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
3期
343-346
,共4页
白淑潇%潘金兰%薛永权%陈苏宁%吴亚芳%王勇%张俊%沈娟
白淑瀟%潘金蘭%薛永權%陳囌寧%吳亞芳%王勇%張俊%瀋娟
백숙소%반금란%설영권%진소저%오아방%왕용%장준%침연
多发性骨髓瘤%低亚二倍体%荧光原位杂交
多髮性骨髓瘤%低亞二倍體%熒光原位雜交
다발성골수류%저아이배체%형광원위잡교
Multiple myeloma%Low hypodiploid%Fluorescence in situ hybridization
目的 报告1例伴有低亚二倍体复杂异常的多发性骨髓瘤病例并探讨其临床和实验室特点.方法 采用骨髓细胞短期培养法制备染色体,用R显带技术进行核型分析.用13q14、p53、Rbl、lq21一系列单色探针和IgH/CCND1双色双融合探针对其进行荧光原位杂交检测.用流式细胞仪检测DNA含量.结果 R显带核型分析提示该患者5个细胞为包含35条染色体的低亚二倍体核型,3个细胞为低亚二倍体克隆的复制,另外4个细胞为正常核型.间期荧光原位杂交证实核型中存在1号、13号、14号、17号染色体单体,且显示marl来源于11号染色体并造成CCND1基因的扩增.流式细胞仪检测DNA含量显示其有低亚二倍体克隆峰,DNA指数为0.8426.结论 低亚二倍体核型在多发性骨髓瘤中发生率极低,荧光原位杂交技术是检测多发性骨髓瘤分子异常的可靠手段.
目的 報告1例伴有低亞二倍體複雜異常的多髮性骨髓瘤病例併探討其臨床和實驗室特點.方法 採用骨髓細胞短期培養法製備染色體,用R顯帶技術進行覈型分析.用13q14、p53、Rbl、lq21一繫列單色探針和IgH/CCND1雙色雙融閤探針對其進行熒光原位雜交檢測.用流式細胞儀檢測DNA含量.結果 R顯帶覈型分析提示該患者5箇細胞為包含35條染色體的低亞二倍體覈型,3箇細胞為低亞二倍體剋隆的複製,另外4箇細胞為正常覈型.間期熒光原位雜交證實覈型中存在1號、13號、14號、17號染色體單體,且顯示marl來源于11號染色體併造成CCND1基因的擴增.流式細胞儀檢測DNA含量顯示其有低亞二倍體剋隆峰,DNA指數為0.8426.結論 低亞二倍體覈型在多髮性骨髓瘤中髮生率極低,熒光原位雜交技術是檢測多髮性骨髓瘤分子異常的可靠手段.
목적 보고1례반유저아이배체복잡이상적다발성골수류병례병탐토기림상화실험실특점.방법 채용골수세포단기배양법제비염색체,용R현대기술진행핵형분석.용13q14、p53、Rbl、lq21일계렬단색탐침화IgH/CCND1쌍색쌍융합탐침대기진행형광원위잡교검측.용류식세포의검측DNA함량.결과 R현대핵형분석제시해환자5개세포위포함35조염색체적저아이배체핵형,3개세포위저아이배체극륭적복제,령외4개세포위정상핵형.간기형광원위잡교증실핵형중존재1호、13호、14호、17호염색체단체,차현시marl래원우11호염색체병조성CCND1기인적확증.류식세포의검측DNA함량현시기유저아이배체극륭봉,DNA지수위0.8426.결론 저아이배체핵형재다발성골수류중발생솔겁저,형광원위잡교기술시검측다발성골수류분자이상적가고수단.
[Objective]To report the clinical and laboratory characterization of a case of multiple myeloma with low hypodiploid complex karyotyptic abnormalities.[Methods] Cytogeuetic examination of bone marrow performed by 24 h culture method.R-banding technique was used to analyze the karyotype.Interphase fluorescence in situ hybridization (FISH) was performed using chromosome probes such as 13q14,p53,Rbl,lq21 and IgH/CCND1.The DNA content was detected by flow cytometry.[Results] Chromosome analysis revealed complex chromosomal rearrangement.Five cells had a low hypodiploid karyotype with chromosomal number 35.Three ceils had the duplication of the low hypodiploid karyotype.Four ceils had normal karyotype.Monosomy 1,13,14,17 and the mark chromosome 1 derivated from chromosome 11 resulting in the amplication of CCND1 gene were confirmed by interphase FISH.Flow cytometric analysis displayed a low hypodiploid peak with the DNA index of 0.8426.[Conclusion] These results indicated that the low hypodiploidy is a rare abnormality in multiple myeloma.Interphase FISH is a reliable method for detecting molecular abnormalities in multiple myeloma.
