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基于光纤纳米金连接吸附剂检测的游离胎儿 DNA 无创性产前基因筛查在β-地中海贫血早期预测中的应用。

Noninvasive Prenatal Genetic Screening of Cell-Free Fetal DNA for Early Prediction of β-Thalassemia Using Fiber Optic Nanogold-Linked Sorbent Assay.

机构信息

Department of Chemistry and Biochemistry, National Chung Cheng University, 168 University Rd., Minhsiung, Chiayi 621301, Taiwan.

School of Dentistry, Institute of Oral Medicine, National Cheng Kung University, 138 Shengli Rd., North District, Tainan City 704, Taiwan.

出版信息

ACS Sens. 2024 Aug 23;9(8):4207-4215. doi: 10.1021/acssensors.4c01194. Epub 2024 Aug 1.

DOI:10.1021/acssensors.4c01194
PMID:39088458
Abstract

β-Thalassemia is a prevalent type of severe inherited chronic anemia, primarily identified in developing countries. The identification of single nucleotide polymorphisms (SNPs) plays a vital role in the early diagnosis of genetic diseases. Here, we reported the development of an amplification-free fiber optic nanogold-linked sorbent assay method using a fiber optic particle plasmon resonance (FOPPR) biosensor for rapid and ultrasensitive detection of SNPs. Herein, MutS protein was selected as the biorecognition capture probe and immobilized on the sensing region to capture the target mutant DNA, which was hybridized with a single-base mismatched single-stranded DNA labeled by a gold nanoparticle (AuNP). The AuNP acts as a signaling agent to be detected by the FOPPR biosensor when it is bound on the fiber core surface. The method effectively differentiates mismatched double-stranded DNA by MutS protein from perfectly matched/complementary dsDNA. It exhibits an impressively low detection limit for the detection of SNPs at approximately 10 M using low-cost sensor chips and devices. By determination of the ratio of mutant DNA to normal DNA in cell-free genomic DNA from blood samples, this method is promising for diagnosing β-thalassemia in fetuses without invasive testing techniques.

摘要

β-地中海贫血是一种常见的严重遗传性慢性贫血,主要在发展中国家发现。单核苷酸多态性 (SNP) 的鉴定在遗传病的早期诊断中起着至关重要的作用。在这里,我们报告了一种无扩增光纤纳米金连接吸附剂测定法的开发,该方法使用光纤粒子等离子体共振 (FOPPR) 生物传感器,用于快速和超灵敏检测 SNP。在这里,MutS 蛋白被选为生物识别捕获探针,并固定在传感区域以捕获靶突变 DNA,该 DNA 与用金纳米颗粒 (AuNP) 标记的单碱基错配单链 DNA 杂交。当 AuNP 结合在光纤芯表面上时,它充当信号剂,可被 FOPPR 生物传感器检测到。该方法通过 MutS 蛋白有效地从完全匹配/互补的 dsDNA 中区分错配的双链 DNA。它使用低成本的传感器芯片和设备,对 SNP 的检测具有令人印象深刻的低检测限,约为 10M。通过确定来自血液样本的无细胞基因组 DNA 中突变型 DNA 与正常 DNA 的比例,该方法有望用于诊断胎儿的β-地中海贫血,而无需侵入性检测技术。

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