Dried Blood Spot Screening System for Spinal Muscular Atrophy with Allele-Specific Polymerase Chain Reaction and Melting Peak Analysis

脊髓性肌萎缩 SMN1型 聚合酶链反应 干血斑 等位基因 生物 干血 多重聚合酶链反应 新生儿筛查 医学 实时聚合酶链反应 形状记忆合金* 遗传学 基因 化学 色谱法 组合数学 数学
作者
Yogik Onky Silvana Wijaya,Hisahide Nishio,Emma Tabe Eko Niba,Tomoyoshi Shiroshita,Masako Kato,Yoshihiro Bouike,Chisato Tode,Mawaddah Ar Rochmah,Nur Imma Fatimah Harahap,Dian Kesumapramudya Nurputra,Katsushi Okamoto,Toshio Saitô,Atsuko Takeuchi,Poh San Lai,Seiji Yamaguchi,Masakazu Shinohara
出处
期刊:Genetic Testing and Molecular Biomarkers [Mary Ann Liebert]
卷期号:25 (4): 293-301 被引量:3
标识
DOI:10.1089/gtmb.2020.0312
摘要

Background and Aim: Spinal muscular atrophy (SMA) is a lower motor neuron disease with autosomal recessive inheritance caused by homozygous SMN1 deletions. Although SMA has been considered as incurable, newly developed drugs improve life prognoses and motor functions of patients. To maximize the efficacy of the drugs, SMA patients should be treated before symptoms become apparent. Thus, newborn screening for SMA is strongly recommended. In this study, we aimed to establish a new simple screening system based on DNA melting peak analysis. Materials and Methods: A total of 124 dried blood spot (DBS) on FTA® ELUTE cards (51 SMN1-deleted patients with SMA, 20 carriers, and 53 controls) were punched and subjected to direct amplification of SMN1 and CFTR (reference gene). Melting peak analyses were performed to detect SMN1 deletions from DBS samples. Results: A combination of allele-specific polymerase chain reaction (PCR) and melting peak analyses clearly distinguished the DBS samples with and without SMN1. Compared with the results of fresh blood samples, our new system yielded 100% sensitivity and specificity. The advantages of our system include (1) biosafe collection, transfer, and storage for DBS samples, (2) obviating the need for DNA extraction from DBS preventing contamination, (3) preclusion of fluorescent probes leading to low PCR cost, and (4) fast and high-throughput screening for SMN1 deletions. Conclusion: We demonstrate that our system would be applicable to a real-world newborn screening program for SMA, because our new technology is efficient for use in routine clinical laboratories that do not have highly advanced PCR instruments.
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