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一种新型转基因小鼠模型揭示了正常组织和肿瘤组织中8千碱基对人类端粒酶逆转录酶(TERT)基因启动子片段的类人调控。

A novel transgenic mouse model reveals humanlike regulation of an 8-kbp human TERT gene promoter fragment in normal and tumor tissues.

作者信息

Ritz Julia M, Kühle Olaf, Riethdorf Sabine, Sipos Bence, Deppert Wolfgang, Englert Christoph, Günes Cagatay

机构信息

Heinrich-Pette-Institute, Department of Tumor Virology, Hamburg, Germany.

出版信息

Cancer Res. 2005 Feb 15;65(4):1187-96. doi: 10.1158/0008-5472.CAN-04-3046.

DOI:10.1158/0008-5472.CAN-04-3046
PMID:15735002
Abstract

Telomerase activity is repressed in most human somatic tissues during differentiation processes but strongly up-regulated in most human tumors. Regulation of human telomerase activity primarily occurs at the level of transcriptional initiation of the TERT gene, which encodes the catalytic subunit of telomerase. We have generated a novel transgenic mouse model to study the regulation of the human TERT gene promoter in an in vivo system. For this purpose, we have cloned an 8.0-kbp human TERT promoter fragment in front of the bacterial lacZ reporter gene (hTERTp-lacZ), which encodes the beta-galactosidase enzyme. Expression of the reporter gene was monitored by reverse transcription-PCR analysis, 5-bromo-4-chloro-3-indolyl-beta-d-galactopyranoside staining of whole mount preparations, and histologic sections. We find that the activity of the human TERT promoter in most normal mouse tissues recapitulates the expression of the hTERT gene in normal human tissues and is under tighter control when compared with the endogenous mouse TERT gene expression. In testis, where highest lacZ expression was observed, the expression of the reporter gene was restricted to the spermatogonial stem cells and the spermatocytes. Intriguingly, we find increased levels of lacZ expression in mammary tumors of hTERTp-lacZ x p53(+/-) bitransgenic mouse mammary tumor model. Thus, this transgenic mouse model provides a suitable in vivo system to analyze the expression of the human TERT gene under physiologic conditions and during tumorigenesis.

摘要

在分化过程中,端粒酶活性在大多数人类体细胞组织中受到抑制,但在大多数人类肿瘤中则强烈上调。人类端粒酶活性的调节主要发生在TERT基因转录起始水平,该基因编码端粒酶的催化亚基。我们构建了一种新型转基因小鼠模型,用于在体内系统中研究人类TERT基因启动子的调节。为此,我们在细菌lacZ报告基因(hTERTp-lacZ)前克隆了一个8.0-kbp的人类TERT启动子片段,该报告基因编码β-半乳糖苷酶。通过逆转录-PCR分析、全组织5-溴-4-氯-3-吲哚基-β-D-吡喃半乳糖苷染色和组织切片来监测报告基因的表达。我们发现,人类TERT启动子在大多数正常小鼠组织中的活性重现了hTERT基因在正常人类组织中的表达,并且与内源性小鼠TERT基因表达相比受到更严格的控制。在观察到最高lacZ表达的睾丸中,报告基因的表达仅限于精原干细胞和精母细胞。有趣的是,我们在hTERTp-lacZ x p53(+/-)双转基因小鼠乳腺肿瘤模型的乳腺肿瘤中发现lacZ表达水平升高。因此,这种转基因小鼠模型提供了一个合适的体内系统,用于分析人类TERT基因在生理条件下和肿瘤发生过程中的表达。

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