Characterisation of bacteria in ascites—reporting the potential of culture-independent, molecular analysis

Rogers, Geraint B.; Russell, Lloyd E.; Preston, P. G.; Marsh, Peter; Collins, Jane; Saunders, John; Sutton, John; Fine, David; Bruce, Kenneth D.; Wright, Mark

doi:10.1007/s10096-010-0891-5

Cited by 31 publications

(25 citation statements)

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“…However, recent studies using 16S rRNA-based fingerprinting analyses have shown that ascites may also be polymicrobial (10,11) and that the bacterial spectrum is broader than that previously reported in context with SBP (11).…”

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confidence: 71%

Application of Qualitative and Quantitative Real-Time PCR, Direct Sequencing, and Terminal Restriction Fragment Length Polymorphism Analysis for Detection and Identification of Polymicrobial 16S rRNA Genes in Ascites

Krohn¹,

Böhm²,

Engelmann³

et al. 2014

J Clin Microbiol

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Qualitative and quantitative 16S rRNA gene-based real-time PCR and direct sequencing were applied for rapid detection and identification of bacterial DNA (bactDNA) in 356 ascites samples. bactDNA was detected in 35% of samples, with a mean of 3.24 log copies ml ؊1 . Direct sequencing of PCR products revealed 62% mixed chromatograms predominantly belonging to Grampositive bacteria. Terminal restriction fragment length polymorphism (T-RFLP) results of a sample subset confirmed sequence data showing polymicrobial DNA contents in 67% of bactDNA-positive ascites samples. Spontaneous bacterial peritonitis (SBP) is the most severe bacterial infection in patients with decompensated liver disease (1). As evidenced by culture-based diagnosis, Gram-negative bacteria of the genera Escherichia and Klebsiella are the most frequent cause for SBP (2, 3). However, recent data reveal that also Grampositive bacteria such as Staphylococcus and Enterococcus species may be responsible for bacterial peritonitis, especially in hospitalized patients (4, 5). Since detection rates of classical culture techniques are low in the routine setting, the causative agent remains unknown in many cases of SBP (3).Application of culture-independent PCR-based methods for the detection of bacterial DNA (bactDNA) in ascites has been proposed as a suitable tool to improve pathogen identification in patients at risk for SBP (6) and has indicated that bactDNA derives in most cases from a single pathogen (7-9). However, recent studies using 16S rRNA-based fingerprinting analyses have shown that ascites may also be polymicrobial (10,11) and that the bacterial spectrum is broader than that previously reported in context with SBP (11).Based on these findings, we analyzed a set of ascites samples using primers targeting the 16S rRNA gene for qualitative and quantitative PCR and further characterized bactDNA-positive samples by direct sequencing and terminal restriction fragment length polymorphism (T-RFLP) analysis in order to determine the frequency of detectable bactDNA in ascites from patients with end-stage liver disease and to identify the corresponding bacterial agents.A total of 356 ascites samples from 174 patients with liver cirrhosis (77.6% alcoholic, 11.5% cryptogenic, 2.9% viral hepatitis, 1.7% genetic disorders or metabolic diseases, 1.7% autoimmune hepatitis, 0.6% primary biliary cirrhosis, 3.5% nonalcoholic fatty liver disease, and 0.6% cardiac) were obtained at the University Hospital Leipzig, between February 2011 and December 2012. Thirty-seven percent of the patients (n ϭ 61) underwent several diagnostic paracenteses (mean number of paracenteses, 3.9; range, 2 to 11). All patients gave full written informed consent to the study protocol, which was approved by the local ethics committee.Ascitic fluid samples were routinely analyzed for total leukocyte count using an automated blood cell counter and for the presence of bacterial and fungal pathogens by routine microbiological culture with direct inoculation of agar plates.For culture-independe...

