PCAN1基因上游两个功能性NKX3.1结合位点的特征分析，这些位点参与PCAN1基因转录的正调控。

Characterization of two functional NKX3.1 binding sites upstream of the PCAN1 gene that are involved in the positive regulation of PCAN1 gene transcription.

作者信息

Liu Wenwen, Zhang Pengju, Chen Weiwen, Yu Chunxiao, Cui Fuai, Kong Feng, Zhang Jianye, Jiang Anli

机构信息

Institute of Biochemistry and Molecular Biology, Shandong University School of Medicine, Jinan, 250012, China.

出版信息

BMC Mol Biol. 2008 May 4;9:45. doi: 10.1186/1471-2199-9-45.

DOI:10.1186/1471-2199-9-45

PMID:18454873

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2390571/

Abstract

BACKGROUND

NKX3.1 and PCAN1 are both prostate-specific genes related to prostate development and prostate cancer. So far, little is known about the regulatory mechanisms of the expression of these two genes. In the present study, we found that NKX3.1 upregulated PCAN1 gene transcription in LNCaP prostate cancer cells. To understand the regulatory mechanisms, our work focused on identifying the functional NKX3.1 binding sites upstream of the PCAN1 gene, which might be involved in the positive regulation of PCAN1 expression by NKX3.1.

RESULTS

We cloned and characterized a 2.6 kb fragment upstream of the PCAN1 gene. Analysis of the 2.6 kb sequence with MatInspector 2.2 revealed five potential binding sites of NKX3.1 transcription factor. Luciferase reporter assays, electrophoretic mobility shift assays, chromatin immunoprecipitation and RNA interference were performed to study the effects of NKX3.1 on PCAN1 gene expression in prostate cancer cells. Our results showed that PCAN1 promoter activity and mRNA expression were increased by transfection with the NKX3.1 containing plasmid (pcDNA3.1-NKX3.1) and that PCAN1 mRNA expression was decreased by RNA interference targeting human NKX3.1 in LNCaP prostate cancer cells. The results of electrophoretic mobility shift assays and chromatin immunoprecipitation showed that NKX3.1 bound to NBS1 (-1848 to -1836) and NBS3 (-803 to -791) upstream of the PCAN1 gene. The luciferase reporter assays showed that NBS1 and NBS3 enhanced the promoter activity in pGL3-promoter vector with cotransfection of the NKX3.1 containing plasmid. Furthermore, the deletion of NBS1 or both NBS1 and NBS3 reduced PCAN1 promoter activity and abolished the positive regulation of PCAN1 expression by NKX3.1.

CONCLUSION

Our results suggested that two functional NKX3.1 binding sites located at -1848 to -1836 and -803 to -791 upstream of the PCAN1 gene were involved in the positive regulation of PCAN1 gene transcription by NKX3.1.

摘要

背景

NKX3.1和PCAN1均为与前列腺发育及前列腺癌相关的前列腺特异性基因。迄今为止，关于这两个基因表达的调控机制知之甚少。在本研究中，我们发现NKX3.1在LNCaP前列腺癌细胞中上调PCAN1基因转录。为了解调控机制，我们的工作聚焦于鉴定PCAN1基因上游的功能性NKX3.1结合位点，其可能参与NKX3.1对PCAN1表达的正向调控。

结果

我们克隆并鉴定了PCAN1基因上游一个2.6 kb的片段。用MatInspector 2.2分析该2.6 kb序列，发现了五个潜在的NKX3.1转录因子结合位点。进行荧光素酶报告基因检测、电泳迁移率变动分析、染色质免疫沉淀和RNA干扰，以研究NKX3.1对前列腺癌细胞中PCAN1基因表达的影响。我们的结果显示，转染含NKX3.1的质粒（pcDNA3.1-NKX3.1）可增加PCAN1启动子活性和mRNA表达，而在LNCaP前列腺癌细胞中，靶向人NKX3.1的RNA干扰可降低PCAN1 mRNA表达。电泳迁移率变动分析和染色质免疫沉淀结果显示，NKX3.1与PCAN1基因上游的NBS1（-1848至-1836）和NBS3（-803至-791）结合。荧光素酶报告基因检测显示，NBS1和NBS3在与含NKX3.1的质粒共转染时增强了pGL3-启动子载体中的启动子活性。此外，缺失NBS1或同时缺失NBS1和NBS3均降低PCAN1启动子活性，并消除了NKX3.1对PCAN1表达的正向调控。