中华医学遗传学杂志
中華醫學遺傳學雜誌
중화의학유전학잡지
Chinese Journal of Medical Genetics
2015年
4期
468-471
,共4页
李鹏程%刘飞%张明昌%王秋芬%刘木根
李鵬程%劉飛%張明昌%王鞦芬%劉木根
리붕정%류비%장명창%왕추분%류목근
Usher综合征%USH2A基因%剪切突变
Usher綜閤徵%USH2A基因%剪切突變
Usher종합정%USH2A기인%전절돌변
Usher syndrome%USH2A gene%Mutation
目的 探讨一个Usher综合征家系的致病基因突变.方法 对一个疑似为Usher综合征Ⅱ型家系的所有11名成员进行全面的眼科检查和听力测试,并提取外周血基因组DNA,采用PCR和直接测序对先证者进行USH2A基因的突变筛查.以正常人和患者的基因组DNA为模版,分别构建包含USH2A基因第42外显子、第42内含子及第43外显子的野生型和突变型minigene真核表达质粒.采用脂质体法将携带minigene的质粒转染Hela细胞,通过实时定量PCR检测minigene的剪切情况.结果 家系分析和临床诊断提示该家族患有常染色体隐性遗传的Usher综合征Ⅱ型.测序发现先证者的USH2A基因中存在纯合的c.8559-2A>G突变.对其他家系成员进行测序验证发现该突变与疾病共分离.c.8559-2A>G突变为剪切突变,可能引起第42内含子的剪切异常.Minigene结果证实该突变可导致第42内含子不能剪切,从而保留至成熟的mRNA中.结论 USH2A基因c.8559-2A>G突变是该Usher综合征Ⅱ型家系的致病原因.该突变可以导致USH2A pre-mRNA的剪切异常.
目的 探討一箇Usher綜閤徵傢繫的緻病基因突變.方法 對一箇疑似為Usher綜閤徵Ⅱ型傢繫的所有11名成員進行全麵的眼科檢查和聽力測試,併提取外週血基因組DNA,採用PCR和直接測序對先證者進行USH2A基因的突變篩查.以正常人和患者的基因組DNA為模版,分彆構建包含USH2A基因第42外顯子、第42內含子及第43外顯子的野生型和突變型minigene真覈錶達質粒.採用脂質體法將攜帶minigene的質粒轉染Hela細胞,通過實時定量PCR檢測minigene的剪切情況.結果 傢繫分析和臨床診斷提示該傢族患有常染色體隱性遺傳的Usher綜閤徵Ⅱ型.測序髮現先證者的USH2A基因中存在純閤的c.8559-2A>G突變.對其他傢繫成員進行測序驗證髮現該突變與疾病共分離.c.8559-2A>G突變為剪切突變,可能引起第42內含子的剪切異常.Minigene結果證實該突變可導緻第42內含子不能剪切,從而保留至成熟的mRNA中.結論 USH2A基因c.8559-2A>G突變是該Usher綜閤徵Ⅱ型傢繫的緻病原因.該突變可以導緻USH2A pre-mRNA的剪切異常.
목적 탐토일개Usher종합정가계적치병기인돌변.방법 대일개의사위Usher종합정Ⅱ형가계적소유11명성원진행전면적안과검사화은력측시,병제취외주혈기인조DNA,채용PCR화직접측서대선증자진행USH2A기인적돌변사사.이정상인화환자적기인조DNA위모판,분별구건포함USH2A기인제42외현자、제42내함자급제43외현자적야생형화돌변형minigene진핵표체질립.채용지질체법장휴대minigene적질립전염Hela세포,통과실시정량PCR검측minigene적전절정황.결과 가계분석화림상진단제시해가족환유상염색체은성유전적Usher종합정Ⅱ형.측서발현선증자적USH2A기인중존재순합적c.8559-2A>G돌변.대기타가계성원진행측서험증발현해돌변여질병공분리.c.8559-2A>G돌변위전절돌변,가능인기제42내함자적전절이상.Minigene결과증실해돌변가도치제42내함자불능전절,종이보류지성숙적mRNA중.결론 USH2A기인c.8559-2A>G돌변시해Usher종합정Ⅱ형가계적치병원인.해돌변가이도치USH2A pre-mRNA적전절이상.
Objective To investigate the disease-causing mutation in a Chinese family affected with Usher syndrome type Ⅱ.Methods All of the 11 members from the family underwent comprehensive ophthalmologic examination and hearing test,and their genomic DNA were isolated from venous leukocytes.PCR and direct sequencing of USH2A gene were performed for the proband.Wild type and mutant type minigene vectors containing exon 42,intron 42 and exon 43 of the USH2A gene were constructed and transfected into Hela cells by lipofectamine reagent.Reverse transcription (RT)-PCR was carried out to verify the splicing of the minigenes.Results Pedigree analysis and clinical diagnosis indicated that the patients have suffered from autosomal recessive Usher syndrome type Ⅱ.DNA sequencing has detected a homozygous c.8559-2A>G mutation of the USH2A gene in the proband,which has co-segregated with the disease in the family.The mutation has affected a conserved splice site in intron 42,which has led to inactivation of the splice site.Minigene experiment has confirmed the retaining of intron 42 in mature mRNA.Conclusion The c.8559-2A> G mutation in the USH2A gene probably underlies the Usher syndrome type Ⅱ in this family.The splice site mutation has resulted in abnormal splicing of USH2A premRNA.