Towards accurate exclusion of neonatal bacterial meningitis: a feasibility study of a novel 16S rDNA PCR assay

Abelian, Arthur; Mund, Thomas; Curran, Martin D.; Savill, Stuart; Mitra, Nipa; Charan, Carol; Ogilvy-Stuart, Amanda; Dear, Paul H.

doi:10.1186/s12879-020-05160-x

Cited by 6 publications

(4 citation statements)

References 46 publications

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“…Conventional 16S rRNA gene PCR/Sanger sequencing assays have the same advantage as MYcrobiota of being a broad range strategy that removes the need for an a priori knowledge of the potential bacterial pathogen before a test is performed. However, in contrast to MYcrobiota, these methods rely on relatively high concentrations of bacteria in samples and are therefore unlikely to have adequate sensitivity for exclusion of meningitis [ 14 , 15 ]. Another alternative for diagnosing meningitis is the use of commercial meningitis multiplex PCR panels, which also have the advantage of having short processing times [ 5 ].…”

Section: Discussionmentioning

confidence: 99%

Improved Diagnostics in Bacterial Neonatal Meningitis Using a Next-Generation Sequencing Platform

van der Hoeven,

van der Beek,

Bekker

et al. 2023

Infect Dis Ther

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Introduction Bacterial meningitis in infants is an infrequent but life-threatening condition. Empiric therapy should begin as soon as meningitis is thought likely. Consequently, the causative microorganisms may not always be detected using culturing techniques, as cerebrospinal fluid (CSF) cultures are influenced by antibiotics. Nucleic acid amplification tests, such as polymerase chain reaction (PCR) (multiplex panels), may overcome this limitation but require a priori knowledge of the likely pathogen present within the sample. With this in mind, we investigated to what extent a culture-free, broad-range 16S rRNA gene next-generation sequencing (NGS) platform (MYcrobiota) could add to the microbiological diagnosis of meningitis. Methods Retrospective cohort study at level III neonatal intensive care unit. Included were all infants with suspected meningitis admitted between 10 November 2017 and 31 December 2020. A comparison was made of the bacterial pathogen detection rate between MYcrobiota and conventional bacterial culture. Results In a 3-year period, 37 CSF samples (diagnostic and follow-up) from 35 infants with proven or possible meningitis were available for MYcrobiota testing. MYcrobiota detected the presence of bacterial pathogens in 11 samples (30%), in contrast with the conventional CSF culture, which detected bacteria in 2 of 36 samples (5.6%). Conclusion Addition of 16S rRNA sequencing to conventional culturing greatly improved the identification of the aetiology of bacterial meningitis compared to culturing of CSF samples alone.

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Section: Discussionmentioning

confidence: 99%

Improved Diagnostics in Bacterial Neonatal Meningitis Using a Next-Generation Sequencing Platform

van der Hoeven,

van der Beek,

Bekker

et al. 2023

Infect Dis Ther

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“…Thus, establishing a definite diagnosis of a CNS infection by clinical chemical or cytological routine parameters is still not possible at present. Diagnosis of infections relies on the identification of the causative pathogen by culture or molecular methods (e.g., 16 s rRNA amplification [ 114 ]; multiplex polymerase chain reaction [ 115 ]; metagenomic next-generation sequencing: [ 116 ]). Recent advances in molecular methods will open new avenues for the definite diagnosis of a variety of CNS infections, particularly in the presence of atypical or mild alterations of the composition of the CSF.…”

Section: Discussionmentioning

confidence: 99%

Spatial and temporal variation of routine parameters: pitfalls in the cerebrospinal fluid analysis in central nervous system infections

