中华医学遗传学杂志
中華醫學遺傳學雜誌
중화의학유전학잡지
CHINESE JOURNAL OF MEDICAL GENETICS
2009年
2期
183-186
,共4页
顾梅青%叶军%邱文娟%韩连书%张雅芬%顾学范
顧梅青%葉軍%邱文娟%韓連書%張雅芬%顧學範
고매청%협군%구문연%한련서%장아분%고학범
高苯丙氨酸血症%四氢生物蝶呤缺乏症%6-丙酮酰四氢蝶呤合成酶基因%突变
高苯丙氨痠血癥%四氫生物蝶呤缺乏癥%6-丙酮酰四氫蝶呤閤成酶基因%突變
고분병안산혈증%사경생물접령결핍증%6-병동선사경접령합성매기인%돌변
hyperphenylalaninemia%tetrahydrobiopterin defieiency%6-pyruvoyhe-trahydrobiopterin synthesis gene%mutation
目的 了解中国大陆6-丙酮酰四氢蝶呤合成酶缺乏症(6-pyruvoyltetrahydrobiopterinsynthesis deficiency,PTPSD)基因突变谱.方法 采用PCR-限制性长度多态性及常规基因测序法,对55例PTPSD进行6-丙酮酰四氢蝶呤合成酶基因(6-pyruvoyltetrahydrobiopterin syntheie gene,PTS)检测以得出基因突变类型和频率.寻找热点突变;分析基因型与临床表型的关系.结果 PTS基因突变检出率95.28%,检出18种突变类型.P87S(40.57 0A)、N52S(13.21%)、D96N(12.26%)及IVSInt-291A>G(10.38%)为热点突变,前3种突变导致严重型PTPSD.P87L为国内首次报道,发现5种新突变(Q13X、M80T,IVS4nt-2A>G、L93M、K131N).结论 N52S、P87S、D96N及IVSInt-291A>G为中国人PTS的热点突变,PCR-限制性长度多态性方法进行热点突变筛检可提高基因诊断效率.
目的 瞭解中國大陸6-丙酮酰四氫蝶呤閤成酶缺乏癥(6-pyruvoyltetrahydrobiopterinsynthesis deficiency,PTPSD)基因突變譜.方法 採用PCR-限製性長度多態性及常規基因測序法,對55例PTPSD進行6-丙酮酰四氫蝶呤閤成酶基因(6-pyruvoyltetrahydrobiopterin syntheie gene,PTS)檢測以得齣基因突變類型和頻率.尋找熱點突變;分析基因型與臨床錶型的關繫.結果 PTS基因突變檢齣率95.28%,檢齣18種突變類型.P87S(40.57 0A)、N52S(13.21%)、D96N(12.26%)及IVSInt-291A>G(10.38%)為熱點突變,前3種突變導緻嚴重型PTPSD.P87L為國內首次報道,髮現5種新突變(Q13X、M80T,IVS4nt-2A>G、L93M、K131N).結論 N52S、P87S、D96N及IVSInt-291A>G為中國人PTS的熱點突變,PCR-限製性長度多態性方法進行熱點突變篩檢可提高基因診斷效率.
목적 료해중국대륙6-병동선사경접령합성매결핍증(6-pyruvoyltetrahydrobiopterinsynthesis deficiency,PTPSD)기인돌변보.방법 채용PCR-한제성장도다태성급상규기인측서법,대55례PTPSD진행6-병동선사경접령합성매기인(6-pyruvoyltetrahydrobiopterin syntheie gene,PTS)검측이득출기인돌변류형화빈솔.심조열점돌변;분석기인형여림상표형적관계.결과 PTS기인돌변검출솔95.28%,검출18충돌변류형.P87S(40.57 0A)、N52S(13.21%)、D96N(12.26%)급IVSInt-291A>G(10.38%)위열점돌변,전3충돌변도치엄중형PTPSD.P87L위국내수차보도,발현5충신돌변(Q13X、M80T,IVS4nt-2A>G、L93M、K131N).결론 N52S、P87S、D96N급IVSInt-291A>G위중국인PTS적열점돌변,PCR-한제성장도다태성방법진행열점돌변사검가제고기인진단효솔.
Objective To determine the gene mutation spectrum of patients with 6pyruvoyltetrahydrobiopterin synthesis deficiency (PTPSD) in Mainland China. Methods The 6pyruvoyltetrahydrobiopterin synthesis gene (PTS) was analyzed in 55 PTPSD patients by using PCRrestriction fragment length polymorphism (PCR-RFLP) and direct DNA sequencing. The relationship between the genotype and phenotype was analyzed. Results Eighteen mutations were identified and the detection rate of gene mutation was 95.28%. Four hot-spot mutations, namely P87S(40.57%), N52S (13.21%), D96N(12.26%) and IVSInt-291A>G(10.38%) were found in this study, and the first three were associated with severe phenotype. The P87L was reported firstly in Chinese patients, and the Q13X, M80T, IVS4nt-2A>G, L93M and K131N were novel mutations. Conclusion The P87S, N52S, D96N and IVSInt-291A>G mutations are the hot-spots mutations of the PTS gene in Chinese PTPSD patients. Using PCR-RFLP technique to screen the mutations in the PTS gene can increase the efficiency of gene diagnosis.
