的检测,增加了第二个等位基因特异性引物来检测p.W515R变异,并结合了一个改进的引物来检测p.S505N。方法:W515扩增采用5′标记等位基因特异性正向引物检测p.W515K、p.W515L、p.W515R和p.W515A。p.S505N扩增包括一个带有尾部延伸的等位基因特异性反向引物。片段在ABI 3500遗传分析仪上进行毛细管电泳,使用GeneMapper 6.0 (Thermo Fisher Scientific)进行分析。结果:30个MPL阴性和13个MPL阳性样本先前在参考实验室检测,用MPL LDT检测。结果100%一致。MPL LDT对p.W515型和p.S505N型具有至少5% VAF和10% VAF的检测极限。结论:目前的MPL检测主要集中在p.W515L/K和p.S505N突变。我们设计了一种MPL测试,用于检测p.W515A/L/K/R和p.S505N变体,从而在几乎没有额外费用或技术人员时间的情况下提高了诊断率。
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来源期刊
Journal of Clinical Laboratory Analysis
Journal of Clinical Laboratory Analysis 医学-医学实验技术
CiteScore
5.60
自引率
7.40%
发文量
584
审稿时长
6-12 weeks
期刊介绍: Journal of Clinical Laboratory Analysis publishes original articles on newly developing modes of technology and laboratory assays, with emphasis on their application in current and future clinical laboratory testing. This includes reports from the following fields: immunochemistry and toxicology, hematology and hematopathology, immunopathology, molecular diagnostics, microbiology, genetic testing, immunohematology, and clinical chemistry.
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