中华医学遗传学杂志
中華醫學遺傳學雜誌
중화의학유전학잡지
CHINESE JOURNAL OF MEDICAL GENETICS
2012年
2期
141-144
,共4页
韩鸿玲%林珊%孙丽莎%张鹏%翟德佩
韓鴻玲%林珊%孫麗莎%張鵬%翟德珮
한홍령%림산%손려사%장붕%적덕패
脂蛋白肾小球病%载脂蛋白E%基因突变%氨基酸缺失
脂蛋白腎小毬病%載脂蛋白E%基因突變%氨基痠缺失
지단백신소구병%재지단백E%기인돌변%안기산결실
Lipoprotein glomerulopathy%Apolipoprotein E%Gene mutation%Amino acid deletion
目的 分析1个脂蛋白肾小球病家系的载脂蛋白E(apolipoprotein E,apoE)基因突变.方法 用盐析法提取该家系4名成员和2名正常人的外周血基因组DNA,PCR扩增apoE基因第4外显子、第3外显子以及多态性片段,扩增产物纯化后分别构建到pTA2载体中,克隆载体转化至大肠杆菌DH5α感受态中,经蓝白斑和抗菌素筛选后集菌,提取重组子质粒,EcoRⅠ酶切鉴定是否转化成功,鉴定正确的菌液行双向测序.PCR-限制性片段长度多态性检测apoE基因多态性.结果 家系中先证者及其母亲和姐姐apoE基因第4外显子第484~492位9个碱基(CAAGCTGCG)缺失,为杂合缺失,其导致apoE氨基酸序列第143~145位KLR的3个氨基酸缺失.第3外显子测序未发现异常.apoE基因多态性分析结果与测序结果一致.结论 该家系的脂蛋白肾小球病因可能为apoE基因第484~492位9个碱基(CAAGCTGCG)缺失.
目的 分析1箇脂蛋白腎小毬病傢繫的載脂蛋白E(apolipoprotein E,apoE)基因突變.方法 用鹽析法提取該傢繫4名成員和2名正常人的外週血基因組DNA,PCR擴增apoE基因第4外顯子、第3外顯子以及多態性片段,擴增產物純化後分彆構建到pTA2載體中,剋隆載體轉化至大腸桿菌DH5α感受態中,經藍白斑和抗菌素篩選後集菌,提取重組子質粒,EcoRⅠ酶切鑒定是否轉化成功,鑒定正確的菌液行雙嚮測序.PCR-限製性片段長度多態性檢測apoE基因多態性.結果 傢繫中先證者及其母親和姐姐apoE基因第4外顯子第484~492位9箇堿基(CAAGCTGCG)缺失,為雜閤缺失,其導緻apoE氨基痠序列第143~145位KLR的3箇氨基痠缺失.第3外顯子測序未髮現異常.apoE基因多態性分析結果與測序結果一緻.結論 該傢繫的脂蛋白腎小毬病因可能為apoE基因第484~492位9箇堿基(CAAGCTGCG)缺失.
목적 분석1개지단백신소구병가계적재지단백E(apolipoprotein E,apoE)기인돌변.방법 용염석법제취해가계4명성원화2명정상인적외주혈기인조DNA,PCR확증apoE기인제4외현자、제3외현자이급다태성편단,확증산물순화후분별구건도pTA2재체중,극륭재체전화지대장간균DH5α감수태중,경람백반화항균소사선후집균,제취중조자질립,EcoRⅠ매절감정시부전화성공,감정정학적균액행쌍향측서.PCR-한제성편단장도다태성검측apoE기인다태성.결과 가계중선증자급기모친화저저apoE기인제4외현자제484~492위9개감기(CAAGCTGCG)결실,위잡합결실,기도치apoE안기산서렬제143~145위KLR적3개안기산결실.제3외현자측서미발현이상.apoE기인다태성분석결과여측서결과일치.결론 해가계적지단백신소구병인가능위apoE기인제484~492위9개감기(CAAGCTGCG)결실.
Objective To identify potential mutation of apolipoprotein E(apoE) gene in a male patient affected with lipoprotein glomerulopathy (LPG),his mother and his sister.Methods The patient and his mother both had histologically confirmed LPG.His sister and his father were asymptomatic.Genomic DNA was extracted from peripheral blood samples.PCR products of the coding region of exons 3 and 4 of the apoE gene were cloned into a pTA2 vector and sequenced.Genetic variations of the apoE gene were detected using PCR and restriction fragment length polymorphism (RFLP).Results An apoE gene mutation was identified in the patient's family.Sequence analysis confirmed a 9-bp deletion in the exon 4 of apoE gene from nt 484 to 492.The 9-bp deletion resulted in loss of 3 amino acids at positions 143 145.The sister of the propositus carried the same mutation,though she had neither proteinuria nor elevated plasma apoE.Sequence analysis of exon 3 showed no abnormality.No abnormalities were found in the father's apoE gene sequence.Analysis of genetic variations of the apoE gene by PCR and RFLP confirmed a 57 bp fragment consistent with the 9-bp deletion in exon 4.The father had a normal ε3ε3 genotype.Conclnsion The 9 bp deletion of apoE may be associated with the pathogenesis of LPG.
