Development and application of a canine endogenous internal positive control for use in real-time PCR assays

Real-time PCR (rtPCR) tests have become a method of choice in many diagnostic settings, both animal and human. A concern remains, however, regarding rtPCR assay inhibition during nucleic acid extraction and/or rtPCR reaction process that may result in false-negative results. The use of an internal positive control, either endogenous or exogenous, to mitigate this issue has become more commonplace. We identified and standardized an endogenous internal positive control that can be utilized in rtPCR assays targeting canine-specific pathogens in either a singleplex or multiplex format. The target chosen for the endogenous internal positive control (EIPC-K9) was a highly conserved region in canine mitochondrial DNA. Samples from 240 dogs and 11 other species were screened with EIPC-K9; all canine samples were detected, and no cross-amplification with other species tested was observed. Additionally, no inhibition was noted when comparing singleplex to multiplex rtPCR formats.

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Modification of two capripoxvirus quantitative real-time PCR assays to improve diagnostic sensitivity and include beta-actin as an internal positive control

Journal of Veterinary Diagnostic Investigation ◽

10.1177/1040638717695609 ◽

2017 ◽

Vol 29 (3) ◽

pp. 351-356

Author(s):

Amaresh Das ◽

Ming Y. Deng ◽

Shawn Babiuk ◽

Michael T. McIntosh

Keyword(s):

Real Time ◽

False Negative ◽

Positive Control ◽

Lumpy Skin Disease ◽

Outbreak Management ◽

Negative Results ◽

Beta Actin ◽

False Negative Results ◽

Internal Positive Control ◽

Analytical Sensitivities

Capripoxviruses (CaPVs), consisting of Sheeppox virus (SPV), Goatpox virus (GPV), and Lumpy skin disease virus (LSDV) species, cause economically significant diseases in sheep, goats, and cattle, respectively. Quantitative real-time polymerase chain reaction (qPCR) assays are routinely used for rapid detection of CaPVs in surveillance and outbreak management programs. We further modified and optimized 2 previously published CaPV qPCR assays, referred to as the Balinsky and Bowden assays, by changing commercial PCR reagents used in the tests. The modified assays displayed 100% analytical specificity and showed no apparent changes in analytical sensitivities for detection of CaPVs compared with the original assays. Diagnostic sensitivities, assessed using 50 clinical reference samples from experimentally infected sheep, goats, and cattle, improved from 82% to 92% for the modified Balinsky assay and from 58% to 82% for the modified Bowden assay. The modified qPCR assays were multiplexed for detection of beta-actin as an indicator for potential false-negative results. The multiplex modified qPCR assays exhibited the same diagnostic sensitivities as the singleplex assays suggesting their utility in the detection of CaPVs.

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Detection of Streptococcus pneumoniae in Sputum Samples by Real- Time PCR.

Anti-Infective Agents ◽

10.2174/2211352518999200629165108 ◽

2020 ◽

Vol 18 ◽

Author(s):

Pegah Shakib ◽

Mohammad Reza Zolfaghari

Keyword(s):

Streptococcus Pneumoniae ◽

Real Time ◽

Real Time Pcr ◽

False Negative ◽

Cross Sectional Study ◽

Laboratory Culture ◽

Cross Sectional ◽

Negative Results ◽

False Negative Results ◽

Pcr Method

Background: Conventional laboratory culture-based methods for diagnosis of Streptococcus pneumoniae are time-consuming and yield false negative results. Molecular methods including real-time (RT)-PCR rapid methods and conventional PCR due to higher sensitivity and accuracy have been replaced instead traditional culture assay. The aim of the current study was to evaluate lytA gene for detection of Streptococcus pneumoniae in the cerebrospinal fluid of human patients with meningitis using real-time PCR assay. Material and Methods: In this cross-sectional study, a total of 30 clinical specimens were collected from patients in a period from September to December 2018. In order to evaluate the presence of lytA gene, conventional and real-time PCR methods were used without culture. Results: From 30 sputum samples five (16.66%) isolates were identified as S. pneumoniae by lytA PCR and sequencing. Discussion: In this research, an accurate and rapid real-time PCR method was used, which is based on lytA gene for diagnosis of bacteria so that it can be diagnosed. Based on the sequencing results, the sensitivity for detection of lytA gene was 100% (5/5).