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confidence: 71%

Application of Qualitative and Quantitative Real-Time PCR, Direct Sequencing, and Terminal Restriction Fragment Length Polymorphism Analysis for Detection and Identification of Polymicrobial 16S rRNA Genes in Ascites

Krohn¹,

Böhm²,

Engelmann³

et al. 2014

J Clin Microbiol

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“…Following incubation, pellets were exposed to light for 10 min using an LED Active Blue equipment light source (Ingenia Biosystems, Terrassa, Spain). Total DNA extraction was then performed as described previously [13]. Full details of the protocol used are provided as Methods S1.…”

Section: Methodsmentioning

confidence: 99%

“…This assay was described previously [24], and applied in the analysis of ascites [13]. Full details of the protocol used are provided as Methods S1.…”

Section: Methodsmentioning

confidence: 99%

“…Here, approaches typically exploit the phylogenetically informative 16S ribosomal RNA gene, and include quantitative (Q) PCR (a means of determining bacterial load) and pyrosequencing (a massive parallel sequencing approach that allows the rapid, high depth characterisation of bacterial composition). Such approaches have been applied across a wide range of clinical contexts, including the analysis of intestinal microbial communities of cirrhotic patients [12], and the identification of bacterial species present in ascites [13] (although the presented study is the first reported use of pyrosequencing in this context). However, whilst having the potential to be greatly informative, such molecular techniques are weakened by their inability to distinguish between DNA present in viable bacterial cells, from that present in dead bacteria or in the extracellular environment.…”

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confidence: 99%

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Ascitic Microbiota Composition Is Correlated with Clinical Severity in Cirrhosis with Portal Hypertension

et al. 2013

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Identification of pathogenic bacteria in ascites correlates with poor clinical outcomes. Ascites samples are commonly reported culture-negative, even where frank infection is indicated. Culture-independent methods have previously reported bacterial DNA in ascites, however, whether this represents viable bacterial populations has not been determined. We report the first application of 16S rRNA gene pyrosequencing and quantitative PCR in conjunction with propidium monoazide sample treatment to characterise the viable bacterial composition of ascites. Twenty five cirrhotic patients undergoing paracentesis provided ascites. Samples were treated with propidium monoazide to exclude non-viable bacterial DNA. Total bacterial load was quantified by 16S rRNA Q-PCR with species identity and relative abundance determined by 16S rRNA gene pyrosequencing. Correlation of molecular microbiology data with clinical measures and diagnostic microbiology was performed. Viable bacterial signal was obtained in 84% of ascites samples, both by Q-PCR and pyrosequencing. Approximately 190,000 ribosomal pyrosequences were obtained, representing 236 species, including both gut and non gut-associated species. Substantial variation in the species detected was observed between patients. Statistically significant relationships were identified between the bacterial community similarity and clinical measures, including ascitic polymorphonuclear leukocyte count and Child-Pugh class. Viable bacteria are present in the ascites of a majority of patients with cirrhosis including those with no clinical signs of infection. Microbiota composition significantly correlates with clinical measures. Entry of bacteria into ascites is unlikely to be limited to translocation from the gut, raising fundamental questions about the processes that underlie the development of spontaneous bacterial peritonitis.

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“…Molecular methods based on species-specific PCR or broad- range PCR for detecting the 16S rRNA gene followed by sequencing for species identification are being increasingly used for the etiological diagnosis of purulent infections, including SBP, septic arthritis, or CAPD-related peritonitis (4,7,8,12,18,19). These assays have been shown to improve the diagnostic efficiency of culture methods due to their higher sensitivities, especially with samples obtained from patients who have been exposed to antibiotics prior to specimen sampling.…”

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Performance of the LightCycler SeptiFast Test M ^grade in Detecting Microbial Pathogens in Purulent Fluids

