Matrka Marie C, Hennigan Robert F, Kappes Ferdinand, DeLay Monica L, Lambert Paul F, Aronow Bruce J, Wells Susanne I
a Cancer and Blood Diseases Institute; Cincinnati Children's Hospital Medical Center and University of Cincinnati ; Cincinnati , OH USA.
b Department of Biological Sciences ; Xi'an Jiaotong-Liverpool University , Suzhou , Jiangsu Province , China.
Cell Cycle. 2015;14(24):3939-53. doi: 10.1080/15384101.2015.1044177. Epub 2015 May 6.
The DEK gene encodes a nuclear protein that binds chromatin and is involved in various fundamental nuclear processes including transcription, RNA splicing, DNA replication and DNA repair. Several cancer types characteristically over-express DEK at the earliest stages of transformation. In order to explore relevant mechanisms whereby DEK supports oncogenicity, we utilized cancer databases to identify gene transcripts whose expression patterns are tightly correlated with that of DEK. We identified an enrichment of genes involved in mitosis and thus investigated the regulation and possible function of DEK in cell division. Immunofluorescence analyses revealed that DEK dissociates from DNA in early prophase and re-associates with DNA during telophase in human keratinocytes. Mitotic cell populations displayed a sharp reduction in DEK protein levels compared to the corresponding interphase population, suggesting DEK may be degraded or otherwise removed from the cell prior to mitosis. Interestingly, DEK overexpression stimulated its own aberrant association with chromatin throughout mitosis. Furthermore, DEK co-localized with anaphase bridges, chromosome fragments, and micronuclei, suggesting a specific association with mitotically defective chromosomes. We found that DEK over-expression in both non-transformed and transformed cells is sufficient to stimulate micronucleus formation. These data support a model wherein normal chromosomal clearance of DEK is required for maintenance of high fidelity cell division and chromosomal integrity. Therefore, the overexpression of DEK and its incomplete removal from mitotic chromosomes promotes genomic instability through the generation of genetically abnormal daughter cells. Consequently, DEK over-expression may be involved in the initial steps of developing oncogenic mutations in cells leading to cancer initiation.
DEK基因编码一种与染色质结合的核蛋白,参与包括转录、RNA剪接、DNA复制和DNA修复等各种基本的核过程。几种癌症类型在转化的最早阶段通常会过度表达DEK。为了探索DEK支持致癌性的相关机制,我们利用癌症数据库来识别其表达模式与DEK紧密相关的基因转录本。我们发现参与有丝分裂的基因富集,因此研究了DEK在细胞分裂中的调控及可能的功能。免疫荧光分析显示,在人类角质形成细胞中,DEK在前期早期与DNA解离,并在末期重新与DNA结合。与相应的间期细胞群体相比,有丝分裂细胞群体中DEK蛋白水平急剧下降,这表明DEK可能在有丝分裂前被降解或以其他方式从细胞中去除。有趣的是,DEK过表达在整个有丝分裂过程中刺激了其自身与染色质的异常结合。此外,DEK与后期桥、染色体片段和微核共定位,表明与有丝分裂缺陷染色体存在特定关联。我们发现,在未转化和转化细胞中过表达DEK都足以刺激微核形成。这些数据支持了一个模型,即维持高保真细胞分裂和染色体完整性需要DEK正常的染色体清除。因此,DEK的过表达及其从有丝分裂染色体上的不完全去除会通过产生基因异常的子细胞促进基因组不稳定导致癌症发生的细胞中致癌突变的初始步骤。