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1、�64�中华临床医师杂志(电子版)2011年1月第5卷第1期�ChinJClinicians(ElectronicEdition),January1,2011,Vo.l5,No.1�论著�DNA片段长度分析检测急性髓性白血病CEBPA基因突变阮国瑞�牛继红�李玲娣�张瑶�李金兰�秦亚溱�赖悦云�刘艳荣许兰平�黄晓军�陈珊珊���摘要��目的�建立检测急性髓性白血病(AML)髓系转录因子CCAAT增强子结合蛋白�A(CEBPA)基因突变的快速筛查方法。方法�采用聚合酶链式反应(PCR)扩增产物片段长度分析及序列分析方法检测107例初治AML患者C
2、EBPA基因全部编码区突变情况。来自同种基因移植供者的38例正常人作为对照。结果�同时用测序及片段长度分析的方法检测了107例AML患者及38例正常人CEBPA突变的情况,在排除了已知的多态位点以后,在107例AML患者中筛查出22例患者存在CEBPA突变,其中4例患者存在2种CEBPA突变,18例患者存在1种CEBPA突变,而在38例正常人中没有发现CEBPA突变。与测序结果比较,片段长度分析检测CEBPA突变是敏感和有效的。结论�片段长度分析是一种快速、敏感地筛查CEBPA基因突变的方法,适合常规的AML诊断。�关键词��白血病,粒细胞,急
3、性;�CCAAT增强子结合蛋白�;�聚合酶链式反应;�序列分析,DNADNAfragmentlengthanalysisforscreeningofCEBPAmutationsinacutemyeloidleukaemia�RUANGuo�rui,NIUJi�hong,LILing�di,ZHANGYao,LIJin�lan,QINYa�zhen,LAIYue�yun,LIUYan�rong,XULan�ping,HUANGXiao�jun,CHENShan�shan.InstituteofHematology,PekingUniversity
4、People�sHospital,Beijing100044,ChinaCorrespondingauthor:RUANGuo�rui,Email:ruanguoru@ipkuph.edu.cn�Abstract��Objective�ToestablisharapidscreeningmethodforCEBPA(CCAAT�EnhancerBindingProtein�alpha,CEBPA)mutations.Methods�WedetectedmutationsthroughouttheentirecodingregionoftheCE
5、BPAgenein107untreatedAMLpatientsusingpolymerasechainreaction(PCR)followedbysequenceanalysisandfragmentlengthanalysis.Thirty�eightnormaldonorsfromtheallogeneicstemcelltransplantationwereservedascontro.lResults�Weevaluatedtheapproachbyanalysing107AMLpatientand38normalsamplesby
6、bothfragmentlengthanalysisandnucleotidesequencing.Twenty�twocaseswithCEBPAmutationwerefoundin107AMLpatientsafterexcludingallknownCEBPApolymorphisms.Of4CEBPAmutatedpatientshadtwomutationsand18patientshadasinglemutation.Nomutationwasfoundin38normalsamples.CEBPAmutationdetectio
7、nbyfragmentlengthanalysisissensitiveandefficientwhencomparedtonucleotidesequencing.Conclusions�WeestablishedafastandsensitiveCEBPAmutationscreeningmethodforroutineAMLdiagnostics.���Keywords��Leukemia,myelocytic,acute;�CCAAT�enhancer�bindingprotein�alpha;�Polymerasechainreact
8、ion;�Sequenceanalysis,DNA��急性髓性白血病(acutemyeloidleukemia,AML)是由髓系造血干/祖细胞发生累积
