听力学及言语疾病杂志
聽力學及言語疾病雜誌
은역학급언어질병잡지
Journal of Audiology and Speech Pathology
2015年
6期
569-574
,共6页
伍丽东%唐宁%严提珍%李哲涛%李健鸿%李伍高%庞红%罗世强%邱琪
伍麗東%唐寧%嚴提珍%李哲濤%李健鴻%李伍高%龐紅%囉世彊%邱琪
오려동%당저%엄제진%리철도%리건홍%리오고%방홍%라세강%구기
非综合征型聋%易感基因%基因芯片%Sanger测序
非綜閤徵型聾%易感基因%基因芯片%Sanger測序
비종합정형롱%역감기인%기인심편%Sanger측서
Nonsyndromic hearing loss%Susceptibility gene%DNA microarray%Sanger sequencing
目的:应用基因芯片联合Sanger测序技术检测广西壮族自治区听力言语康复中心非综合征型聋患者的基因突变谱系及基因型,为基因诊断、遗传咨询及防聋治聋提供参考。方法对广西壮族自治区听力言语康复中心136例双侧重度及以上程度感音神经性非综合征型聋患儿采集外周血并提取基因组DNA ,用遗传性聋基因芯片对4个耳聋易感基因的9个突变位点(GJB2基因:c .35delG、c .235delC、c .176del16、c .299delAT ;GJB3基因:c .538C> T ;SLC26A4基因:c .919-2A> G、c .2168A> G ;mtDNA 12SrRNA 基因:m .1494C> T、m .1555A>G)进行分析。基因芯片技术未确诊的样本采用Sanger测序法进一步检测。结果通过基因芯片技术在20例聋儿中检出GJB2、SLC26A4和线粒体12SrRNA基因突变,总检出率为14.71%(20/136);结合Sanger测序技术,34例聋儿检出GJB2、SLC26A4和12SrRNA基因突变,总检出率为25%(34/136),发现6种基因芯片技术未检出的SLC26A4突变位点(c .259G> T、c .754C> T、c .1229C> T、c .1548_1549insC、c .1705+5A> G和c .2086C> T )。GJB2基因以c .235delC突变为主,SLC26A4基因以c .919-2A> G、c .754C> T 和c .1229C> T 为主;GJB2和SLC26A4基因突变者占本组病例基因突变总例数的38.24%(13/34)和58.82%(20/34)。结论基因芯片联合Sanger测序技术可以提高非综合征型聋患者基因突变的检出率;广西壮族自治区听力言语康复中心非综合征型聋患者热点突变基因以GJB2和SLC26A4基因为常见。
目的:應用基因芯片聯閤Sanger測序技術檢測廣西壯族自治區聽力言語康複中心非綜閤徵型聾患者的基因突變譜繫及基因型,為基因診斷、遺傳咨詢及防聾治聾提供參攷。方法對廣西壯族自治區聽力言語康複中心136例雙側重度及以上程度感音神經性非綜閤徵型聾患兒採集外週血併提取基因組DNA ,用遺傳性聾基因芯片對4箇耳聾易感基因的9箇突變位點(GJB2基因:c .35delG、c .235delC、c .176del16、c .299delAT ;GJB3基因:c .538C> T ;SLC26A4基因:c .919-2A> G、c .2168A> G ;mtDNA 12SrRNA 基因:m .1494C> T、m .1555A>G)進行分析。基因芯片技術未確診的樣本採用Sanger測序法進一步檢測。結果通過基因芯片技術在20例聾兒中檢齣GJB2、SLC26A4和線粒體12SrRNA基因突變,總檢齣率為14.71%(20/136);結閤Sanger測序技術,34例聾兒檢齣GJB2、SLC26A4和12SrRNA基因突變,總檢齣率為25%(34/136),髮現6種基因芯片技術未檢齣的SLC26A4突變位點(c .259G> T、c .754C> T、c .1229C> T、c .1548_1549insC、c .1705+5A> G和c .2086C> T )。GJB2基因以c .235delC突變為主,SLC26A4基因以c .919-2A> G、c .754C> T 和c .1229C> T 為主;GJB2和SLC26A4基因突變者佔本組病例基因突變總例數的38.24%(13/34)和58.82%(20/34)。結論基因芯片聯閤Sanger測序技術可以提高非綜閤徵型聾患者基因突變的檢齣率;廣西壯族自治區聽力言語康複中心非綜閤徵型聾患者熱點突變基因以GJB2和SLC26A4基因為常見。
목적:응용기인심편연합Sanger측서기술검측엄서장족자치구은력언어강복중심비종합정형롱환자적기인돌변보계급기인형,위기인진단、유전자순급방롱치롱제공삼고。방법대엄서장족자치구은력언어강복중심136례쌍측중도급이상정도감음신경성비종합정형롱환인채집외주혈병제취기인조DNA ,용유전성롱기인심편대4개이롱역감기인적9개돌변위점(GJB2기인:c .35delG、c .235delC、c .176del16、c .299delAT ;GJB3기인:c .538C> T ;SLC26A4기인:c .919-2A> G、c .2168A> G ;mtDNA 12SrRNA 기인:m .1494C> T、m .1555A>G)진행분석。기인심편기술미학진적양본채용Sanger측서법진일보검측。