Implications of stx loss for clinical diagnostics of Shiga toxin-producing Escherichia coli

Senthakumaran, Thulasika; Brandal, Lin Thorstensen; Lindstedt, Bjørn-Arne; Jørgensen, Silje Bakken; Charnock, Colin; Tunsjø, Hege Smith

doi:10.1007/s10096-018-3384-6

Cited by 20 publications

(23 citation statements)

References 34 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…In addition, the presence of multiple fragments of stx-coding phages may be related to the loss of phages by sub-cultivation, which has already been demonstrated [15,16,38,51]. Based on our results, we would agree with Senthakumaran et al [38] who concluded that STEC with intact prophages may be uncommon and difficult to detect. Also, using WGS these authors observed the existence of a stx-negative "in vivo" strain O145:H28 with characteristics similar to another STEC strain of the same serotype [38].…”

Section: Plos Onesupporting

confidence: 91%

“…Environments with a high bacterial density promote transfer of phages, with phages being both gained and lost by bacterial members within this dynamic environment [50]. In addition, the presence of multiple fragments of stx-coding phages may be related to the loss of phages by sub-cultivation, which has already been demonstrated [15,16,38,51]. Based on our results, we would agree with Senthakumaran et al [38] who concluded that STEC with intact prophages may be uncommon and difficult to detect.…”

Section: Plos Onesupporting

confidence: 89%

“…Possibly, amplification of a free stx-encoding phage may have occurred at initial isolation as the two Citrobacter isolated in the present study did not have stx-encoding phage fragments in their genomes. Other PCR-based studies of E. coli have also either detected free stx-encoding phages or hypothesized the loss of stx after sub-cultivation [13,16,38]. Free stx-phages have been found in Citrobacter spp.…”

Section: Isolation Of Citrobacter Sppmentioning

confidence: 99%

See 2 more Smart Citations

Inconsistent PCR detection of Shiga toxin-producing Escherichia coli: Insights from whole genome sequence analyses

et al. 2021

View full text Add to dashboard Cite

Shiga toxin-producing Escherichia coli (STEC) have been linked to food-borne disease outbreaks. As PCR is routinely used to screen foods for STEC, it is important that factors leading to inconsistent detection of STEC by PCR are understood. This study used whole genome sequencing (WGS) to investigate causes of inconsistent PCR detection of stx1, stx2, and serogroup-specific genes. Fifty strains isolated from Alberta feedlot cattle from three different studies were selected with inconsistent or consistent detection of stx and serogroup by PCR. All isolates were initially classified as STEC by PCR. Sequencing was performed using Illumina MiSeq® with sample library by Nextera XT. Virtual PCRs were performed using Geneious and bacteriophage content was determined using PHASTER. Sequencing coverage ranged from 47 to 102x, averaging 74x, with sequences deposited in the NCBI database. Eleven strains were confirmed by WGS as STEC having complete stxA and stxB subunits. However, truncated stx fragments occurred in twenty-two other isolates, some having multiple stx fragments in the genome. Isolates with complete stx by WGS had consistent stx1 and stx2 detection by PCR, although one also having a stx2 fragment had inconsistent stx2 PCR. For all STEC and 18/39 non-STEC, serogroups determined by PCR agreed with those determined by WGS. An additional three WGS serotypes were inconclusive and two isolates were Citrobacter spp. Results demonstrate that stx fragments associated with stx-carrying bacteriophages in the E. coli genome may contribute to inconsistent detection of stx1 and stx2 by PCR. Fourteen isolates had integrated stx bacteriophage but lacked complete or fragmentary stx possibly due to partial bacteriophage excision after sub-cultivation or other unclear mechanisms. The majority of STEC isolates (7/11) did not have identifiable bacteriophage DNA in the contig(s) where stx was located, likely increasing the stability of stx in the bacterial genome and its detection by PCR.

show abstract

Section: Plos Onesupporting

confidence: 91%

Section: Plos Onesupporting

confidence: 89%

Section: Isolation Of Citrobacter Sppmentioning

confidence: 99%

See 1 more Smart Citation

Inconsistent PCR detection of Shiga toxin-producing Escherichia coli: Insights from whole genome sequence analyses

et al. 2021

View full text Add to dashboard Cite

show abstract

“…In this study, it was possible to detect two samples with free Stx phage particles (3.8% of PCR-positive/culture-negative samples) in CFS but with the use of PMA-qPCR it was also possible to identify dead cells in the samples, together with free Stx particles and inducible Stx phages in two samples (3.8%) and in eight samples with inducible Stx phages (15.1%) (Figure 2b), further demonstrating the differing causes for culture negative samples. The stx1 and stx2 genes are mobile virulence factors, located on the genome of temperate bacteriophages [46][47][48][49] which are able to integrate in the E.coli genome during lysogeny, resulting in The stx1 and stx2 genes are mobile virulence factors, located on the genome of temperate bacteriophages [46][47][48][49] which are able to integrate in the E.coli genome during lysogeny, resulting in acquired ability to express the Shiga toxin [29]; however, the prophages can be induced to enter the lytic cycle producing toxin and new phage particles [50]. In this study, mitomycin C was used for the lytic cycle induction in the enriched samples resulting in an increase of number of positive samples for the plaque assay (Table 2, 35 samples).…”

