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人类端粒酶逆转录酶(hTERT)中新型可变剪接位点的表征:正常组织和肿瘤组织mRNA亚型的表达分析及相互关联

Characterization of novel alternative splicing sites in human telomerase reverse transcriptase (hTERT): analysis of expression and mutual correlation in mRNA isoforms from normal and tumour tissues.

作者信息

Saebøe-Larssen Stein, Fossberg Ellen, Gaudernack Gustav

机构信息

Section for Immunotherapy, Department of Immunology, The Norwegian Radium Hospital, Cancer Research Institute, University of Oslo, N-0310 Oslo, Norway.

出版信息

BMC Mol Biol. 2006 Aug 29;7:26. doi: 10.1186/1471-2199-7-26.

Abstract

BACKGROUND

Human telomerase reverse transcriptase (hTERT) is a key component for synthesis and maintenance of telomeres on chromosome ends and is required for the continued proliferation of cells. Estimation of hTERT expression therefore has broad relevance in oncology and stem cell research. Several splicing variants of hTERT have been described whose regulated expression contributes to the control of telomerase activity. Knowledge of the different hTERT mRNA isoforms and the ability to distinguish between them is an important issue when evaluating telomerase expression.

RESULTS

By establishing cDNA-clone panels from lung and colon tissues, we could map hTERT clones individually for differences in DNA sequence. This made possible the identification of novel alternatively spliced sites as well as analysis of their frequency and mutual correlation in mRNA isoforms. Ten different alternatively spliced sites were detected, of which six were novel sites resulting from alternative splicing of intron 2 or 14. The majority of hTERT cDNA clones from normal and tumour lung and colon tissues encoded truncated proteins ending close after exon 2 or 6.

CONCLUSION

The increased complexity in telomerase expression revealed here has implications for our understanding of telomerase regulation and for the choice of suitable methods for addressing hTERT expression.

摘要

背景

人端粒酶逆转录酶(hTERT)是染色体末端端粒合成与维持的关键成分,是细胞持续增殖所必需的。因此,hTERT表达的评估在肿瘤学和干细胞研究中具有广泛的相关性。已经描述了hTERT的几种剪接变体,其表达调控有助于端粒酶活性的控制。在评估端粒酶表达时,了解不同的hTERT mRNA亚型以及区分它们的能力是一个重要问题。

结果

通过从肺和结肠组织建立cDNA克隆文库,我们能够分别绘制hTERT克隆的DNA序列差异图。这使得鉴定新的可变剪接位点以及分析它们在mRNA亚型中的频率和相互关系成为可能。检测到10个不同的可变剪接位点,其中6个是由内含子2或14的可变剪接产生的新位点。来自正常和肿瘤肺及结肠组织的大多数hTERT cDNA克隆编码在第2或第6外显子后不久终止的截短蛋白。

结论

这里揭示的端粒酶表达复杂性的增加对我们理解端粒酶调控以及选择合适的方法来研究hTERT表达具有重要意义。

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