A dual-purpose polymerase engineered for direct sequencing of pseudouridine and queuosine

Author:

Huber Luisa B1,Kaur Navpreet2,Henkel Melanie1,Marchand Virginie3,Motorin Yuri4,Ehrenhofer-Murray Ann E2,Marx Andreas1ORCID

Affiliation:

1. Department of Chemistry, Konstanz Research School Chemical Biology, University of Konstanz , Universitätsstraße 10, 78464 Konstanz , Germany

2. Institut für Biologie, Humboldt-Universität zu Berlin , Philippstraße 13, Rhoda-Erdmann-Haus, 10099 Berlin , Germany

3. Epitranscriptomics and RNA Sequencing Core Facility, Université de Lorraine, CNRS, INSERM, IBSLor (UAR2008/US40) , F- 54000 Nancy , France

4. Université de Lorraine, CNRS, IMoPA (UMR7365) , F- 54000 Nancy , France

Abstract

Abstract More than 170 posttranscriptional RNA modifications are so far known on both coding and noncoding RNA species. Within this group, pseudouridine (Ψ) and queuosine (Q) represent conserved RNA modifications with fundamental functional roles in regulating translation. Current detection methods of these modifications, which both are reverse transcription (RT)-silent, are mostly based on the chemical treatment of RNA prior to analysis. To overcome the drawbacks associated with indirect detection strategies, we have engineered an RT-active DNA polymerase variant called RT-KTq I614Y that produces error RT signatures specific for Ψ or Q without prior chemical treatment of the RNA samples. Combining this polymerase with next-generation sequencing techniques allows the direct identification of Ψ and Q sites of untreated RNA samples using a single enzymatic tool.

Funder

Deutsche Forschungsgemeinschaft

University of Konstanz

Publisher

Oxford University Press (OUP)

Subject

Genetics

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