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Differing Effects of Standard and Harsh Nucleic Acid Extraction Procedures on Diagnostic Helminth Real-Time PCRs Applied to Human Stool Samples

Pathogens ◽

10.3390/pathogens10020188 ◽

2021 ◽

Vol 10 (2) ◽

pp. 188

Author(s):

Tanja Hoffmann ◽

Andreas Hahn ◽

Jaco J. Verweij ◽

Gérard Leboulle ◽

Olfert Landt ◽

...

Keyword(s):

Nucleic Acid ◽

Real Time ◽

Real Time Pcr ◽

Acid Extraction ◽

Nucleic Acid Extraction ◽

Pcr Assay ◽

Bead Beating ◽

Stool Samples ◽

Pcr Assays ◽

Human Stool

This study aimed to assess standard and harsher nucleic acid extraction schemes for diagnostic helminth real-time PCR approaches from stool samples. A standard procedure for nucleic acid extraction from stool and a procedure including bead-beating as well as proteinase K digestion were compared with group-, genus-, and species-specific real-time PCR assays targeting helminths and nonhelminth pathogens in human stool samples. From 25 different in-house and commercial helminth real-time PCR assays applied to 77 stool samples comprising 67 historic samples and 10 external quality assessment scheme samples positively tested for helminths, higher numbers of positive test results were observed after bead-beating-based nucleic acid extraction for 5/25 (20%) real-time PCR assays irrespective of specificity issues. Lower cycle threshold values were observed for one real-time PCR assay after the standard extraction scheme, and for four assays after the bead-beating-based scheme. Agreement between real-time PCR results after both nucleic acid extraction strategies according to Cohen’s kappa ranged from poor to almost perfect for the different assays. Varying agreement was observed in eight nonhelminth real-time PCR assays applied to 67 historic stool samples. The study indicates highly variable effects of harsh nucleic acid extraction approaches depending on the real-time PCR assay used.

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False Negative Results in High Viremia Parvovirus B19-Samples Tested with Real-Time PCR

Polish Journal of Microbiology ◽

10.33073/pjm-2010-020 ◽

2010 ◽

Vol 59 (2) ◽

pp. 129-132 ◽

Cited By ~ 4

Author(s):

PIOTR GRABARCZYK ◽

ALEKSANDRA KALIŃSKA ◽

EWA SULKOWSKA ◽

EWA BROJER

Keyword(s):

Positive Result ◽

Real Time ◽

Real Time Pcr ◽

Parvovirus B19 ◽

False Negative ◽

Immunocompromised Patients ◽

Negative Results ◽

False Negative Results ◽

Parvovirus B 19 ◽

The Way

Extremely high viremia is observed during some viruses infection, especialy in immunocompromised patients. False negative results of Parvovirus B 19 DNA tests performed with real-time PCR in high viremic samples are reported. The way of fluorescence diagrams analysis and algorithm of positive result confirmation to exclude such phenomenon are proposed.

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False-Negative Results of a Validated Real-Time PCR Protocol for Diagnosis of Newcastle Disease Due to Genetic Variability of the Matrix Gene

Journal of Clinical Microbiology ◽

10.1128/jcm.00895-09 ◽

2009 ◽

Vol 47 (11) ◽

pp. 3791-3792 ◽

Cited By ~ 24

Author(s):

G. Cattoli ◽

C. De Battisti ◽

S. Marciano ◽

S. Ormelli ◽

I. Monne ◽

...

Keyword(s):

Genetic Variability ◽

Real Time ◽

Newcastle Disease ◽

Real Time Pcr ◽

False Negative ◽

Negative Results ◽

Matrix Gene ◽

False Negative Results ◽

The Matrix

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Assessment of Commercial DNA Cleanup Kits for Elimination of Real-Time PCR Inhibitors in the Detection of Cyclospora cayetanensis in Cilantro

Journal of Food Protection ◽

10.4315/jfp-20-139 ◽

2020 ◽

Vol 83 (11) ◽

pp. 1863-1870

Author(s):

ANGELA ASSURIAN ◽

HELEN MURPHY ◽

ALICIA SHIPLEY ◽

HEDIYE NESE CINAR ◽

ALEXANDRE DA SILVA ◽

...

