Tan Yue-qiu, Di Yu-fen, Song Yuan-zong, Cheng De-hua, Li Lu-yun, Lu Guang-xiu
Institute of Reproduction and Stem Cell Engineering, Central South University, Changsha, Hunan, 410078 P. R. China.
Zhonghua Yi Xue Yi Chuan Xue Za Zhi. 2007 Aug;24(4):392-6.
To characterize a supernumerary marker chromosome (SMC) by comparative genomic hybridization (CGH), fluorescence in situ hybridization (FISH) and traditional cytogenetic techniques, and to explore the clinical application of these techniques in delineating de novo marker chromosomes.
A mental retardation patient received chromosome test by ordinary G banding. CGH and FISH techniques were used to analyze the origin of the de novo SMC, and N banding technique and C banding techniques were used to analyze the SMC structure. The phenotypic effects of the SMC were analyzed after the karyotype was determined.
By G banding technique, the patient was showed to have a mosaic karyotype with SMC: mos.47, XX, +mar [31]/48, XX, +2mar[29]. CGH analysis showed a gain of 15q11 --> q14, and the result was confirmed by FISH with chromosome 15 painting probe. The further FISH analysis showed the SMC had two signals with UBE3A probe for detecting Prader-willi syndrome/Angelman syndrome (PWS/AS). N banding and C banding analysis showed the SMC had a double satellite and double centromere, respectively. Combined with the above results, the karyotype of the patient was: mos.47, XX, +der (15) (pter --> q14::q14 --> pter) [31]/48, XX, +2der (15) (pter --> q14::q14 --> pter) [29]. ish der(15)(WCP15+, UBE3A++, PML-).
CGH is a valuable method to detect imbalanced chromosomal rearrangement. Combined with FISH and the traditional cytogenetic technique, it provides a valuable technique platform for characterizing the structure of the de novo SMC, and a basis for exploring the relation between karyotype and phenotype, prognosis and recurrent risk.
通过比较基因组杂交(CGH)、荧光原位杂交(FISH)和传统细胞遗传学技术对一条额外的标记染色体(SMC)进行特征分析,并探讨这些技术在描绘新发标记染色体中的临床应用。
一名智力发育迟缓患者接受了普通G显带染色体检测。采用CGH和FISH技术分析新发SMC的起源,采用N显带技术和C显带技术分析SMC的结构。确定核型后分析SMC的表型效应。
通过G显带技术,显示该患者为含有SMC的嵌合核型:mos.47, XX, +mar [31]/48, XX, +2mar[29]。CGH分析显示15q11→q14存在增益,用15号染色体涂染探针进行FISH验证了该结果。进一步的FISH分析显示,该SMC在用检测普拉德-威利综合征/安吉尔曼综合征(PWS/AS)的UBE3A探针检测时有两个信号。N显带和C显带分析分别显示该SMC有双随体和双着丝粒。结合上述结果,该患者的核型为:mos.47, XX, +der (15) (pter→q14::q14→pter) [31]/48, XX, +2der (15) (pter→q14::q14→pter) [29]。ish der(15)(WCP15+, UBE3A++, PML-)。
CGH是检测染色体不平衡重排的一种有价值的方法。结合FISH和传统细胞遗传学技术,它为描绘新发SMC的结构提供了一个有价值的技术平台,也为探索核型与表型、预后及复发风险之间的关系奠定了基础。