Abstract
Factors responsible for false-negative results (F-N) in RT-PCR assay for detecting N. meningitidis in serum and CSF samples were investigated. As the meningococcal disease should be rapidly treated because of its high mortality and epidemic potential, the F-N in diagnostic testing may cause treatment failures and/or on disease restraint in community. Thus, it is crucial to learn the factors which cause F-N in RT-PCR assays. The F-N were induced by inhibition, low quantity of target DNA in extracted samples, and inadequate temperature employed at PCR annealing procedure. As bacterial DNA concentration in samples might be highly variable, the ideal sample volume to be extracted could not be defined. As previously recommended for N. meningitidis gene-grouping by RT-PCR assay, the annealing temperature at 60 °C was not suitable for B and W135 genogroups. Altogether, these factors induced F-N in 31 samples; therefore, 30 % of N. meningitidis detected by RT-PCR were classified as non-genogrouped. The inhibitors and/or the low amount of target DNA induced F-N on RT-PCR, independently of the specimen volume used for extracting DNA. However, adjustments on the PCR annealing temperature and amount of extracted DNA added into the reaction might avoid the occurrence of the majority of F-N.
Highlights
Bacterial meningitis is a serious disease that requires laboratory confirmation for optimal management
Since the introduction of multiplex real-time PCR (RT-PCR) for diagnosis of bacterial meningitis in Greater São Paulo, two unexpected situations have arisen: (i) we have identified 6 serum samples with false negative RTPCR results for N. meningitidis, and (ii) 25 cerebrospinal fluid (CSF) samples with false negative serogroup-specific RT-PCR results for serogroups B (n=15) and W135 (n=10)
To overcome the lack of culture results, laboratories have used other methods to detect the presence of N. meningitidis, H. influenzae and S. pneumoniae in clinical samples
Summary
Bacterial meningitis is a serious disease that requires laboratory confirmation for optimal management. In April 2007, we begun using multiplex RTPCR for the diagnosis of bacterial meningitis caused by N. meningitidis[4], S. pneumoniae[5], and H. influenzae[3] on cerebrospinal fluid (CSF) and serum samples in Greater São Paulo, Brazil[6]. Since the introduction of multiplex RT-PCR for diagnosis of bacterial meningitis in Greater São Paulo, two unexpected situations have arisen: (i) we have identified 6 serum samples with false negative RTPCR results for N. meningitidis, and (ii) 25 CSF samples with false negative serogroup-specific RT-PCR results for serogroups B (n=15) and W135 (n=10). As RT-PCR is more sensitive and specific than most non-culture diagnostic methods including CIE, the possibility of false negative RT-PCR results is of great interest. The objective of this study was to investigate the reasons for these 31 false negative RT-PCR results
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