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小鼠肺肿瘤中p16INK4a的缺失与差异表达

Deletion and differential expression of p16INK4a in mouse lung tumors.

作者信息

Belinsky S A, Swafford D S, Middleton S K, Kennedy C H, Tesfaigzi J

机构信息

Inhalation Toxicology Research Institute, Albuquerque, NM 87185, USA.

出版信息

Carcinogenesis. 1997 Jan;18(1):115-20. doi: 10.1093/carcin/18.1.115.

DOI:10.1093/carcin/18.1.115
PMID:9054597
Abstract

Recent allelotyping of chemical-induced lung tumors in hybrid mice has detected loss of heterozygosity on chromosome 4 in a region involving the interferon-alpha (IFN-alpha gene cluster that is syntenic to human chromosome 9p21-22, the location of the p16INK4a (p16) and p15INK4b (p15) tumor suppressor genes. The purpose of the current investigation was to characterize the expression of p16 and p15 in lung tumors and tumor-derived cell lines induced in A/J mice by exposure to the tobacco-specific nitrosamine, 4-methylnitrosamino-1-(3-pyridyl)-1-butanone (NNK). Expression of p16 and p15 was detected in all primary lung tumors; however, levels of expression of p16 differed by up to 15-fold between tumors. This is the first study to note a marked difference in the expression of the p16 gene in primary lung tumors. The apparent low levels of expression seen in approximately half of the tumors was not attributed to deletion, mutation or methylation of the p16 gene. Conversely, the high levels of p16 expression were not the result of effects on the retinoblastoma gene (Rb) or cyclin D1 proteins but most likely in response to a dysfunction elsewhere within this pathway. In contrast to the detection of p16 expression in primary tumors, this gene was deleted in all four cell lines. Three of four cell lines also showed loss of the p15 gene. Mapping of these homozygous deletions on chromosome 4 revealed that the p16 gene resides near the D4MIT77 marker, which is located approximately 12 cM proximal to the IFN-alpha gene cluster, thereby implicating the p16 gene as one of the targets within the allelic deletions detected previously in primary lung tumors from hybrid mice.

摘要

最近对杂交小鼠化学诱导的肺肿瘤进行的等位基因分型检测发现,在涉及干扰素-α(IFN-α)基因簇的4号染色体区域出现杂合性缺失,该区域与人9号染色体p21 - 22同源,而这正是p16INK4a(p16)和p15INK4b(p15)肿瘤抑制基因的定位。本研究的目的是表征A/J小鼠暴露于烟草特异性亚硝胺4-甲基亚硝胺基-1-(3-吡啶基)-1-丁酮(NNK)后诱导产生的肺肿瘤及肿瘤衍生细胞系中p16和p15的表达情况。在所有原发性肺肿瘤中均检测到p16和p15的表达;然而,不同肿瘤之间p16的表达水平差异高达15倍。这是首次注意到原发性肺肿瘤中p16基因表达存在显著差异的研究。在大约一半的肿瘤中观察到的明显低表达水平并非归因于p16基因的缺失、突变或甲基化。相反,p16的高表达水平并非视网膜母细胞瘤基因(Rb)或细胞周期蛋白D1蛋白作用的结果,而很可能是对该通路其他部位功能障碍的反应。与原发性肿瘤中检测到p16表达相反,在所有四个细胞系中该基因均被缺失。四个细胞系中的三个也显示p15基因缺失。对4号染色体上这些纯合缺失的定位显示,p16基因位于D4MIT77标记附近,该标记位于IFN-α基因簇近端约12 cM处,从而表明p16基因是先前在杂交小鼠原发性肺肿瘤中检测到的等位基因缺失内的靶点之一。

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