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一种用于筛查中国人群中与非综合征性听力损失相关的四个基因中的二十种突变的反向斑点杂交检测法。

A reverse dot blot assay for the screening of twenty mutations in four genes associated with NSHL in a Chinese population.

作者信息

Li Siping, Peng Qi, Liao Shengyun, Li Wenrui, Ma Qiang, Lu Xiaomei

机构信息

Department of Laboratory, Dongguan Children's Hospital, Dongguan, Guangdong, China.

Department of Medical and Molecular Genetics, Dongguan Institute of Pediatrics, Dongguan, Guangdong, China.

出版信息

PLoS One. 2017 May 15;12(5):e0177196. doi: 10.1371/journal.pone.0177196. eCollection 2017.

DOI:10.1371/journal.pone.0177196
PMID:28505178
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5432070/
Abstract

BACKGROUND

Congenital deafness is one of the most distressing disorders affecting humanity and exhibits a high incidence worldwide. Most cases of congenital deafness in the Chinese population are caused by defects in a limited number of genes. A convenient and reliable method for detecting common deafness-related gene mutations in the Chinese population is required.

METHODS

We developed a PCR-reverse dot blot (RDB) assay for screening 20 hotspot mutations of GJB2, GJB3, SLC26A4, and MT-RNR1, which are common non-syndromic hearing loss (NSHL)-associated genes in the Chinese population. The PCR-RDB assay consists of multiplex PCR amplifications of 10 fragments in the target sequence of the four above-mentioned genes in wild-type and mutant genomic DNA samples followed by hybridization to a test strip containing allele-specific oligonucleotide probes. We applied our method to a set of 225 neonates with deafness gene mutations and 30 normal neonates.

RESULTS

The test was validated through direct sequencing in a blinded study with 100% concordance.

CONCLUSIONS

The results demonstrated that our reverse dot blot assay is a reliable and effective genetic screening method for identifying carriers and individuals with NSHL among the Chinese population.

摘要

背景

先天性耳聋是影响人类的最令人痛苦的疾病之一,在全球范围内发病率很高。中国人群中大多数先天性耳聋病例是由少数基因缺陷引起的。需要一种方便可靠的方法来检测中国人群中常见的与耳聋相关的基因突变。

方法

我们开发了一种聚合酶链反应-反向点杂交(PCR-RDB)检测方法,用于筛查GJB2、GJB3、SLC26A4和MT-RNR1的20个热点突变,这些是中国人群中常见的非综合征性听力损失(NSHL)相关基因。PCR-RDB检测方法包括对野生型和突变基因组DNA样本中上述四个基因的目标序列中的10个片段进行多重PCR扩增,然后与包含等位基因特异性寡核苷酸探针的测试条杂交。我们将我们的方法应用于一组225例患有耳聋基因突变的新生儿和30例正常新生儿。

结果

在一项盲法研究中通过直接测序验证了该检测方法,一致性为100%。

结论

结果表明,我们的反向点杂交检测方法是一种可靠有效的基因筛查方法,可用于在中国人群中识别NSHL携带者和个体。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b650/5432070/59fbd4bf7280/pone.0177196.g001.jpg

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