More Pathogenicity or Just More Pathogens?—On the Interpretation Problem of Multiple Pathogen Detections with Diagnostic Multiplex Assays

Zautner, Andreas E.; Groß, Uwe; Emele, Matthias F.; Hagen, Ralf Matthias; Frickmann, Hagen

doi:10.3389/fmicb.2017.01210

Cited by 36 publications

(34 citation statements)

References 67 publications

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“…A second, and more powerful strategy is to focus on levels of the genetic sequence observed. If mef(A) is helping a pathogen cause disease, it will be enriched to a higher copy number than it would be as a sporadic colonizer diluted into a healthy microbial community [65,66]. By providing quantitative data on relative levels of mef(A), our RPA assay is ideally suited to this approach, making the determination of an infection a matter of comparing the detected gene level with a threshold (after normalizing to total bacterial load).…”

Section: Discussionmentioning

confidence: 99%

“…By providing quantitative data on relative levels of mef(A), our RPA assay is ideally suited to this approach, making the determination of an infection a matter of comparing the detected gene level with a threshold (after normalizing to total bacterial load). Critically, future work must focus on empirically setting the threshold by testing many clinical samples, from both healthy and sick patients [65]. By providing a validated, easy-to-use rapid molecular assay, the present study represents a vital first step in this process.…”

Section: Discussionmentioning

confidence: 99%

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Rapid molecular detection of macrolide resistance

2019

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BackgroundEmerging antimicrobial resistance is a significant threat to human health. However, methods for rapidly diagnosing antimicrobial resistance generally require multi-day culture-based assays. Macrolide efflux gene A, mef(A), provides resistance against erythromycin and azithromycin and is known to be laterally transferred among a wide range of bacterial species.MethodsWe use Recombinase Polymerase Assay (RPA) to detect the antimicrobial resistance gene mef(A) from raw lysates without nucleic acid purification. To validate these results we performed broth dilution assays to assess antimicrobial resistance to erythromycin and ampicillin (a negative control).ResultsWe validate the detection of mef(A) in raw lysates of Streptococcus pyogenes, S. pneumoniae, S. salivarius, and Enterococcus faecium bacterial lysates within 7–10 min of assay time. We show that detection of mef(A) accurately predicts real antimicrobial resistance assessed by traditional culture methods, and that the assay is robust to high levels of spiked-in non-specific nucleic acid contaminant. The assay was unaffected by single-nucleotide polymorphisms within divergent mef(A) gene sequences, strengthening its utility as a robust diagnostic tool.ConclusionsThis finding opens the door to implementation of rapid genomic diagnostics in a clinical setting, while providing researchers a rapid, cost-effective tool to track antibiotic resistance in both pathogens and commensal strains.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Rapid molecular detection of macrolide resistance

2019

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“…First, with increasingly sensitive diagnostic testing platforms, it can be difficult to distinguish viral carriage from true infection. 172 Rates of asymptomatic viral carriage range from 2 to 17%, depending on the patient population studied. 8,23,86,173 The specificity of PCR-based testing likely varies significantly, depending on both the age of the patient and the pathogen identified.…”

Section: Areas Of Uncertaintymentioning

confidence: 99%

Other Respiratory Viruses as a Cause of Community-Acquired Pneumonia

Walter

2020

Semin Respir Crit Care Med

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AbstractCommunity-acquired pneumonia (CAP) is a major cause of morbidity and mortality worldwide. There is growing appreciation of the burden of noninfluenza viral pathogens in CAP. Due to multiple factors including pneumococcal vaccination programs, declining rates of cigarette smoking, an aging population, and increasingly sensitive diagnostic tests, respiratory viruses are now the most common pathogens detected in CAP, outpacing Streptococcus pneumoniae. Noninfluenza respiratory pathogens are widely accepted as causal pathogens in CAP including in immunocompetent patients. This review provides an overview of five noninfluenza respiratory viral pathogens commonly implicated in CAP pathogenesis: rhinovirus, human metapneumovirus, respiratory syncytial virus, human parainfluenza virus, and human adenoviruses. Nucleic acid amplification testing platforms and their impact on antimicrobial stewardship efforts are also considered.

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“…Further, the discrimination between an asymptomatic colonization and a clinically relevant infection relies upon the development of standardized quantitative cut off cyclethreshold (C t ) † values. 45 However, it is not clear that a relationship actually exists between the number of microorganisms present in an individual's specimen and the presence of healthy carriage or disease within the individual. One means of overcoming the problematic amplication of non-target DNA is to utilize multiplex-touchdown PCR (MT-PCR), which combines the features of a multiplex PCR (incorporating primers for a number of DNA targets) with touchdown PCR (which involves a cycling program, in which the annealing temperature is gradually reduced from a value above the estimated melting temperature (T m ) of the primers ‡ until it reaches the calculated annealing temperature [the touchdown temperature]), to increase the PCR specicity, sensitivity and yield.…”

Section: Nucleic Acidsmentioning

confidence: 99%