中华皮肤科杂志
中華皮膚科雜誌
중화피부과잡지
Chinese Journal of Dermatology
2010年
2期
85-87
,共3页
马俊红%肖生祥%安金刚%王晓鹏%许庆强%董颖颖%冯义国
馬俊紅%肖生祥%安金剛%王曉鵬%許慶彊%董穎穎%馮義國
마준홍%초생상%안금강%왕효붕%허경강%동영영%풍의국
原卟啉病%红细胞生成性%亚铁螯合酶%突变
原卟啉病%紅細胞生成性%亞鐵螯閤酶%突變
원계람병%홍세포생성성%아철오합매%돌변
Protoporphyria%erythropoietic%Ferrochelatase%Mutation
目的 通过对一例红细胞生成性原卟啉病家系亚铁螫合酶基因突变检测,探讨红细胞生成性原卟啉病的遗传特征.方法 收集一例红细胞生成性原卟啉病家系中4例患者及3例表型正常者和50例无亲缘关系健康个体外周血标本,采用PCR扩增亚铁螯合酶基因全部11个外显子及侧翼序列并进行直接测序.结果 先证者及其母亲、姐姐、表兄、外祖父中检测到一个新的剪接突变位点间隔序列(IVS)3+1G→A,其外祖母和父亲未发现该突变;正常对照未发现此突变.先证者及其父亲、姐姐、表兄、外祖父两个单核苷酸多态性为IVS1-3T/C和IVS3-48C/T,而先证者的母亲与外祖母为IVS1-23C/C和IVS3-48T/T.结论 发现红细胞生成性原卟啉病家系一个新的基因突变位点,该突变可能与两个低表达等位基因IVS1-23T和IVS3-48C共同导致红细胞生成性原卟啉病的临床表型.
目的 通過對一例紅細胞生成性原卟啉病傢繫亞鐵螫閤酶基因突變檢測,探討紅細胞生成性原卟啉病的遺傳特徵.方法 收集一例紅細胞生成性原卟啉病傢繫中4例患者及3例錶型正常者和50例無親緣關繫健康箇體外週血標本,採用PCR擴增亞鐵螯閤酶基因全部11箇外顯子及側翼序列併進行直接測序.結果 先證者及其母親、姐姐、錶兄、外祖父中檢測到一箇新的剪接突變位點間隔序列(IVS)3+1G→A,其外祖母和父親未髮現該突變;正常對照未髮現此突變.先證者及其父親、姐姐、錶兄、外祖父兩箇單覈苷痠多態性為IVS1-3T/C和IVS3-48C/T,而先證者的母親與外祖母為IVS1-23C/C和IVS3-48T/T.結論 髮現紅細胞生成性原卟啉病傢繫一箇新的基因突變位點,該突變可能與兩箇低錶達等位基因IVS1-23T和IVS3-48C共同導緻紅細胞生成性原卟啉病的臨床錶型.
목적 통과대일례홍세포생성성원계람병가계아철석합매기인돌변검측,탐토홍세포생성성원계람병적유전특정.방법 수집일례홍세포생성성원계람병가계중4례환자급3례표형정상자화50례무친연관계건강개체외주혈표본,채용PCR확증아철오합매기인전부11개외현자급측익서렬병진행직접측서.결과 선증자급기모친、저저、표형、외조부중검측도일개신적전접돌변위점간격서렬(IVS)3+1G→A,기외조모화부친미발현해돌변;정상대조미발현차돌변.선증자급기부친、저저、표형、외조부량개단핵감산다태성위IVS1-3T/C화IVS3-48C/T,이선증자적모친여외조모위IVS1-23C/C화IVS3-48T/T.결론 발현홍세포생성성원계람병가계일개신적기인돌변위점,해돌변가능여량개저표체등위기인IVS1-23T화IVS3-48C공동도치홍세포생성성원계람병적림상표형.
Objective To characterize the inheritance of erythropoietic protoporphyria (EPP) by detecting the mutations of ferroehelatase (FECH) gene in a Chinese family with EPP. Methods Peripheral blood samples were obtained from 4 patients and 3 unaffected individuals in a family with EPP, as well as from 50 unrelated healthy human controls. PCR was performed to amplify all the 11 exons and flanking sequence of FECH gene followed by direct sequencing. Results A splicing mutation,I.e., IVS3+1G→A, was identified in the proband as well as his symptomatic sister, cousin, grandfather and asymptomatic mother, but not in his asymptomatic father, grandmother, or unrelated healthy controls. The genotypes IVS1-23 T/C and IVS3-48 C/T were noted in the proband, his father, sister, cousin and grandfather, but absent in his mother or grandmother who carried IVS1-23 C/C and IVS3-48 T/T genotypes. Conclusions A novel splicing mutation is found in the FECH gene in a Chinese EPP family, which, together with two lowly expressed alleles IVS1-23T and IVS3-48C, is likely to be responsible for the clinical phenotype of EPP in this family.
