Development of conventional and real-time multiplex PCR assays for the detection of nosocomial pathogens

Anbazhagan, Deepa; Wang, Seok Mui; Mansor, Marzida; Yan, Gracie Ong Siok; Yusof, Mohd Yasim Mohd; Sekaran, Shamala Devi

doi:10.1590/s1517-83822011000200006

Cited by 38 publications

(29 citation statements)

References 32 publications

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“…In a bid to combat the laborious time that we spend on the post amplification using gel electrophoresis, to increase both sensitivity and specificity while paying more attention to the reliability of the test result, real time Polymerase Change Reaction (real time-PCR) was required [8,13,15]. Real time PCR is a very powerful and rapid nucleic acid amplifying devices that is also simple to use.…”

Section: Quantitative Real-time Pcr (Qpcr)mentioning

confidence: 99%

“…This simply means that both the amplification and analysis occur together. [13,14,15] In contrast to the conventional PCR, either Deoxyribonucleic acid (DNA) dyes or the fluorescent probes are among the reagents mixture added before running the machine. Since there is no need to transfer samples from a thermocycler to gel electrophoresis reading, (Samples are automatically analyzed and the results are shown on the computer screen).…”

Section: Quantitative Real-time Pcr (Qpcr)mentioning

confidence: 99%

“…Sensitivity is the ability to detect the smallest of amount of DNA, cDNA or RNA for a reaction and serial dilution (e.g. 2 X 102 to 2 X 1010) is used to determine the sensitivity of PCR assay [13]. qPCR has achieved a milestone in the field of water monitoring.…”

Section: Quantitative Real-time Pcr (Qpcr)mentioning

confidence: 99%

“…Among these NATs, PCR still stood distinct. On top of its ability in rapidly detecting pathogenic DNA, PCR tests are also highly sensitive and specific [8,11,12,13].…”

Section: Introductionmentioning

confidence: 99%

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Untitled

2017

RJLBPCS

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Isolation, detection and quantification of pathogenic DNA is the novel approach when it comes to the diagnosis of infectious disease. In every laboratory more especially in the waterborne pathogenic research laboratories, achieving an accurate result is always the main goal.Efficient and reliable results are not achieved using only the old conventional methods due to number of reasons. To this end, molecular methods that include real-time polymerase chain reactions (real-time PCRs) for the detection of nucleic acid stand novel. In this review, the efficiency, sensitivity and reliability of singleplex and multiplex real-time PCR are thoroughly considered. Further analysis on their contrasting validities was also briefed on. Articles were randomly selected with some specificity to the previous water microbiology studies. From the review, it is clear that both the use of singleplex and multiplex real-time PCR are always valid for the waterborne pathogen detection. However, majority of the researchers would prefer to choose multiplex over singleplex. Both has shown a considerable validity but running for multiple target in single reaction tube assured both the economic cost and saves time.

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Section: Quantitative Real-time Pcr (Qpcr)mentioning

confidence: 99%

Section: Quantitative Real-time Pcr (Qpcr)mentioning

confidence: 99%

Section: Quantitative Real-time Pcr (Qpcr)mentioning

confidence: 99%

“…Among these NATs, PCR still stood distinct. On top of its ability in rapidly detecting pathogenic DNA, PCR tests are also highly sensitive and specific [8,11,12,13].…”

Section: Introductionmentioning

confidence: 99%

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Untitled

2017

RJLBPCS

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“…The qPCR amplification reactions followed the protocol described by Anbazhagan et al [14] with some modifications. In a final total of 25 µL reaction, 3 pmol of each primer, 10 ng genomic DNA from clinical specimens, 12.5 µL SYBR Green PCR Master Mix (Invitrogen Life Technologies, Carlsbad, USA), and deionized water were included.…”

Section: Multiplex Qpcrmentioning

confidence: 99%

Etiological profile of early neonatal bacterial sepsis by multiplex qPCR

Silva-Junior

Martins

Xavier

et al. 2016

J Infect Dev Ctries

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Introduction: Given the major impact in terms of morbidity and mortality that episodes of early neonatal sepsis (ENS) have on both newborns and health systems, this study aimed to identify the etiological profile of early neonatal bacterial sepsis by a multiplex quantitative real-time polymerase chain reaction (qPCR). Methodology: Blood samples from newborns diagnosed with clinical ENS and hospitalized in neonatal intensive care units (NICUs) were collected and analyzed using the multiplex qPCR method to detect Streptococcus agalactiae, Escherichia coli, Klebsiella pneumoniae, Pseudomonas aeruginosa, Enterobacter sp., Serratia sp., and Staphylococcus aureus. A universal primer was used in the analysis. Results: A total of 150 neonates with clinical sepsis and 10 newborns as healthy controls were included in the study. The group with clinical sepsis was 100% positive for the presence of bacterial genomic DNA through the universal primer. The control group showed negativity by qPCR. The multiplex qPCR analysis showed that 76% of the samples were positive for Escherichia coli, 34% for Staphylococcus aureus, 13.3% for Streptococcus agalactiae, 7.3% for Pseudomonas aeruginosa, and 0.7% for Enterobacter sp. and Serratia sp. Multiplex qPCR of patients with clinical sepsis matched with 8.1% of the blood samples that tested positive by the microbiological method. Conclusions: Rapid and sensitive detection of the pathogens causing ENS by this new multi-target approach based on multiplex qPCR could potentially excel compared to microbiological methods, with the simple objective of facilitating the progression to a more rapid and specific antimicrobial therapy, avoiding the abuse of antibiotics in NICUs.

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