荧光原位杂交及荧光定量PCR技术检测急性早幼粒细胞白血病患者PML-RARα融合基因比较

Comparison between FISH and fluorescent quantitative PCR in detecting PML-RARα fusion gene of APL patients

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摘要目的比较荧光原位杂交（FISH）及荧光定量PCR技术对急性早幼粒细胞白血病（APL）患者PML-RARα融合基因检测的灵敏度和特异度.方法选取75例APL患者,同时应用FISH及荧光定量PCR方法检测患者PML-RARα融合基因的表达情况.结果共检测初发与复发或缓解患者88例次,总相符率为96.59%;检测初发患者14例,相符率为100%;检测复发或缓解患者74例次,相符率为95.95%;检测干细胞来源的标本6例次,相符率为100%.结论对于初发的APL患者,FISH与荧光定量PCR的灵敏度相同,FISH技术操作更为简单,省时直观.对于残留的检测,FISH的灵敏度不如荧光定量PCR. Objective To detect the PML-RARα fusion gene expression of APL patients with FISH and fluorescent quantitative PCR and discuss the sensitivity and specificity of two techniques. Methods The detection of the PML-RARα fusion gene expression of 75 APL patients with FISH and fluorescent quantitative PCR were carried out simultaneously. Results Eighty eight patients of primary and relapse or remission phases were examinated and total conformity rate was 96.59 %. Fourteen primary patients were detected and conformity rate was 100 %. Seventy four relapse or remission patients were detected and conformity rate was 95.95 %. Stem cell essays were detected for six times and conformity rate was 100 %. Conclusion The sensitivity of FISH and fluorescent quantitative PCR is identical for primary APL patients and FISH is more sensitive. But the sensitivity of FISH is weaker than that of fluorescent quantitative PCR for detection of residue disease.

作者李蔚李艳丽赵雪飞邱林马军

机构地区哈尔滨血液病肿瘤研究所

出处《白血病．淋巴瘤》 CAS 2010年第3期143-145,共3页 Journal of Leukemia & Lymphoma

关键词原位杂交荧光聚合酶链反应基因融合 In situ hybridization,fluorescence Polymerase chain reaction Gene fusion

分类号 R733.7 [医药卫生—肿瘤]

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参考文献7

1袁健,熊文,陈建波,古洪标.染色体分析及FISH法对急性早幼粒细胞白血病诊断的临床意义[J].实用癌症杂志,2007,22(3):266-268. 被引量：3
2孙雪梅,陈蕾蕾,许景艳,谢品浩,杨永公,陈军浩,范洵楠,欧阳建.应用荧光原位杂交技术动态观察急性早幼粒细胞白血病患者PML-RARα融合基因的变化[J].临床血液学杂志,2005,18(3):133-135. 被引量：7
3范耀山.分子细胞遗传学--技术与应用.北京:科学出版社,2007:10.
4Krauter J,Peter W,Pascheberg U,et al.Detection of karyotypic aberration in acute myeloblastic leukemia:a prospective comparison between PCR/FISH and standard cytogenetics in 140 patients with de novo AML.British Journal of Hematology,1998,103:72-78.
5卢建,章钧,何蕴韶.荧光原位杂交技术及其临床应用[J].分子诊断与治疗杂志,2009,1(1):38-42. 被引量：9
6Temperani P,Vaccari P,Giacobbi F,et al.Assessment of minimal residual disease,in acute promyelocytic leukemia with t (15;17) by chromosome painting.EurJ Haematol,1995,55:10-13.
7Gonzalez M,Barragan E,Bolufer P,et al.Pretreatment characteristics and clinical outcome of acute promyelocytic leukemia patients according to the PML-RARα isoforms:a study of the PETHEMA group.BrJ Haematol,2001,114:99-103.

二级参考文献51

1孙雪梅,陈蕾蕾,许景艳,谢品浩,杨永公,陈军浩,范洵楠,欧阳建.应用荧光原位杂交技术动态观察急性早幼粒细胞白血病患者PML-RARα融合基因的变化[J].临床血液学杂志,2005,18(3):133-135. 被引量：7
2杜冰,徐开林,黄一虹,王林,何徐彭,鹿群先,潘秀英.急性早幼粒细胞白血病PML/RARα融合基因检测及临床意义[J].临床荟萃,2006,21(15):1101-1102. 被引量：1
3Berger R, Le Coniat M, Derre J, et al. Cytogenetic studies in acute promyelocytic leukemia: a survey of secondary chromosomal abnormalities. Genes Chromosomes Cancer, 1991, 3:332-337.
4DewaldG,Juneal A,Schad C,et al.Cytogenetic and molecular genetic methods for diagnosis and treatment response in chronic granuloeytic leukemia[J].Cancer Genet Cytogenet,1997,94(1):59.
5GrimwadeD,Biondi A,Mozziconacci MJ,et al.Characterization of acute promyelocytic leukemia cases lacking the classic t(15;17):results of the European Working Party[J].Blood,2000,96:1297.
6PaulssonK,Fioretos T,Strombeck B,et al.Trisomy 8 as the sole chromosomal aberration in myelocytic malignancies:a muhicolor and locus specific fluorescence in situ hybridization study[J].Cancer Genet Cytogenet,2003,140:66.
7OzpolatB,Lopez-Berestein G.Liposomal-all-trans-retinoic acid in treatment of acute promyelocytic leukemia[J].Leuk Lymphoma,2002,43(5):933.
8SucicM,Zadro R,BurazerB,et al.Acute P romyelocytic leukemia M3:cytomorphologic,immunophenotyp ic,cytogenetic,and molecular variants[J].J Hematother Stem Cell Res,2002,11(6):941.
9Anton H. N. Hopman,Christina E. M. Voorter,Frans C. S. Ramaekers.Detection of genomic changes in cancer byin situ hybridization[J]. Molecular Biology Reports . 1994 (1)
10Ian Dunham,Christoph Lengauer,Thomas Cremer,Terry Featherstone.Rapid generation of chromosome-specific alphoid DNA probes using the polymerase chain reaction[J]. Human Genetics . 1992 (4)

