TBP2是非洲爪蟾卵母细胞转录中TBP的替代物。

TBP2 is a substitute for TBP in Xenopus oocyte transcription.

作者信息

Akhtar Waseem, Veenstra Gert Jan C

机构信息

Department of Molecular Biology, Faculty of Science, Nijmegen Centre for Molecular Life Sciences, Radboud University Nijmegen, The Netherlands.

出版信息

BMC Biol. 2009 Aug 3;7:45. doi: 10.1186/1741-7007-7-45.

DOI:10.1186/1741-7007-7-45

PMID:19650908

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2731028/

Abstract

BACKGROUND

TATA-box-binding protein 2 (TBP2/TRF3) is a vertebrate-specific paralog of TBP that shares with TBP a highly conserved carboxy-terminal domain and the ability to bind the TATA box. TBP2 is highly expressed in oocytes whereas TBP is more abundant in embryos.

RESULTS

We find that TBP2 is proteolytically degraded upon meiotic maturation; after germinal vesicle breakdown relatively low levels of TBP2 expression persist. Furthermore, TBP2 localizes to the transcriptionally active loops of lampbrush chromosomes and is recruited to a number of injected promoters in oocyte nuclei. Using an altered binding specificity mutant reporter system we show that TBP2 promotes RNA polymerase II transcription in vivo. Intriguingly, TBP, which in oocytes is undetectable at the protein level, can functionally replace TBP2 when ectopically expressed in oocytes, showing that switching of initiation factors can be driven by changes in their expression. Proteolytic degradation of TBP2 is not required for repression of transcription during meiotic maturation, suggesting a redundant role in this repression or a role in initiation factor switching between oocytes and embryos.

CONCLUSION

The expression and transcriptional activity of TBP2 in oocytes show that TBP2 is the predominant initiation factor in oocytes, which is substituted by TBP on a subset of promoters in embryos as a result of proteolytic degradation of TBP2 during meiotic maturation.

摘要

背景

TATA盒结合蛋白2（TBP2/TRF3）是TBP的脊椎动物特异性旁系同源物，与TBP共享高度保守的羧基末端结构域以及结合TATA盒的能力。TBP2在卵母细胞中高度表达，而TBP在胚胎中更为丰富。

结果

我们发现TBP2在减数分裂成熟时会被蛋白水解降解；在生发泡破裂后，TBP2的表达水平相对较低仍会持续存在。此外，TBP2定位于灯刷染色体的转录活性环，并被招募到卵母细胞核中多个注射的启动子上。使用改变结合特异性的突变报告系统，我们表明TBP2在体内促进RNA聚合酶II转录。有趣的是，在卵母细胞中蛋白水平无法检测到的TBP，当在卵母细胞中异位表达时可以在功能上替代TBP2，这表明起始因子的切换可以由它们表达的变化驱动。减数分裂成熟期间转录抑制并不需要TBP2的蛋白水解降解，这表明其在这种抑制中具有冗余作用或在卵母细胞和胚胎之间的起始因子切换中起作用。

结论

TBP2在卵母细胞中的表达和转录活性表明，TBP2是卵母细胞中的主要起始因子，由于减数分裂成熟期间TBP2的蛋白水解降解，胚胎中一部分启动子上的TBP2被TBP替代。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ea59/2731028/d367493d644e/1741-7007-7-45-1.jpg

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TBP2是非洲爪蟾卵母细胞转录中TBP的替代物。

TBP2 is a substitute for TBP in Xenopus oocyte transcription.

作者信息

Akhtar Waseem, Veenstra Gert Jan C

机构信息

Department of Molecular Biology, Faculty of Science, Nijmegen Centre for Molecular Life Sciences, Radboud University Nijmegen, The Netherlands.