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默克尔细胞癌中的RB1基因:所有肿瘤中均存在高甲基化,且多瘤病毒阴性亚组中同时存在杂合性缺失。

RB1 gene in Merkel cell carcinoma: hypermethylation in all tumors and concurrent heterozygous deletions in the polyomavirus-negative subgroup.

作者信息

Sahi Helka, Savola Suvi, Sihto Harri, Koljonen Virve, Bohling Tom, Knuutila Sakari

机构信息

Department of Pathology, Helsinki University and HUSLAB, Helsinki, Finland; Department of Plastic Surgery, Helsinki University Hospital, Helsinki, Finland.

出版信息

APMIS. 2014 Dec;122(12):1157-66. doi: 10.1111/apm.12274. Epub 2014 Apr 16.

DOI:10.1111/apm.12274
PMID:24735260
Abstract

Sequestration of the tumor suppressor retinoblastoma protein (RB) by the Merkel cell polyomavirus (MCV) is a crucial step in the pathogenesis of Merkel cell carcinoma (MCC). RB expression is frequently lost, particularly in MCV-negative MCC tumors, through yet unknown mechanisms. We compared the genomic copy number changes of 13 MCV-positive and 13 -negative MCC tumors by array comparative genomic hybridization. The analysis revealed increased genomic instability, amplification of 1p34.3-1p34.2, and losses of 11p in the absence of MCV infection. Deletions of the RB1 locus were also detected at high rates in MCV-negative tumors. None of the tumors with heterozygous RB1 losses expressed RB in immunohistochemistry. RB1 promoter hypermethylation was studied with a methylation-specific multiplex ligation-dependent probe amplification technique. The RB1 promoter was methylated in all tumor specimens at CpG islands located close to the ATG start codon, albeit at low levels. The pattern of hypermethylation was similar in all MCC samples, despite RB expression, survival or MCV status. In conclusion, the frequent heterozygous losses of the RB1 locus could partly explain the decreased RB expression in MCV-negative MCC tumors, although the effects of RB1 mutations, coinciding promoter hypermethylation and, for example, miRNA regulation, cannot be excluded.

摘要

默克尔细胞多瘤病毒(MCV)隔离肿瘤抑制因子视网膜母细胞瘤蛋白(RB)是默克尔细胞癌(MCC)发病机制中的关键步骤。RB表达常常缺失,尤其是在MCV阴性的MCC肿瘤中,其机制尚不清楚。我们通过阵列比较基因组杂交比较了13例MCV阳性和13例MCV阴性MCC肿瘤的基因组拷贝数变化。分析显示,在无MCV感染的情况下,基因组不稳定性增加,1p34.3 - 1p34.2区域扩增,11p缺失。在MCV阴性肿瘤中也检测到高频率的RB1基因座缺失。免疫组化显示,RB1杂合缺失的肿瘤均未表达RB。采用甲基化特异性多重连接依赖探针扩增技术研究RB1启动子高甲基化。尽管甲基化水平较低,但在所有肿瘤标本中,靠近ATG起始密码子的CpG岛处的RB1启动子均发生了甲基化。尽管存在RB表达、生存情况或MCV状态差异,但所有MCC样本中的高甲基化模式相似。总之,RB1基因座频繁的杂合缺失可能部分解释了MCV阴性MCC肿瘤中RB表达降低的原因,尽管不能排除RB1突变、同时发生的启动子高甲基化以及例如miRNA调控等的影响。

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