Topologically correct synthetic reconstruction of pathogen social behavior found in deep tissue sites

Clark, Stacie; Thibault, Derek; Shull, Lauren M.; Davis, Kimberly M.; Aunins, Emily; Opijnen, Tim van; Isberg, Ralph R.

doi:10.1101/2020.04.27.065144

Cited by 1 publication

(2 citation statements)

References 41 publications

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“…In comparison with TIMER42, hmp reporter signal was significantly enriched at the periphery (Fig 7B). This hmp reporter signal pattern was consistent with our previously published results (22,26,37) but suggested that NO stress was not significantly slowing bacterial growth within host tissues, based on TIMER42 signal accumulation in some, but not all, peripheral cells. Representative images indicate there was substantial overlap between dps and TIMER42 signals, and that hmp and TIMER42 are detecting distinct subsets of bacteria (Fig 7C).…”

Section: Timer42 Signal Correlates With Dps Expression In Vivosupporting

confidence: 92%

“…Cultures of the TIMER42 Phmp::gfp and TIMER42 Phmp::gfp-ssrA strains were exposed to 2.5mM DETA-NONOate for 4h, and fluorescence microscopy was used to detect fluorescent signals within individual bacterial cells. The 2.5mM dose was chosen for these experiments based on our previous studies, which showed this dose is sufficient to promote hmp reporter expression (22,26,37). Treatment with the NO donor compound resulted in high levels of hmp reporter expression with both strains (Fig 6A), and TIMER42 signal accumulation (Fig 6B).…”

Section: No Stress Is Sufficient To Promote Timer42 Signal Accumulationmentioning

confidence: 99%

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Modifying TIMER, a slow-folding DsRed derivative, for optimal use in quickly-dividing bacteria

Patel

O’Hara

Aunins

et al. 2021

Preprint

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It is now well appreciated that members of pathogenic bacterial populations exhibit heterogeneity in growth rates and metabolic activity, and it is known this can impact the ability to eliminate all members of the bacterial population during antibiotic treatment. It remains unclear which pathways promote slowed bacterial growth within host tissues, primarily because it has been difficult to identify and isolate slow growing bacteria from host tissues for downstream analyses. To overcome this limitation, we have developed a novel variant of TIMER, a slow-folding fluorescent protein, to identify subsets of slowly dividing bacteria within host tissues. The original TIMER folds too slowly for fluorescence accumulation in quickly replicating bacterial species (Escherichia coli, Yersinia pseudotuberculosis), however this TIMER42 variant accumulates signal in late stationary phase cultures of E. coli and Y. pseudotuberculosis. We show TIMER42 signal also accumulates during exposure to sources of nitric oxide (NO), suggesting TIMER42 signal detects growth-arrested bacterial cells. In a mouse model of Y. pseudotuberculosis deep tissue infection, TIMER42 signal is clearly detected, and primarily accumulates in bacteria expressing markers of stationary phase growth. There was not significant overlap between TIMER42 signal and NO-exposed subpopulations of bacteria within host tissues, suggesting NO stress was transient, allowing bacteria to recover from this stress and resume replication. This novel TIMER42 variant represents a new faster folding TIMER that will enable additional studies of slow-growing subpopulations of bacteria, specifically within bacterial species that quickly divide.Author SummaryWe have generated a variant of TIMER that can be used to mark slow-growing subsets of Yersinia pseudotuberculosis, which has a relatively short division time, similar to E. coli. We used a combination of site-directed and random mutagenesis to generate the TIMER42 variant, which has red fluorescent signal accumulation in post-exponential or stationary phase cells. We found that nitric oxide (NO) stress is sufficient to promote TIMER42 signal accumulation in culture, however within host tissues, TIMER42 signal correlates with a stationary phase reporter (dps). These results suggest NO may cause an immediate arrest in bacterial cell division, but during growth in host tissues exposure to NO is transient, allowing bacteria to recover from this stress and resume cell division. Thus instead of indicating a response to host stressors, TIMER42 signal accumulation within host tissues appears to identify slow-growing cells that are experiencing nutrient limitation.

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Section: Timer42 Signal Correlates With Dps Expression In Vivosupporting

confidence: 92%

Section: No Stress Is Sufficient To Promote Timer42 Signal Accumulationmentioning

confidence: 99%

Modifying TIMER, a slow-folding DsRed derivative, for optimal use in quickly-dividing bacteria

Patel

O’Hara

Aunins

et al. 2021

Preprint

Self Cite

View full text Add to dashboard Cite

show abstract

Topologically correct synthetic reconstruction of pathogen social behavior found in deep tissue sites

Cited by 1 publication

References 41 publications

Modifying TIMER, a slow-folding DsRed derivative, for optimal use in quickly-dividing bacteria

Modifying TIMER, a slow-folding DsRed derivative, for optimal use in quickly-dividing bacteria

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