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Confirmatory assays for detection of Neisseria gonorrhoeae using porA pseudogene Real???Time PCR based methods
Joint Event on 8th Annual Congress on CLINICAL MICROBIOLOGY & INFECTIOUS DISEASES & 13th World Congress on VIROLOGY, INFECTIONS AND OUTBREAKS
December 05-06, 2018 | Vancouver, Canada
Imarenezor EPK
Federal University Wukari, Nigeria
Posters & Accepted Abstracts: Clin Microbiol
Abstract:
Background: Since the advent of molecular techniques, diagnosis of Neisseria gonorrhoeae has been ruin by false positive results
when compared with culture, which is currently the gold standard. False positive results are often due to the cross???reaction of nucleic
acid amplification test (NAAT) with closely related non-pathogenic Neisseria species. Regardless of the availability of commercial
NAATs for N. gonorrhoeae, issues surrounding the specificity of these platforms persist.
Objectives: This research aims to institute, heighten and compare the sensitivity and specificity of previously available N. gonorrhoeae
real???time assays which target the porA pseudogene.
Methods: In the course of the investigation, 156 gonococci specimens and 30 non-gonococci culture specimens were used. Optimization
of the PorA pseudogene real???time PCR was carried out by varying the concentration of magnesium chloride as follows: 5mM ranges
between 19.08 (4.31) and 23.27 (17.57), 4mM ranges from 17.18 (1.15) and 22.01 (16.43) and for 3mM the range is from 21.71
(2.20) and 27.33 (15.27) with the standard deviation in bracket and as well as the forward and reverse primers which have varying
concentration as 50mM, 300mM and 900mM for both.
Results: The results obtained show the high specificity of the assays for all 156 gonococci culture specimens gave positive results, whilst
the 30 non-gonococci specimens gave negative results. This shows that PorA pseudogene real-time PCR is a suitable assay for the
confirmation of putative N. gonorrhoeae cultures and can assist in identification, particularly in cases where traditional biochemical
and immunology tests have failed. The potential of the PorA pseudogene real???time PCR to detect the presence of N. gonorrhoeae
specific DNA directly from clinical samples was then evaluated. An initial experiment was performed which involved the addition
of a primer and probe set which acted as an internal control, it was determined that the internal control did not compromise the
sensitivity of the PorA pseudogene real???time PCR assay and could be used reliably to screen for assay inhibition. The PorA pseudogene
real???time PCR was then used to examine some clinical specimens which had been examined previously at three laboratories, each of
which different commercial N. gonorrhoeae NAAT platforms were used. The results from this investigation show a high specificity
evidence of PorA pseudogene real-time PCR when compared to previous results obtained from the other laboratories.
Conclusion: The study has succeeded in establishing to very large extent that the PorA pseudogene real???time PCR is a very valuable
assay for the detection and confirmation of N. gonorrhoeae specific DNA from both putative cultures and directly from clinical
samples.
Biography :
E-mail: kimarenezor@yahoo.com