Epitranscriptomics, the study of chemical modifications on RNA molecules, plays a crucial role in elucidating the regulatory mechanisms involved in post-transcriptional gene expression. Dihydrouridine (D) has garnered significant attention due to its potential impact on RNA structure and function. In this master thesis, we explore the transcriptome-wide occupancy of D within the model organism Schizosaccharomyces pombe and compare the efficacy of the labor-intensive recent method Rho-Seq with nanopore sequencing. Indeed, Rho-seq presents certain limitations, including slow processing, variability, and complex procedural steps. These drawbacks hinder the efficiency and accuracy of D detection.
On the other hand, nanopore sequencing, a state-of-the-art technology in the field of epitranscriptomics, offers numerous advantages over conventional techniques such as an enhanced sensitivity, enabling the detection of low-abundance D modifications but also the reduction of the processing time by eliminating the multiple-steps protocol involved in primer extension and Rho-sequencing and the potential of long-read sequencing, allowing for the identification of D modifications in full-length RNA molecules beyond tRNAs, particularly challenging to achieve using other methods.
| la date de réponse | 15 janv. 2024 |
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| langue originale | Anglais |
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| L'institution diplômante | |
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| Superviseur | Carlo Yague-Sanz (Promoteur) |
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Studying the detection and distribution of an epitranscriptomic mark: Dihydrouridine with nanopore sequencing: a new method for the detection of RNA modifications
LOMBARD, P. (Auteur). 15 janv. 2024
Student thesis: Master types › Master en biochimie et biologie moléculaire et cellulaire à finalité didactique