결과통과기인심편기술재20례롱인중검출GJB2、SLC26A4화선립체12SrRNA기인돌변,총검출솔위14.71%(20/136);결합Sanger측서기술,34례롱인검출GJB2、SLC26A4화12SrRNA기인돌변,총검출솔위25%(34/136),발현6충기인심편기술미검출적SLC26A4돌변위점(c .259G> T、c .754C> T、c .1229C> T、c .1548_1549insC、c .1705+5A> G화c .2086C> T )。GJB2기인이c .235delC돌변위주,SLC26A4기인이c .919-2A> G、c .754C> T 화c .1229C> T 위주;GJB2화SLC26A4기인돌변자점본조병례기인돌변총례수적38.24%(13/34)화58.82%(20/34)。결론기인심편연합Sanger측서기술가이제고비종합정형롱환자기인돌변적검출솔;엄서장족자치구은력언어강복중심비종합정형롱환자열점돌변기인이GJB2화SLC26A4기인위상견。
Objective To study genotypes in nonsyndromic hearing loss (NSHL ) patients from Guangxi Zhuang Autonomous Region hearing speech rehabilitation center using DNA microarray in combination with Sanger sequencing .Methods Deaf patients received routine physical and otorhinolaryngoloical examinations as well as pure tone autiometry .Brainstem auditory evoked potential test was performed in uncooperative children .Blood samples were obtained from a total of 136 patients ,male 81 ,female 55 ,age from one year five month to seventeen ,having nonsyndromic hearing loss .Genomic DNA was extracted and then 9 hot mutation spots in 4 susceptibility genes were detected by DNA microarray .GJB2 and SLC26A was further detected by Sanger sequencing in the patients with negative results and heterozygotes .Results Among the 136 patients with nonsyndromic hearing loss ,20 cases were positive for GJB2 gene ,SLC26A4 gene or mitochondrial 12SrRNA gene mutations .There were 14 .71% (20/136)patients were positive for hot mutation spots in the deafness related genes ,25% (34/136)patients carried muta‐tions of deafness related genes using DNA microarray in combination with Sanger sequencing .Six SLC26A4 rare mutations (c .259G> T ,c .754C> T ,c .1229C> T ,c .1548_1549insC ,c .1705+5A>G and c .2086C> T) were de‐tected by Sanger sequencing .c .235delC was the most common mutation in GJB2 gene .c .919-2A>G ,c .754C> T and c .1229C> T were the common mutations in SLC26A4 gene .The mutation rate of GJB2 and SLC26A4 was 38 . 24% .and 58 .82% ,respectively .Conclusion Prevalent deafness-associated gene mutations in the nine loci studied were less frequently detected in nonsyndromic hearing loss patients from Guangxi Zhuang Autonomous Region hear‐ing speech rehabilitation center .It can improve the detection rate of deafness gene mutations by using gene microar‐ray in combination with Sanger sequencing .GJB2 and SLC26A4 are the common causative genes .