Abstract

The transcription of human telomerase gene hTERT is regulated by transcription factors (TFs), including Sp1 family proteins, and its chromatin environment. To understand its regulation in a relevant chromatin context, we employed bacterial artificial chromosome reporters containing 160 kb of human genomic sequence containing the hTERT gene. Upon chromosomal integration, the bacterial artificial chromosomes recapitulated endogenous hTERT expression, contrary to transient reporters. Sp1/Sp3 expression did not correlate with hTERT promoter activity, and these TFs bound to the hTERT promoters in both telomerase-positive and telomerase-negative cells. Mutation of the proximal GC-box resulted in a dramatic decrease of hTERT promoter activity, and mutations of all five GC-boxes eliminated its transcriptional activity. Neither mutations of GC-boxes nor knockdown of endogenous Sp1 impacted promoter binding by other TFs, including E-box-binding proteins, and histone acetylation and trimethylation of histone H3K9 at the hTERT promoter in telomerase-positive and -negative cells. The result indicated that promoter binding by Sp1/Sp3 was essential, but not a limiting step, for hTERT transcription. hTERT transcription required a permissive chromatin environment. Importantly, our data also revealed different functions of GC-boxes and E-boxes in hTERT regulation; although GC-boxes were essential for promoter activity, factors bound to the E-boxes functioned to de-repress hTERT promoter.

Highlights

  • Regulation of telomerase gene by Sp1 family proteins remains contradictory in previous studies

  • We studied the roles of these transcription factors (TFs) at the hTERT promoter in the context of a chromatinized transgenic bacterial artificial chromosome (BAC) reporter

  • The expression of Sp1 and Sp3 did not correlate with hTERT transcription, they both contributed to hTERT transcriptional activation, and their binding sites, the five GC-boxes, were crucial for the hTERT promoter function

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Summary

Introduction

Regulation of telomerase gene (hTERT) by Sp1 family proteins remains contradictory in previous studies. Results: In chromatinized BAC reporters, Sp1/Sp3 binding to the promoter was essential for hTERT transcription, but did not affect its repression.

Results
Conclusion

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