Characterizing the Escherichia coli O157:H7 Proteome Including Protein Associations with Higher Order Assemblies

Pieper, Rembert; Zhang, Quanshun; Clark, David; Huang, Shih Ting; Suh, Moo-Jin; Braisted, John C.; Payne, Samuel H.; Fleischmann, Robert; Peterson, Scott N.; Tzipori, Saul

doi:10.1371/journal.pone.0026554

Cited by 22 publications

(29 citation statements)

References 80 publications

(100 reference statements)

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“…Nano-electrospray into the source was followed by mass analysis and spectral acquisition in automated MS/MS mode, with the top five parent ions selected for fragmentation in scans of the m/z range 350–2,000 and a dynamic exclusion setting of 90 sec. The LC-MS/MS workflow using the LTQ-XL ion trap system (Thermo Fisher Scientific) was previously described in more detail [34]. The instrument was calibrated prior to performance of LC-MS/MS experiments with 200 nmol human [Glu 1 -fibrinopeptide B (M.W.…”

Section: Methodsmentioning

confidence: 99%

Integrated next-generation sequencing of 16S rDNA and metaproteomics differentiate the healthy urine microbiome from asymptomatic bacteriuria in neuropathic bladder associated with spinal cord injury

et al. 2012

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BackgroundClinical dogma is that healthy urine is sterile and the presence of bacteria with an inflammatory response is indicative of urinary tract infection (UTI). Asymptomatic bacteriuria (ABU) represents the state in which bacteria are present but the inflammatory response is negligible. Differentiating ABU from UTI is diagnostically challenging, but critical because overtreatment of ABU can perpetuate antimicrobial resistance while undertreatment of UTI can result in increased morbidity and mortality. In this study, we describe key characteristics of the healthy and ABU urine microbiomes utilizing 16S rRNA gene (16S rDNA) sequencing and metaproteomics, with the future goal of utilizing this information to personalize the treatment of UTI based on key individual characteristics.MethodsA cross-sectional study of 26 healthy controls and 27 healthy subjects at risk for ABU due to spinal cord injury-related neuropathic bladder (NB) was conducted. Of the 27 subjects with NB, 8 voided normally, 8 utilized intermittent catheterization, and 11 utilized indwelling Foley urethral catheterization for bladder drainage. Urine was obtained by clean catch in voiders, or directly from the catheter in subjects utilizing catheters. Urinalysis, urine culture and 16S rDNA sequencing were performed on all samples, with metaproteomic analysis performed on a subsample.ResultsA total of 589454 quality-filtered 16S rDNA sequence reads were processed through a NextGen 16S rDNA analysis pipeline. Urine microbiomes differ by normal bladder function vs. NB, gender, type of bladder catheter utilized, and duration of NB. The top ten bacterial taxa showing the most relative abundance and change among samples were Lactobacillales, Enterobacteriales, Actinomycetales, Bacillales, Clostridiales, Bacteroidales, Burkholderiales, Pseudomonadales, Bifidobacteriales and Coriobacteriales. Metaproteomics confirmed the 16S rDNA results, and functional human protein-pathogen interactions were noted in subjects where host defenses were initiated.ConclusionsCounter to clinical belief, healthy urine is not sterile. The healthy urine microbiome is characterized by a preponderance of Lactobacillales in women and Corynebacterium in men. The presence and duration of NB and method of urinary catheterization alter the healthy urine microbiome. An integrated approach of 16S rDNA sequencing with metaproteomics improves our understanding of healthy urine and facilitates a more personalized approach to prevention and treatment of infection.

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Section: Methodsmentioning

confidence: 99%

Integrated next-generation sequencing of 16S rDNA and metaproteomics differentiate the healthy urine microbiome from asymptomatic bacteriuria in neuropathic bladder associated with spinal cord injury

et al. 2012

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“…Lysates in TTE buffer were thawed, supplemented with chicken lysozyme (150 g/ml), and agitated at 20°C for 1 h. Protein extraction and size exclusion chromatography (SEC) steps were essentially performed as described previously (49), with the exception that only two SEC protein fractions were collected, one in the mass range above 15 kDa and the other lower than 15 kDa. Based on SDS-PAGE analysis, the lower SEC mass fraction contained most of the lysozyme and was discarded.…”