et al. 2011

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The performance of the LightCycler SeptiFast (SF) assay was compared to that of culture methods in the detection of microorganisms in 43 purulent fluids from patients with pyogenic infections. The SF assay was more sensitive than the culture methods (86% versus 61%, respectively), irrespective of whether the infections were mono-or polymicrobial.The LightCycler SeptiFast (SF) test is a commercially available multiplex real-time PCR assay able to detect a wide range of bacterial and fungal organisms commonly involved in systemic infections (10). The SF assay has been shown to be a valuable ancillary method for the etiological diagnosis of bacteremia, sepsis, endocarditis, and more recently, periprosthetic joint infections, particularly in patients who have received antibiotics prior to diagnostic testing (1-3, 5, 6, 9, 10, 13-17). Molecular methods can allow the rapid detection of the microorganisms involved in severe pyogenic infections, thus leading to a more efficient and targeted early therapeutic intervention, which could translate into major clinical benefits for patients. To the best of our knowledge, there is no published experience on the performance characteristics of the SF assay for the detection of microorganisms in purulent fluids.A total of 43 purulent fluids obtained from 41 patients (29 male and 12 female; mean age, 64.1 years) over a period of 5 months (July to November 2010) were included in this study, as follows: 11 biliary fluid samples from patients with acute cholangitis, 7 pleural fluid samples from patients with empyema secondary to mesothelioma, lung cancer, or community-acquired and nosocomial pneumonia, 7 peritoneal fluid samples from patients with secondary peritonitis, 7 dialysis effluents from 6 patients with continuous ambulatory peritoneal dialysis (CAPD)-related peritonitis, 5 purulent liquid samples from 4 patients with intra-abdominal abscesses secondary to abdominal surgery, 4 purulent (Ͼ250 polymorphonuclear leukocytes/l) ascites fluid samples from cirrhotic patients with spontaneous bacterial peritonitis (SBP), and 2 intra-articular fluid samples from patients with acute septic arthritis. A total of 31 of the 41 patients had been treated with broad-spectrum antibiotics prior to sampling, as follows. All patients (n ϭ 11) undergoing biliary surgery, 3 patients subjected to thoracocentesis for empyema, and 3 patients undergoing laparotomy for secondary peritonitis received perioperative antimicrobial prophylaxis with amoxicillin-clavulanic. All patients with intra-abdominal abscesses and 4 patients with secondary peritonitis were empirically treated with ciprofloxacin plus metronidazole for a median of 2 days (range, 1 to 4 days) prior to specimen sampling. Four patients with secondary empyema had been treated with imipenem, imipenem plus metronidazole, or imipenem plus vancomycin for a median of 1 day prior to specimen sampling (range, 1 to 3 days). One patient with CAPD, one patient with SBP, and one patient with septic arthritis were treated with vancomycin or ceftriaxone ...

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Characterisation of bacteria in ascites—reporting the potential of culture-independent, molecular analysis

Cited by 31 publications

References 32 publications

Application of Qualitative and Quantitative Real-Time PCR, Direct Sequencing, and Terminal Restriction Fragment Length Polymorphism Analysis for Detection and Identification of Polymicrobial 16S rRNA Genes in Ascites

Application of Qualitative and Quantitative Real-Time PCR, Direct Sequencing, and Terminal Restriction Fragment Length Polymorphism Analysis for Detection and Identification of Polymicrobial 16S rRNA Genes in Ascites

Ascitic Microbiota Composition Is Correlated with Clinical Severity in Cirrhosis with Portal Hypertension

Performance of the LightCycler SeptiFast Test M ^grade in Detecting Microbial Pathogens in Purulent Fluids

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Characterisation of bacteria in ascites—reporting the potential of culture-independent, molecular analysis

Cited by 31 publications

References 32 publications

Application of Qualitative and Quantitative Real-Time PCR, Direct Sequencing, and Terminal Restriction Fragment Length Polymorphism Analysis for Detection and Identification of Polymicrobial 16S rRNA Genes in Ascites

Application of Qualitative and Quantitative Real-Time PCR, Direct Sequencing, and Terminal Restriction Fragment Length Polymorphism Analysis for Detection and Identification of Polymicrobial 16S rRNA Genes in Ascites

Ascitic Microbiota Composition Is Correlated with Clinical Severity in Cirrhosis with Portal Hypertension

Performance of the LightCycler SeptiFast Test M grade in Detecting Microbial Pathogens in Purulent Fluids

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Performance of the LightCycler SeptiFast Test M ^grade in Detecting Microbial Pathogens in Purulent Fluids