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A genetic assay for transcription errors reveals multilayer control of RNA polymerase II fidelity.


ABSTRACT: We developed a highly sensitive assay to detect transcription errors in vivo. The assay is based on suppression of a missense mutation in the active site tyrosine in the Cre recombinase. Because Cre acts as tetramer, background from translation errors are negligible. Functional Cre resulting from rare transcription errors that restore the tyrosine codon can be detected by Cre-dependent rearrangement of reporter genes. Hence, transient transcription errors are captured as stable genetic changes. We used this Cre-based reporter to screen for mutations of Saccharomyces cerevisiae RPB1 (RPO21) that increase the level of misincorporation during transcription. The mutations are in three domains of Rpb1, the trigger loop, the bridge helix, and in sites involved in binding to TFIIS. Biochemical characterization demonstrates that these variants have elevated misincorporation, and/or ability to extend mispaired bases, or defects in TFIIS mediated editing.

SUBMITTER: Irvin JD 

PROVIDER: S-EPMC4168980 | biostudies-literature | 2014 Sep

REPOSITORIES: biostudies-literature

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A genetic assay for transcription errors reveals multilayer control of RNA polymerase II fidelity.

Irvin Jordan D JD   Kireeva Maria L ML   Gotte Deanna R DR   Shafer Brenda K BK   Huang Ingold I   Kashlev Mikhail M   Strathern Jeffrey N JN  

PLoS genetics 20140918 9


We developed a highly sensitive assay to detect transcription errors in vivo. The assay is based on suppression of a missense mutation in the active site tyrosine in the Cre recombinase. Because Cre acts as tetramer, background from translation errors are negligible. Functional Cre resulting from rare transcription errors that restore the tyrosine codon can be detected by Cre-dependent rearrangement of reporter genes. Hence, transient transcription errors are captured as stable genetic changes.  ...[more]

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