Section: Discussionmentioning

confidence: 99%

Investigation of the Causes of Shigatoxigenic Escherichia coli PCR Positive and Culture Negative Samples

et al. 2020

View full text Add to dashboard Cite

Molecular methods may reveal the presence of pathogens in samples through the detection of specific target gene(s) associated with microorganisms, but often, the subsequent cultural isolation of the pathogen is not possible. This discrepancy may be related to low concentration of the cells, presence of dead cells, competitive microflora, injured cells and cells in a viable but non-culturable state, free DNA and the presence of free bacteriophages which can carry the target gene causing the PCR-positive/culture-negative results. Shiga-toxigenic Escherichia coli (STEC) was used as a model for studying this phenomenon, based on the phage-encoded cytotoxins genes (Stx family) as the detection target in samples through real-time qPCR. Stx phages can be integrated in the STEC chromosome or can be isolated as free particles in the environment. In this study, a combination of PCR with culturing was used for investigating the presence of the stx1 and stx2 genes in 155 ovine recto-anal junction swab samples (method (a)-PCR). Samples which were PCR-positive and culture-negative were subjected to additional analyses including detection of dead STEC cells (method (b)-PCR-PMA dye assay), presence of Stx phages (method (c)-plaque assays) and inducible integrated phages (method (d)-phage induction). Method (a) showed that even though 121 samples gave a PCR-positive result (78%), only 68 samples yielded a culturable isolate (43.9%). Among the 53 (34.2%) PCR-positive/culture-negative samples, 21 (39.6%) samples were shown to have STEC dead cells only, eight (15.1%) had a combination of dead cells and inducible stx phage, while two samples (3.8%) had a combination of dead cells, inducible phage and free stx phage, and a further two samples had Stx1 free phages only (3.8%). It was thus possible to reduce the samples with no explanation to 20 (37.7% of 53 samples), representing a further step towards an improved understanding of the STEC PCR-positive/culture-negative phenomenon.

show abstract

“…Where reservoirs of stxencoding bacteriophage coincide with receptive serogroup backgrounds, there exists the potential for evolution of emergent STEC strains. In particular, O26 stx status is known to be dynamic, with loss and acquisition of stx phage demonstrated in vitro and in vivo(53)(54)(55)(56). Individual pat samples from two herds in our study yielded both stx-negative and positive O26 isolates, suggesting that either the source animal wason March 21, 2021 by guest http://aem.asm.org/ Downloaded from colonised by two differing O26 strains, or by the same strain from which stx genes had been lost or acquired within the gut, or during laboratory culture.…”

mentioning

confidence: 99%

Prevalence and Epidemiology of Non-O157 Escherichia coli Serogroups O26, O103, O111, and O145 and Shiga Toxin Gene Carriage in Scottish Cattle, 2014–2015

Hoyle

Keith

Williamson

et al. 2021

Appl Environ Microbiol

View full text Add to dashboard Cite

Cattle are a reservoir for Shiga toxin-producing Escherichia coli (STEC), zoonotic pathogens that cause serious clinical disease. Scotland has a higher incidence of STEC infection in the human population than the European average. The aim of this study was to investigate the prevalence and epidemiology of non-O157 serogroups O26, O103, O111, O145, and Shiga toxin gene carriage, in Scottish cattle. Faecal samples (n = 2783) were collected from 110 herds between 2014-2015 and screened by real-time PCR. Herd-level prevalence (95% CI) for O103, O26 and O145 was estimated as 0.71 (0.62, 0.79), 0.43 (0.34, 0.52) and 0.23 (0.16, 0.32), respectively. Only two herds were positive for O111. Shiga toxin prevalence was high in both herds and pats, particularly for stx2 (herd-level: 0.99, 95% CI: 0.94, 1.0). O26 bacterial strains were isolated from 36 herds on culture. Fifteen herds yielded O26 stx-positive isolates that additionally harboured the intimin gene; six of these herds shed highly pathogenic stx2a-positive strains. Multiple serogroups were detected in herds and pats, with only 25 herds negative for all serogroups. Despite overlap in detection, regional and seasonal effects were observed. Higher herd prevalence for O26, O103 and stx1 occurred in the South West and this region was significant for stx2 at the pat-level (P = 0.015). Significant seasonal variation was observed for O145 prevalence, highest in autumn (P = 0.032). Negative herds were associated with Central Scotland and winter. Herds positive for all serogroups were associated with autumn, larger herd size and were not housed at sampling. IMPORTANCE Cattle are reservoirs for Shiga toxin Escherichia coli (STEC), bacteria shed in animal faeces. Human are infected through consumption of contaminated food or water, and by direct contact, causing serious disease and kidney failure in the most vulnerable. The contribution of non-O157 serogroups to STEC illness was underestimated for many years, due to the lack of specific tests. Recently non-O157 human cases have increased, with O26 STEC of particular note. It is therefore vital to investigate the level and composition of non-O157 in the cattle reservoir, and compare to historical levels and the clinical situation. In this study we found cattle prevalence high for toxin, as well as O103 and O26 serogroups. Pathogenic O26 STEC were isolated from 14% of study herds, with toxin subtypes similar to that seen in Scottish clinical cases. This study highlights the current risk to public health from non-O157 STEC in Scottish cattle.

show abstract

Implications of stx loss for clinical diagnostics of Shiga toxin-producing Escherichia coli

Cited by 20 publications

References 34 publications

Inconsistent PCR detection of Shiga toxin-producing Escherichia coli: Insights from whole genome sequence analyses

Inconsistent PCR detection of Shiga toxin-producing Escherichia coli: Insights from whole genome sequence analyses

Investigation of the Causes of Shigatoxigenic Escherichia coli PCR Positive and Culture Negative Samples

Prevalence and Epidemiology of Non-O157 Escherichia coli Serogroups O26, O103, O111, and O145 and Shiga Toxin Gene Carriage in Scottish Cattle, 2014–2015

Contact Info

Product

Resources

About