利用人附睾蛋白4启动子在卵巢癌细胞中进行转录靶向。

Transcriptional targeting in ovarian cancer cells using the human epididymis protein 4 promoter.

作者信息

Berry Nicholas B, Cho Yong Mee, Harrington Maureen A, Williams Stephen D, Foley John, Nephew Kenneth P

机构信息

Medical Sciences, Indiana University School of Medicine, Bloomington, IN 47405, USA.

出版信息

Gynecol Oncol. 2004 Mar;92(3):896-904. doi: 10.1016/j.ygyno.2003.12.024.

DOI:10.1016/j.ygyno.2003.12.024

PMID:14984958

Abstract

OBJECTIVE

Limitations of current ovarian cancer gene therapies include lack of specificity and transduction of normal tissues. One strategy toward overcoming these limitations is to direct gene therapy specifically to ovarian cancer cells by using tissue- and tumor-specific promoters. The whey-acidic protein human epididymis protein 4 (HE4) is frequently overexpressed in ovarian cancer, suggesting that the HE4 promoter is highly transcriptionally active in the disease. The objective of this study was to isolate the HE4 promoter and examine its ability to selectively activate reporter gene expression in an ovarian cancer-specific manner.

METHODS

To investigate transcriptional targeting in ovarian cancer gene therapy, we isolated a region of the HE4 promoter from -530 to +122 (pHE4-652; relative to the ATG start site of HE4) and placed it upstream of a luciferase reporter gene plasmid to generate pHE4-652-luc. The activity of the pHE4-652-luc reporter construct was characterized in transient transfection assays in a panel of epithelial ovarian cancer cell lines (SKOV-3, SKOV-3x, CP70, HeyC2, A2780, A2780CP, OVCAR-3), non-ovarian tumor cell lines, and primary cultures of normal cells. The activity of two other candidate gene therapy promoters, human telomerase reverse transcriptase (hTERT) and OSP1, was also characterized in these cell lines.

RESULTS

The HE4 promoter was active in 5/7 ovarian cancer cell lines with the range of activity spanning 0.06- to 3-fold that observed for a positive control, cotransfected reporter construct (SV-40-luc). Minimal pHE4-652 promoter activity, defined as < or =5% of the activity detected with the SV-40-luc construct, was observed in the non-ovarian tumor cell lines and normal cells. The hTERT and the OSP1 promoters were active in the ovarian cancer lines. hTERT activity was highest in the CP70 cell line, and OSP1 activity was highest in the SKOV-3x cell line. Modest OSP1 and hTERT promoter activity was observed in normal cell lines and in selected non-ovarian cancer cell lines.

CONCLUSION

This is the first report using the pHE4-652 promoter to drive specific reporter gene expression in epithelial ovarian cancer cell lines, and we are continuing to develop this promoter for use in transcriptional targeting in ovarian cancer gene therapy.

摘要

目的

目前卵巢癌基因治疗的局限性包括缺乏特异性以及对正常组织的转导。克服这些局限性的一种策略是通过使用组织和肿瘤特异性启动子将基因治疗特异性地导向卵巢癌细胞。乳清酸性蛋白人附睾蛋白4（HE4）在卵巢癌中经常过度表达，这表明HE4启动子在该疾病中具有高度转录活性。本研究的目的是分离HE4启动子，并检测其以卵巢癌特异性方式选择性激活报告基因表达的能力。

方法

为了研究卵巢癌基因治疗中的转录靶向性，我们从-530至+122分离出HE4启动子区域（pHE4-652；相对于HE4的ATG起始位点），并将其置于荧光素酶报告基因质粒的上游，以生成pHE4-652-luc。在一组上皮性卵巢癌细胞系（SKOV-3、SKOV-3x、CP70、HeyC2、A2780、A2780CP、OVCAR-3）、非卵巢肿瘤细胞系和正常细胞原代培养物的瞬时转染实验中，对pHE4-652-luc报告基因构建体的活性进行了表征。另外两个候选基因治疗启动子，人端粒酶逆转录酶（hTERT）和OSP1的活性也在这些细胞系中进行了表征。

结果

HE4启动子在7个卵巢癌细胞系中的5个中具有活性，活性范围为共转染报告基因构建体（SV-40-luc）所观察到活性的0.06至3倍。在非卵巢肿瘤细胞系和正常细胞中观察到最小的pHE4-652启动子活性，定义为<或=SV-40-luc构建体检测到活性的5%。hTERT和OSP1启动子在卵巢癌细胞系中具有活性。hTERT活性在CP70细胞系中最高，OSP1活性在SKOV-3x细胞系中最高。在正常细胞系和选定的非卵巢癌细胞系中观察到适度的OSP1和hTERT启动子活性。