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3q25-q26扩增单元的基因组和表达分析揭示TLOC1/SEC62可能是前列腺癌中的一个靶基因。

Genomic and expression analysis of the 3q25-q26 amplification unit reveals TLOC1/SEC62 as a probable target gene in prostate cancer.

作者信息

Jung Volker, Kindich Roland, Kamradt Jörn, Jung Martin, Müller Mirko, Schulz Wolfgang A, Engers Rainer, Unteregger Gerhard, Stöckle Michael, Zimmermann Richard, Wullich Bernd

机构信息

Clinic of Urology and Pediatric Urology, University of the Saarland, 66421 Homburg/Saar, Germany.

出版信息

Mol Cancer Res. 2006 Mar;4(3):169-76. doi: 10.1158/1541-7786.MCR-05-0165.

DOI:10.1158/1541-7786.MCR-05-0165
PMID:16547154
Abstract

Gain at chromosome 3q25-q26 has been reported to commonly occur in prostate cancer. To map the 3q25-q26 amplification unit and to identify the candidate genes of amplification, we did fluorescence in situ hybridization and quantitative real-time PCR for gene copy number and mRNA expression measurements in prostate cancer cell lines and prostate cancer samples from radical prostatectomy specimens. The minimal overlapping region of DNA copy number gains in the cell lines could be narrowed down to 700 kb at 3q26.2. Of all positional and functional candidates in this region, the gene TLOC1/SEC62 revealed the highest frequency (50%) of copy number gains in the prostate cancer samples and was found to be up-regulated at the mRNA level in all samples analyzed. TLOC1/Sec62 protein was also shown to be overexpressed by Western blot analysis. Intriguingly, the TLOC1/SEC62 gene copy number was increased in prostate tumors from patients who had a lower risk of and a longer time to progression following radical prostatectomy. These findings make TLOC1/SEC62 the best candidate within the 3q amplification unit in prostate cancer. TLOC1/Sec62 protein is a component of the endoplasmic reticulum protein translocation machinery, whose function during prostate carcinogenesis remains to be determined.

摘要

据报道,3q25-q26染色体区域的扩增在前列腺癌中普遍存在。为了绘制3q25-q26扩增单元图谱并鉴定扩增的候选基因,我们对前列腺癌细胞系以及根治性前列腺切除标本中的前列腺癌样本进行了荧光原位杂交和定量实时PCR,以测量基因拷贝数和mRNA表达。细胞系中DNA拷贝数增加的最小重叠区域可缩小至3q26.2处的700 kb。在该区域所有的位置和功能候选基因中,TLOC1/SEC62基因在前列腺癌样本中显示出最高的拷贝数增加频率(50%),并且在所有分析样本的mRNA水平上均上调。蛋白质印迹分析也显示TLOC1/Sec62蛋白过表达。有趣的是,在根治性前列腺切除术后进展风险较低且进展时间较长的患者的前列腺肿瘤中,TLOC1/SEC62基因拷贝数增加。这些发现使TLOC1/SEC62成为前列腺癌3q扩增单元内的最佳候选基因。TLOC1/Sec62蛋白是内质网蛋白质转运机制的一个组成部分,其在前列腺癌发生过程中的功能仍有待确定。

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