[Application of PCR reverse dot blot in non-syndromic deafness gene detection]

Yalan Liu; Shushan Sang; Jie Ling; Chufeng He; Lingyun Mei; Yong Feng

doi:10.13201/j.issn.1001-1781.2020.02.013

[Application of PCR reverse dot blot in non-syndromic deafness gene detection]

Lin Chuang Er Bi Yan Hou Tou Jing Wai Ke Za Zhi. 2020 Feb;34(2):153-157. doi: 10.13201/j.issn.1001-1781.2020.02.013.

[Article in Chinese]

Authors

Yalan Liu^{1

2}, Shushan Sang^{1

2}, Jie Ling³, Chufeng He^{1

2}, Lingyun Mei^{1

2}, Yong Feng^{1

2}

Affiliations

¹ Department of Otolaryngology Head and Neck Surgery，Xiangya Hospital，Central South University，Changsha，410008，China.
² Xiangya Hospital，Central South University，Province Key Laboratory of Otolaryngology Critical Diseases.
³ Institute of Molecular Precision Medicine，Xiangya Hospital，Central South University.

PMID: 32086922
PMCID: PMC10128405
DOI: 10.13201/j.issn.1001-1781.2020.02.013

Abstract
in English, Chinese

Objective:To detect 20 common deafness gene mutations in non- syndromic deafness patients in China using PCR- RDB, and analyze and summarize the mutation data to explore the clinical value of this method. Method:The PCR- RDB and Sanger sequencing were used to detect 20 common mutations of four deafness genes（GJB2, GJB3, SLC26A4 and mtDNA） in 500 patients with non- syndromic hearing loss . The Sanger sequencing was used to compare the sensitivity, specificity, positive predictive value, negative predictive value, and total coincidence rate of the deafness mutation detected by PCR- RDB. Result:A total of 500 samples were detected. 147 wild- type samples, 81 homozygous mutant samples, 240 heterozygous mutant samples, 32 composite heterozygous mutant samples were detected using the PCR- RDB within the range of 20 gene mutations, which were identical to the Sanger sequencing results. GJB2 c.235delC and SLC26A4 c.919- 2 A>G are the most common hotspot mutations in this study, followed by mtDNA m. 1555 A>G. Compared with the Sanger sequencing method, the sensitivity, specificity, positive predictive value, negative predictive value, and total coincidence rate of the real- time fluorescence PCR melting curve method were 100%, and the Kappa value was one. Conclusion:PCR reverse dot-blot hybridization is a simple, rapid, sensitive and specific method for detecting 20 mutations of 4 common deafness genes in Chinese population, it is expected to be used in clinical detection of deafness genes in the future.

目的：在中国非综合征型遗传性聋患者人群中，采用PCR-反向点杂交法检测涵盖中国人群常见4个耳聋基因的20种基因突变，分析总结突变数据，探讨该方法在遗传性聋基因检测中的临床实用价值。 方法：分别采用PCR-反向点杂交法和Sanger测序法，对500例非综合征型遗传性聋患者行4个耳聋相关基因（GJB2、GJB3、SLC26A4和mtDNA）共20种突变检测。以Sanger测序法结果为金标准，探讨PCR-反向点杂交法检测耳聋突变的阳性符合率、阴性符合率、总符合率、灵敏度、特异性、阳性预测值和阴性预测值等检测性能指标。 结果：共检测500例样本，在20种基因突变的突变型范围内，使用PCR-反向点杂交法检出147例野生型样本，81例纯合突变型样本，240例杂合突变型样本，32例复合杂合突变型样本，与Sanger测序法结果完全一致。GJB2 c.235delC和SLC26A4 c.919-2 A>G是本研究中最为常见的热点突变，其次是mtDNA m.1555 A>G。对比Sanger测序法，PCR-反向点杂交法检测20个耳聋基因突变位点的灵敏度（阳性符合率）、特异性（阴性符合率）、阳性预测值、阴性预测值、总符合率均为100%，Kappa值为1。 结论：PCR-反向点杂交法用于耳聋基因突变的检测，具有简便、快速、灵敏度高、特异性强等优点，可准确检出中国人群常见4个耳聋基因的20种基因突变的突变型，将来有望用于耳聋基因的临床检测。.

Keywords: PCR; gene mutation; hereditary deafness; molecular hybridization.

MeSH terms

China
Connexin 26
Connexins / genetics
DNA Mutational Analysis*
DNA, Mitochondrial / genetics
Deafness / genetics*
Humans
Mutation
Polymerase Chain Reaction
Sulfate Transporters / genetics

Substances

Connexins
DNA, Mitochondrial
GJB2 protein, human
SLC26A4 protein, human
Sulfate Transporters
Connexin 26
GJB3 protein, human

Abstract in English, Chinese

MeSH terms

Substances

Abstract
in English, Chinese