共引文献16

1党辉,张艳,丘镜滢,何琦,师岩,王峥,冯德秀,吕珊.荧光原位杂交技术研究慢性粒细胞白血病隐匿型变异易位[J].临床血液学杂志,2006,19(4):195-197. 被引量：2
2袁健,熊文,陈建波,古洪标.染色体分析及FISH法对急性早幼粒细胞白血病诊断的临床意义[J].实用癌症杂志,2007,22(3):266-268. 被引量：3
3朱梅玉.ATRA联合As_2O_3治疗急性早幼粒细胞白血病疗效观察[J].实用全科医学,2007,5(7):625-625. 被引量：2
4彭来君,沈孛,林圣云.702例恶性血液病的骨髓细胞染色体核型分析[J].浙江实用医学,2008,13(5):315-316. 被引量：1
5陈伟红,卓家才,汪鹏程,黄瑞宏,陈成坚,李长钢.白血病MLL基因重排及其融合基因检测的临床意义[J].临床血液学杂志,2008,21(6):566-568. 被引量：6
6杨光,赵瑾,石磊,王恺,解菊芬,马莉.急性早幼粒细胞白血病PML/RARα融合基因的检测[J].中国现代医生,2009,47(11):36-37. 被引量：1
7鲍燕,曹来英,魏敏,孙艳梅.荧光原位杂交技术在产前遗传学诊断中的研究[J].中国儿童保健杂志,2010,18(2):104-106.
8张鼎,胡小梅,胡爱武.荧光原位杂交技术及其在遗传学中的应用进展[J].中华全科医学,2010,8(6):762-764. 被引量：5
9刘继秀,梁雯.宫颈癌研究现状[J].中国基层医药,2011,18(3):406-408. 被引量：13
10陈琦,贾宇臣,王利,郑源强.荧光原位杂交技术及其在医学诊断上的应用[J].现代生物医学进展,2012,12(5):988-991. 被引量：2

1余凯远,翁志梁,李澄棣.尿脱落细胞荧光原位杂交技术诊断膀胱癌的价值[J].国外医学（泌尿系统分册）,2005,25(4):449-452. 被引量：6
2宋欣,陈薇,宋志刚,吕亚莉,钟梅,李向红.肺癌中EGFR蛋白表达和基因扩增相关性研究[J].军医进修学院学报,2010,31(2):169-170. 被引量：5
3庞程,邱敏捷,吴炳权,杨志坚,刘肇华,陈敏坚,徐乐.荧光原位杂交联合核基质蛋白22检测在诊断膀胱癌中应用[J].解放军医药杂志,2016,28(12):62-64. 被引量：4
4李志爽,孟庆勇,于琼,周志强,李丽.定量多基因荧光原位杂交检测乳腺癌中c-myc和CCNE2基因扩增[J].中华病理学杂志,2014,43(7):455-458.
5梁光林,吴炜,夏瑞祥.慢性淋巴细胞白血病的遗传学异常及其临床意义[J].安徽医学,2010,31(9):1130-1132. 被引量：1
6刘亚东(综述),顾沈阳(审校).荧光原位杂交技术在膀胱肿瘤复发中的应用[J].国际泌尿系统杂志,2011,31(4):494-497.
7李翎,郭猛,王春英,王兴武,李胜.胰母细胞瘤一例荧光原位杂交检测[J].肿瘤防治杂志,2005,12(18):1439-1439.
8肺癌诊断:荧光原位杂交比细胞学更精准[J].实用心脑肺血管病杂志,2006,14(9):685-685.
9方宇,曾思恩,肖胜军,莫文法.荧光原位杂交对乳腺癌HER2基因的检测及临床应用[J].重庆医学,2011,40(5):460-461. 被引量：4
10李艳,王新允,刘婷,朱丛中,孙翠云,王爱香,赵凤云.survivin mRNA及蛋白在肺癌组织芯片中的表达及意义[J].肿瘤,2006,26(9):839-841. 被引量：1

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荧光原位杂交及荧光定量PCR技术检测急性早幼粒细胞白血病患者PML-RARα融合基因比较

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