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Whole-Genome Identification of Transcriptional Start Sites by Differential RNA-seq in Bacteria
Umeå University, Faculty of Medicine, Molecular Infection Medicine Sweden (MIMS). Umeå University, Faculty of Medicine, Umeå Centre for Microbial Research (UCMR). Umeå University, Faculty of Medicine, Department of Molecular Biology (Faculty of Medicine). (Andrea Puhar)ORCID iD: 0000-0002-0984-6286
Umeå University, Faculty of Medicine, Molecular Infection Medicine Sweden (MIMS). Umeå University, Faculty of Medicine, Umeå Centre for Microbial Research (UCMR). Umeå University, Faculty of Medicine, Department of Molecular Biology (Faculty of Medicine). (Andrea Puhar)ORCID iD: 0000-0002-9915-002x
2020 (English)In: Bio-protocol, E-ISSN 2331-8325, Vol. 10, no 18, article id e3757Article in journal (Refereed) Published
Abstract [en]

Gene transcription in bacteria often starts some nucleotides upstream of the start codon. Identifying the specific Transcriptional Start Site (TSS) is essential for genetic manipulation, as in many cases upstream of the start codon there are sequence elements that are involved in gene expression regulation. Taken into account the classical gene structure, we are able to identify two kinds of transcriptional start site: primary and secondary. A primary transcriptional start site is located some nucleotides upstream of the translational start site, while a secondary transcriptional start site is located within the gene encoding sequence.Here, we present a step by step protocol for genome-wide transcriptional start sites determination by differential RNA-sequencing (dRNA-seq) using the enteric pathogen Shigella flexneri serotype 5a strain M90T as model. However, this method can be employed in any other bacterial species of choice. In the first steps, total RNA is purified from bacterial cultures using the hot phenol method. Ribosomal RNA (rRNA) is specifically depleted via hybridization probes using a commercial kit. A 5′-monophosphate-dependent exonuclease (TEX)-treated RNA library enriched in primary transcripts is then prepared for comparison with a library that has not undergone TEX-treatment, followed by ligation of an RNA linker adaptor of known sequence allowing the determination of TSS with single nucleotide precision. Finally, the RNA is processed for Illumina sequencing library preparation and sequenced as purchased service. TSS are identified by in-house bioinformatic analysis.Our protocol is cost-effective as it minimizes the use of commercial kits and employs freely available software.

Place, publisher, year, edition, pages
Bio-protocol , 2020. Vol. 10, no 18, article id e3757
Keywords [en]
dRNA-seq, Transcriptional start site, TSS, RNA purification, Hot phenol RNA extraction, rRNA depletion, 5′-monophosphate-dependent exonuclease (TEX), Phenol chloroform:isoamyl alcohol RNA extraction, Bacterial gene regulation, RNA precipitation, RNA phosphorylation
National Category
Microbiology Genetics Bioinformatics and Systems Biology
Research subject
Microbiology
Identifiers
URN: urn:nbn:se:umu:diva-175314DOI: 10.21769/BioProtoc.3757ISI: 000583375100008OAI: oai:DiVA.org:umu-175314DiVA, id: diva2:1470483
Funder
The Kempe Foundations, JCK-1528Knut and Alice Wallenberg Foundation, KAW 2015.0225Available from: 2020-09-24 Created: 2020-09-24 Last updated: 2022-09-15Bibliographically approved

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Cervantes-Rivera, RamónPuhar, Andrea

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Molecular Infection Medicine Sweden (MIMS)Umeå Centre for Microbial Research (UCMR)Department of Molecular Biology (Faculty of Medicine)
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