Djukic

Lange

Erbguth

et al. 2022

J Neuroinflammation

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The cerebrospinal fluid (CSF) space is convoluted. CSF flow oscillates with a net flow from the ventricles towards the cerebral and spinal subarachnoid space. This flow is influenced by heartbeats, breath, head or body movements as well as the activity of the ciliated epithelium of the plexus and ventricular ependyma. The shape of the CSF space and the CSF flow preclude rapid equilibration of cells, proteins and smaller compounds between the different parts of the compartment. In this review including reinterpretation of previously published data we illustrate, how anatomical and (patho)physiological conditions can influence routine CSF analysis. Equilibration of the components of the CSF depends on the size of the molecule or particle, e.g., lactate is distributed in the CSF more homogeneously than proteins or cells. The concentrations of blood-derived compounds usually increase from the ventricles to the lumbar CSF space, whereas the concentrations of brain-derived compounds usually decrease. Under special conditions, in particular when distribution is impaired, the rostro-caudal gradient of blood-derived compounds can be reversed. In the last century, several researchers attempted to define typical CSF findings for the diagnosis of several inflammatory diseases based on routine parameters. Because of the high spatial and temporal variations, findings considered typical of certain CNS diseases often are absent in parts of or even in the entire CSF compartment. In CNS infections, identification of the pathogen by culture, antigen detection or molecular methods is essential for diagnosis.

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“…One of these studies has particularly shown that targeted PCR is a useful adjunct to diagnostic and treatment modalities, providing important supplemental information compared to what is provided solely by standard bacterial culture results [ 18 ]. Attempts to determine the use of this molecular tool in the diagnosis of meningitis has also been made, although the clinical relevance remains ambiguous due to very small sample sizes in these studies [ 19 , 29 ]. In the same way, other researchers have looked into its clinical importance in blood and urine samples in the diagnosis of neonatal sepsis [ 20 , 21 , 22 , 23 , 24 , 25 , 26 , 27 , 28 ].…”

Section: Discussionmentioning

confidence: 99%

“…To date, there is a paucity of data on the clinical utility of 16S rRNA sequencing in pediatric infections [ 2 , 6 ]. Few studies highlight the diagnostic utility of 16S rRNA sequencing in select pediatric infections [ 16 , 17 , 18 , 19 , 20 ]. Most of these studies have attempted to isolate its clinical usefulness in the diagnosis of neonatal sepsis [ 21 , 22 , 23 , 24 , 25 ].…”

Section: Introductionmentioning

confidence: 99%

Determining the Clinical Utility of 16S rRNA Sequencing in the Management of Culture-Negative Pediatric Infections

et al. 2022

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The use of 16S rRNA sequencing in culture-negative infections has improved identification of bacterial pathogens in select scenarios, but its clinical impact requires further elucidation, especially in the pediatric population. This retrospective study aims to determine the clinical utility of 16S rRNA sequencing on the clinical management of pediatric culture-negative infections in our institution. Significant clinical utility was identified in 30 (40.5%) of 74 clinical samples (p < 0.0001). Of all specimens, pulmonary samples yielded the most clinical utility (n = 9, 30%), followed equally by joint fluid (n = 6, 20%) and bone (n = 6, 20%), with no difference between fluid and fresh tissue specimens (p = 0.346). Although the difference was not statistically significant (p = 0.4111), the overall use of broad-spectrum coverage was decreased. The median number of antibiotics was decreased from two to one (p < 0.0001) based on 16S rRNA sequencing results. The results suggest that 16S rRNA sequencing has a significant impact on decreasing the number of antibiotics used in the treatment of pediatric culture-negative infections. 16S rRNA sequencing performed on pulmonary specimens has the highest likelihood of identifying a pathogen compared to other specimen types. Additional cost–benefit analysis needs to be completed to further determine clinical benefit.

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Towards accurate exclusion of neonatal bacterial meningitis: a feasibility study of a novel 16S rDNA PCR assay

Cited by 6 publications

References 46 publications

Improved Diagnostics in Bacterial Neonatal Meningitis Using a Next-Generation Sequencing Platform

Improved Diagnostics in Bacterial Neonatal Meningitis Using a Next-Generation Sequencing Platform

Spatial and temporal variation of routine parameters: pitfalls in the cerebrospinal fluid analysis in central nervous system infections

Determining the Clinical Utility of 16S rRNA Sequencing in the Management of Culture-Negative Pediatric Infections

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