数字液滴聚合酶链式反应与定量聚合酶链式反应在脂蛋白(a)环IV型2重复多态性遗传表征中的比较。

IF 2.6 4区 医学 Q2 MEDICAL LABORATORY TECHNOLOGY Journal of Clinical Laboratory Analysis Pub Date : 2024-03-05 DOI:10.1002/jcla.24998
Giulia Barbieri, Giulia Cassioli, Ada Kura, Rebecca Orsi, Alberto Magi, Martina Berteotti, Giusi Maria Scaturro, Elena Lotti, Anna Maria Gori, Rossella Marcucci, Betti Giusti, Elena Sticchi
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引用次数: 0

摘要

背景:脂蛋白(a)[Lp(a)]水平的变异与动脉粥样硬化血栓风险的增加有关,主要归因于编码脂蛋白(a)的 LPA 基因,而 Kringle IV 2 型(KIV2)拷贝数变异(CNV)是主要的遗传决定因素。脂蛋白(a)的遗传特征正在不断增加;然而,这种变体的特殊结构特征对开发有效的检测方法构成了重大挑战。本研究旨在比较定量实时 PCR(qPCR)和数字液滴 PCR(ddPCR)在评估 KIV2 重复多态性方面的作用:我们分析了 100 名接受心血管风险检测的受试者,并对其血浆脂蛋白(a)水平进行了评估:结果:两种方法获得的 CNV 值之间的相关性分析略有显著性(R = 0.413,p = 0.00002),这是因为 qPCR 与 ddPCR 相比数据分散性更大。在不同实验过程中进行的内部对照 C1、C2 和 C3 测量显示,ddPCR 具有更高的稳定性,与 qPCR 相比,该方法测定的测定内/测定间变异系数更小,也证明了这一点。两种技术都证实了脂蛋白(a)水平与 CNV 值之间存在明显的反相关性,但用 ddPCR 评估的相关性高于 qPCR(分别为 R = -0.393,p = 0.000053;R = -0.220,p = 0.028)。当根据 500 mg/L Lp(a) 临界值将受试者分为两组时,Lp(a) 水平较高的受试者的 KIV2 重复数明显较低,ddPCR 比 qPCR 的证据更充分(分别为 p = 0.000013 和 p = 0.001):获得的数据支持 ddPCR 在评估 KIV2 重复序列多态性方面具有更好的性能。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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Digital droplet PCR versus quantitative PCR for lipoprotein (a) kringle IV type 2 repeat polymorphism genetic characterization

Background

Lipoprotein(a) [Lp(a)] level variability, related to atherothrombotic risk increase, is mainly attributed to LPA gene, encoding apolipoprotein(a), with kringle IV type 2 (KIV2) copy number variation (CNV) acting as the primary genetic determinant. Genetic characterization of Lp(a) is in continuous growth; nevertheless, the peculiar structural characteristics of this variant constitute a significant challenge to the development of effective detection methods. The aim of the study was to compare quantitative real-time PCR (qPCR) and digital droplet PCR (ddPCR) in the evaluation of KIV2 repeat polymorphism.

Methods

We analysed 100 subjects tested for cardiovascular risk in which Lp(a) plasma levels were assessed.

Results

Correlation analysis between CNV values obtained with the two methods was slightly significant (R = 0.413, p = 0.00002), because of the wider data dispersion in qPCR compared with ddPCR. Internal controls C1, C2 and C3 measurements throughout different experimental sessions revealed the superior stability of ddPCR, which was supported by a reduced intra/inter-assay coefficient of variation determined in this method compared to qPCR. A significant inverse correlation between Lp(a) levels and CNV values was confirmed for both techniques, but it was higher when evaluated by ddPCR than qPCR (R = −0.393, p = 0.000053 vs R = −0.220, p = 0.028, respectively). When dividing subjects into two groups according to 500 mg/L Lp(a) cut-off value, a significantly lower number of KIV2 repeats emerged among subjects with greater Lp(a) levels, with stronger evidence in ddPCR than in qPCR (p = 0.000013 and p = 0.001, respectively).

Conclusions

Data obtained support a better performance of ddPCR in the evaluation of KIV2 repeat polymorphism.

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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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