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CRISPR/Cas9 recombineering-mediated deep mutational scanning of essential genes in Escherichia coli

  • Alaksh Choudhury
  • , Jacob A. Fenster
  • , Reilly G. Fankhauser
  • , Joel L. Kaar
  • , Olivier Tenaillon
  • , Ryan T. Gill
  • University of Colorado
  • Laboratoire de Probabilités et Modèles Aléatoires
  • University of Colorado Boulder
  • Danish Technical University

Résultats de recherche: Contribution à un journalArticleRevue par des pairs

Résumé

Deep mutational scanning can provide significant insights into the function of essential genes in bacteria. Here, we developed a high-throughput method for mutating essential genes of Escherichia coli in their native genetic context. We used Cas9-mediated recombineering to introduce a library of mutations, created by error-prone PCR, within a gene fragment on the genome using a single gRNA pre-validated for high efficiency. Tracking mutation frequency through deep sequencing revealed biases in the position and the number of the introduced mutations. We overcame these biases by increasing the homology arm length and blocking mismatch repair to achieve a mutation efficiency of 85% for non-essential genes and 55% for essential genes. These experiments also improved our understanding of poorly characterized recombineering process using dsDNA donors with single nucleotide changes. Finally, we applied our technology to target rpoB, the beta subunit of RNA polymerase, to study resistance against rifampicin. In a single experiment, we validate multiple biochemical and clinical observations made in the previous decades and provide insights into resistance compensation with the study of double mutants.

langue originaleAnglais
Numéro d'articlee9265
journalMolecular Systems Biology
Volume16
Numéro de publication3
Les DOIs
étatPublié - 1 mars 2020
Modification externeOui

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