2013
DOI: 10.1371/journal.pone.0080597
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Simultaneous Transcriptional Profiling of Bacteria and Their Host Cells

Abstract: We developed an RNA-Seq-based method to simultaneously capture prokaryotic and eukaryotic expression profiles of cells infected with intracellular bacteria. As proof of principle, this method was applied to Chlamydia trachomatis-infected epithelial cell monolayers in vitro, successfully obtaining transcriptomes of both C. trachomatis and the host cells at 1 and 24 hours post-infection. Chlamydiae are obligate intracellular bacterial pathogens that cause a range of mammalian diseases. In humans chlamydiae are r… Show more

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Cited by 117 publications
(137 citation statements)
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References 110 publications
(142 reference statements)
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“…103 Host factors associated with scar formation and other fibrotic conditions were also recently reported as being released from epithelial cell monolayers as soon as 1 hour postinfection with C. trachomatis serovar E, and these findings have formed the basis of a hypothesis involving multiple feedback loops to explain Chlamydia-induced fibrotic scarring of fallopian tubes. 104,105 These explanations for the pathology induced by chlamydial infections add to previous work showing an involvement of heat shock protein 60 and a proposed model of molecular mimicry which has been discussed extensively by Hafner.…”
supporting
confidence: 60%
“…103 Host factors associated with scar formation and other fibrotic conditions were also recently reported as being released from epithelial cell monolayers as soon as 1 hour postinfection with C. trachomatis serovar E, and these findings have formed the basis of a hypothesis involving multiple feedback loops to explain Chlamydia-induced fibrotic scarring of fallopian tubes. 104,105 These explanations for the pathology induced by chlamydial infections add to previous work showing an involvement of heat shock protein 60 and a proposed model of molecular mimicry which has been discussed extensively by Hafner.…”
supporting
confidence: 60%
“…The ubiquitous polyadenylation of eukaryotic mRNAs and the sequence similarity of ribosomal transcripts facilitates the experimental protocol as it enables the poly(A) enrichment or ribosomal depletion for host and pathogen in a single step. Recently a few publications have reported the application of RNA-seq to a model of bacterial infection of plant leaves (Asai et al, 2014;Socquet-Juglard et al, 2013), porcine enterocytes (Vannucci et al, 2013), or human epithelial carcinoma cells (Humphrys et al, 2013). However, these suffered from the lack of an enrichment of invaded cells, resulting in a low bacterial transcriptome coverage, and/or from a shallow sequencing depth, hampering an in-depth profiling of the host response.…”
Section: Dual Rna-seq: Potential and Scope For Future Improvementsmentioning
confidence: 99%
“…Gene expression profiling with RNA-seq is consistent with results obtained by microarrays (Liu et al 2007;Marioni et al 2008;Bradford et al 2010;Malone and Oliver 2011) but is significantly more sensitive, with a much greater dynamic range (Wang et al 2009). These traits and the probe-independent nature of RNAseq make it possible to analyze the transcriptomes of multiple species (e.g., pathogen and host) simultaneously (Tierney et al 2012;Westermann et al 2012;Humphrys et al 2013).…”
mentioning
confidence: 99%