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通过可变5'非翻译区的表达对gli1癌基因进行转录后调控。

Post-transcriptional regulation of the gli1 oncogene by the expression of alternative 5' untranslated regions.

作者信息

Wang X Q, Rothnagel J A

机构信息

Department of Biochemistry and the Institute for Molecular Bioscience, The University of Queensland, Brisbane, Queensland 4072, Australia.

出版信息

J Biol Chem. 2001 Jan 12;276(2):1311-6. doi: 10.1074/jbc.M005191200.

Abstract

The oncogene GLI1 is involved in the formation of basal cell carcinoma and other tumor types as a result of the aberrant signaling of the Sonic hedgehog-Patched pathway. In this study, we have identified alternative GLI1 transcripts that differ in their 5' untranslated regions (UTRs) and are generated by exon skipping. These are denoted alpha-UTR, beta-UTR, and gamma-UTR according to the number of noncoding exons possessed (three, two, and one, respectively). The alpha- and beta-UTR forms represent the major Gli1 transcripts expressed in mouse tissues, whereas the gamma-UTR is present at relatively low levels but is markedly induced in mouse skin treated with 12-O-tetradecanoylphorbol 13-acetate. Transcripts corresponding to the murine beta and gamma forms were identified in human tissues, but significantly, only the gamma-UTR form was present in basal cell carcinomas and in proliferating cultures of a keratinocyte cell line. Flow cytometry analysis determined that the gamma-UTR variant expresses a heterologous reporter gene 14-23-fold higher than the alpha-UTR and 5-13-fold higher than the beta-UTR in a variety of cell types. Because expression of the gamma-UTR variant correlates with proliferation, consistent with a role for GLI1 in growth promotion, up-regulation of GLI1 expression through skipping of 5' noncoding exons may be an important tumorigenic mechanism.

摘要

致癌基因GLI1因Sonic hedgehog-Patched信号通路异常而参与基底细胞癌和其他肿瘤类型的形成。在本研究中,我们鉴定出了5'非翻译区(UTR)不同且由外显子跳跃产生的GLI1可变转录本。根据所含非编码外显子的数量(分别为三个、两个和一个),这些转录本分别被命名为α-UTR、β-UTR和γ-UTR。α-UTR和β-UTR形式是小鼠组织中表达的主要Gli1转录本,而γ-UTR的表达水平相对较低,但在用12-O-十四酰佛波醇-13-乙酸酯处理的小鼠皮肤中显著诱导表达。在人类组织中鉴定出了与小鼠β和γ形式相对应的转录本,但值得注意的是,只有γ-UTR形式存在于基底细胞癌和角质形成细胞系的增殖培养物中。流式细胞术分析确定,在多种细胞类型中,γ-UTR变体表达异源报告基因的水平比α-UTR高14 - 23倍,比β-UTR高5 - 13倍。由于γ-UTR变体的表达与增殖相关,这与GLI1在促进生长中的作用一致,通过跳过5'非编码外显子上调GLI1表达可能是一种重要的致瘤机制。

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