Literature DB >> 7651406

RNA polymerase III transcription in synthetic nuclei assembled in vitro from defined DNA templates.

K S Ullman1, D J Forbes.   

Abstract

Although much is known of the basic control of transcription, little is understood of the way in which the structural organization of the nucleus affects transcription. Synthetic nuclei, assembled de novo in extracts of Xenopus eggs, would be predicted to have a large potential for approaching the role of nuclear structure in RNA biogenesis. Synthetic nuclei provide a system in which the genetic content of the nuclei, as well as the structural and enzymatic proteins within the nuclei, can be manipulated. In this study, we have begun to examine transcription in such nuclei by using the most simple of templates, RNA polymerase III (pol III)-transcribed genes. DNA encoding tRNA or 5S genes was added to an assembly extract, and nuclei were formed entirely from the pol III templates. Conditions which allowed nuclear assembly and pol III transcription to take place efficiently and simultaneously in the assembly extract were found. To examine whether pol III transcription could initiate within synthetic nuclei, or instead was inhibited in nuclei and initiated only on rare unincorporated templates, we identified transcriptional inhibitors that were excluded from nuclei. We found that these inhibitors, heparin and dextran sulfate, blocked pol III transcription in the absence of assembly but did not do so following nuclear assembly. At the concentrations used, the inhibitors had no deleterious effect on nuclear structure itself or on nuclear import. We conclude that pol III transcription is active in synthetic nuclei, and this conclusion is further strengthened by the finding that pol III transcripts could be coisolated with synthetic nuclei. The rapid and direct transcriptional analysis possible with pol III templates, coupled with the simple experimental criteria developed in this study for distinguishing between nuclear and non-nuclear transcription, should now allow a molecular analysis of the effect of nuclear structure on transcriptional and posttranscriptional control.

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Year:  1995        PMID: 7651406      PMCID: PMC230733          DOI: 10.1128/MCB.15.9.4873

Source DB:  PubMed          Journal:  Mol Cell Biol        ISSN: 0270-7306            Impact factor:   4.272


  88 in total

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5.  Mitotic repression of RNA polymerase III transcription in vitro mediated by phosphorylation of a TFIIIB component.

Authors:  J M Gottesfeld; V J Wolf; T Dang; D J Forbes; P Hartl
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  7 in total

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2.  Nuclear localization signal peptides induce molecular delivery along microtubules.

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3.  Analysis of nuclear reconstitution, nuclear envelope assembly, and nuclear pore assembly using Xenopus in vitro assays.

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Review 4.  Non-genetic contributions of the sperm nucleus to embryonic development.

Authors:  Yasuhiro Yamauchi; Jeffrey A Shaman; W Steven Ward
Journal:  Asian J Androl       Date:  2010-10-18       Impact factor: 3.285

5.  Major binding sites for the nuclear import receptor are the internal nucleoporin Nup153 and the adjacent nuclear filament protein Tpr.

Authors:  S Shah; S Tugendreich; D Forbes
Journal:  J Cell Biol       Date:  1998-04-06       Impact factor: 10.539

6.  Transportin regulates major mitotic assembly events: from spindle to nuclear pore assembly.

Authors:  Corine K Lau; Valerie A Delmar; Rene C Chan; Quang Phung; Cyril Bernis; Boris Fichtman; Beth A Rasala; Douglass J Forbes
Journal:  Mol Biol Cell       Date:  2009-07-29       Impact factor: 4.138

7.  Xenopus importin beta validates human importin beta as a cell cycle negative regulator.

Authors:  Valerie A Delmar; Rene C Chan; Douglass J Forbes
Journal:  BMC Cell Biol       Date:  2008-03-22       Impact factor: 4.241

  7 in total

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