Choi Yong-Woo, Choi Jin Soo, Zheng Long Tai, Lim Yun Jeong, Yoon Hyoung Kyu, Kim Yeul Hong, Wang Young-Pil, Lim Young
Department of Anesthesiology, St. Mary's Hospital, The Catholic University, Seoul, South Korea.
Lung Cancer. 2007 Jan;55(1):43-51. doi: 10.1016/j.lungcan.2006.09.018. Epub 2006 Nov 15.
Genomic alterations have been identified in lung cancer tissues and reported in numerous studies. To analyze genomic aberrations in lung cancer patients, we used array comparative genomic hybridization (array CGH) in 14 squamous cell lung carcinoma (SqC) tissues. Copy number gain and loss in chromosomal regions were detected, and the corresponding genes were confirmed by real time PCR. Several frequently altered loci, including gain of 3q (36% of samples), were found. The most frequently identified losses were found at 14q32.33 (21% of samples). The relative degree of chromosomal change was analyzed using log2 ratios. High-level DNA amplifications (>0.8 log2 ratio) were detected at 20 regions in 1p, 2q, 3q, 4q, 6q, 7p, 8q, 9p, 10q, 12q, 14q and 19p. We found that the fold change levels were highest at EVI1 (3q26.2), LPP (3q27-28) and FHF-1 (3q28) gene loci. Our results show that array CGH is a useful tool for identification of gene alteration in lung cancer, and that the above-mentioned genes might represent potential candidate genes for pathogenesis and diagnosis of lung cancer.
在肺癌组织中已鉴定出基因组改变,并在众多研究中有所报道。为了分析肺癌患者的基因组畸变,我们对14例肺鳞状细胞癌(SqC)组织进行了阵列比较基因组杂交(array CGH)。检测染色体区域的拷贝数增加和减少,并通过实时PCR确认相应基因。发现了几个频繁改变的位点,包括3q增益(36%的样本)。最常发现的缺失位于14q32.33(21%的样本)。使用log2比值分析染色体变化的相对程度。在1p、2q、3q、4q、6q、7p、8q、9p、10q、12q、14q和19p的20个区域检测到高水平DNA扩增(>0.8 log2比值)。我们发现,EVI1(3q26.2)、LPP(3q27 - 28)和FHF - 1(3q28)基因位点的倍数变化水平最高。我们的结果表明,阵列CGH是鉴定肺癌基因改变的有用工具,上述基因可能代表肺癌发病机制和诊断的潜在候选基因。