Section: Methodsmentioning

confidence: 99%

Analysis of the Proteome of Intracellular Shigella flexneri Reveals Pathways Important for Intracellular Growth

et al. 2013

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Global proteomic analysis was performed with Shigella flexneri strain 2457T in association with three distinct growth environments: S. flexneri growing in broth (in vitro), S. flexneri growing within epithelial cell cytoplasm (intracellular), and S. flexneri that were cultured with, but did not invade, Henle cells (extracellular). Compared to in vitro and extracellular bacteria, intracellular bacteria had increased levels of proteins required for invasion and cell-to-cell spread, including Ipa, Mxi, and Ics proteins. Changes in metabolic pathways in response to the intracellular environment also were evident. There was an increase in glycogen biosynthesis enzymes, altered expression of sugar transporters, and a reduced amount of the carbon storage regulator CsrA. Mixed acid fermentation enzymes were highly expressed intracellularly, while tricarboxylic acid (TCA) cycle oxidoreductive enzymes and most electron transport chain proteins, except CydAB, were markedly decreased. This suggested that fermentation and the CydAB system primarily sustain energy generation intracellularly. Elevated levels of PntAB, which is responsible for NADPH regeneration, suggested a shortage of reducing factors for ATP synthesis. These metabolic changes likely reflect changes in available carbon sources, oxygen levels, and iron availability. Intracellular bacteria showed strong evidence of iron starvation. Iron acquisition systems (Iut, Sit, FhuA, and Feo) and the iron starvation, stress-associated Fe-S cluster assembly (Suf) protein were markedly increased in abundance. Mutational analysis confirmed that the mixed-acid fermentation pathway was required for wild-type intracellular growth and spread of S. flexneri. Thus, iron stress and changes in carbon metabolism may be key factors in the S. flexneri transition from the extra-to the intracellular milieu.

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“…It is also noteworthy that studies of closely related bacterial pathogens (i.e., Escherichia coli or Shigella spp.) have expanded our knowledge on bacterial adaptations upon interactions with their host cells (20,21,22,23,24,25). For instance, Pieper et al studied the Shigella flexneri proteome within infected epithelial cells (24).…”

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Proteomic Analyses of Intracellular Salmonella enterica Serovar Typhimurium Reveal Extensive Bacterial Adaptations to Infected Host Epithelial Cells

Liu

Zhang

et al. 2015

Infect Immun

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Salmonella species can gain access into nonphagocytic cells, where the bacterium proliferates in a unique membrane-bounded compartment. In order to reveal bacterial adaptations to their intracellular niche, here we conducted the first comprehensive proteomic survey of Salmonella isolated from infected epithelial cells. Among ϳ3,300 identified bacterial proteins, we found that about 100 proteins were significantly altered at the onset of Salmonella intracellular replication. In addition to substantially increased iron-uptake capacities, bacterial high-affinity manganese and zinc transporters were also upregulated, suggesting an overall limitation of metal ions in host epithelial cells. We also found that Salmonella induced multiple phosphate utilization pathways. Furthermore, our data suggested upregulation of the two-component PhoPQ system as well as of many downstream virulence factors under its regulation. Our survey also revealed that intracellular Salmonella has increased needs for certain amino acids and biotin. In contrast, Salmonella downregulated glycerol and maltose utilization as well as chemotaxis pathways. While infectious diseases continue to be a major threat to human health, there is an urgent need in rational design and development of new treatment strategies. As a model for studying bacterial pathogenesis, Salmonella spp. cause millions of infections per year ranging from food poisoning to life-threatening systemic typhoid fever (1). Central to its pathogenesis is a syringelike structure known as the type III secretion system (T3SS), which delivers bacterial proteins called effectors directly into eukaryotic host cells (2, 3). The injected proteins are able to modulate various host cellular functions, and over the years extensive studies have been carried out on these effector proteins and/or their interacting host targets. While these studies have contributed substantially to our initial understanding of infection biology, daunting challenges are encountered because conventional reductionism-based studies certainly cannot explain the complex multifactorial nature of host-pathogen interactions (4). Systems-level analyses can provide a panoramic view of the functional host-pathogen interplay and thus are promising in this regard.During infection, the intracellular environment is likely to be very different from what bacteria encounter in rich culture media. It has long been known that various nutritional and environmental differences within host cells force bacterial pathogens to reprogram their gene expression. In fact, transcriptomic studies of intracellular Salmonella within infected macrophages and epithelial cells contributed to our initial understanding of bacterial adaptations in the host environment (5, 6). Because proteins are the final gene products and their changes may not correlate with those of mRNA, direct readout of the bacterial proteome is highly desired. Such measurements, however, have been technically challenging due to the presence of vast amounts of host proteins (7). As a ...

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Characterizing the Escherichia coli O157:H7 Proteome Including Protein Associations with Higher Order Assemblies

Cited by 22 publications

References 80 publications

Integrated next-generation sequencing of 16S rDNA and metaproteomics differentiate the healthy urine microbiome from asymptomatic bacteriuria in neuropathic bladder associated with spinal cord injury

Integrated next-generation sequencing of 16S rDNA and metaproteomics differentiate the healthy urine microbiome from asymptomatic bacteriuria in neuropathic bladder associated with spinal cord injury

Analysis of the Proteome of Intracellular Shigella flexneri Reveals Pathways Important for Intracellular Growth

Proteomic Analyses of Intracellular Salmonella enterica Serovar Typhimurium Reveal Extensive Bacterial Adaptations to Infected Host Epithelial Cells

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