Keyword(s):

Real Time ◽

Real Time Pcr ◽

False Negative ◽

Threshold Values ◽

Cyclospora Cayetanensis ◽

Cycle Threshold ◽

Negative Results ◽

False Negative Results ◽

Pcr Inhibitor ◽

Zymo Research

ABSTRACT Inhibited reactions have occasionally been observed when cilantro samples were processed for the detection of Cyclospora cayetanensis using quantitative real-time PCR (qPCR). Partial or total inhibition of PCR reactions, including qPCR, can occur, leading to decreased sensitivity or false-negative results. If inhibition occurs, this implies the need for additional purification or cleanup treatments of the extracted DNA to remove inhibitors prior to molecular detection. Our objective was to evaluate the performance of five commercial DNA cleanup kits (QIAquick purification kit from Qiagen [kit 1], OneStep PCR inhibitor removal by Zymo Research [kit 2], NucleoSpin genomic DNA cleanup XS from Macherey-Nagel [kit 3], DNA IQ system by Promega [kit 4], and DNeasy PowerPlant pro kit from Qiagen [5]) to minimize qPCR inhibition using the U.S. Food and Drug Administration–validated Bacteriological Analytical Manual (BAM) Chapter 19b method for detection of C. cayetanensis in cilantro samples containing soil. Each of the five commercial DNA cleanup kits evaluated was able to reduce the qPCR internal amplification control cycle threshold values to those considered to be normal for noninhibited samples, allowing unambiguous interpretation of results in cilantro samples seeded at both a high oocyst level (200 oocysts) and a low oocyst level (10 oocysts). Of the five kits compared, kits 1, 2, and 3 did not show significant differences in the detection of C. cayetanensis, while significantly higher cycle threshold values, indicating lower recovery of the target DNA, were observed from kits 4 and/or 5 in samples seeded with 200 and 10 oocysts (P < 0.05). This comparative study provides recommendations on the use of commercial cleanup kits which could be implemented when inhibition is observed in the detection of C. cayetanensis in cilantro samples using the BAM Chapter 19b method. HIGHLIGHTS

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Comparison of BKV quantification using a single automated nucleic acid extraction platform and 3 real-time PCR assays

Diagnostic Microbiology and Infectious Disease ◽

10.1016/j.diagmicrobio.2015.04.006 ◽

2015 ◽

Vol 82 (4) ◽

pp. 297-302 ◽

Cited By ~ 5

Author(s):

A.E. Greer ◽

M.S. Forman ◽

A. Valsamakis

Keyword(s):

Nucleic Acid ◽

Real Time ◽

Real Time Pcr ◽

Acid Extraction ◽

Nucleic Acid Extraction ◽

Pcr Assays

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A Multiplex Real-Time Polymerase Chain Reaction (TaqMan) Assay for the Simultaneous Detection of Meloidogyne chitwoodi and M. fallax

Phytopathology ◽

10.1094/phyto-96-1255 ◽

2006 ◽

Vol 96 (11) ◽

pp. 1255-1262 ◽

Cited By ~ 32

Author(s):

C. Zijlstra ◽

R. A. Van Hoof

Keyword(s):

Polymerase Chain Reaction ◽

Real Time ◽

Real Time Pcr ◽

False Negative ◽

Simultaneous Detection ◽

Chain Reaction ◽

Meloidogyne Chitwoodi ◽

Negative Results ◽

False Negative Results ◽

Polymerase Chain

This study describes a multiplex real-time polymerase chain reaction (PCR) approach for the simultaneous detection of Meloidogyne chitwoodi and M. fallax in a single assay. The approach uses three fluorogenic minor groove binding (MGB) TaqMan probes: one FAM-labeled to detect M. chitwoodi, one VIC-labeled to detect M. fallax, and one NED-labeled to detect the internal amplification control (IAC) to monitor false negative results. One common primer set is used for the amplification of part of the internal transcribed spacer (ITS) region of M. chitwoodi and M. fallax and one primer set for the amplification of the IAC. The test enabled detection of M. chitwoodi and/or M. fallax in DNA samples extracted from batches of juveniles, from single juveniles, and from infected plant material. Compared with current assays to detect M. chitwoodi and M. fallax, the multiplex real-time PCR offers the following advantages: it is faster because the test can simultaneously detect both quarantine species without the need for post-PCR processing; and it is at least 10 times more sensitive than a comparable regular PCR also targeting the ITS sequence. Inclusion of the IAC facilitates the interpretation of the FAM and VIC cycle threshold (Ct) values and can prevent the scoring of false negative results when FAM, VIC, and NED Ct values are high. The test allows precise quantification when only one of the two species is present in the sample. However, experiments with mixtures of genomic DNA of M. chitwoodi and M. fallax revealed that the ability of the multiplex real-time PCR assay to detect small quantities of DNA of one species is reduced when large quantities of DNA of the other species are present.

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False-negative results in Real-Time PCR (RT-PCR) for meningococcal disease diagnosis

REVISTA DO INSTITUTO ADOLFO LUTZ ◽

10.18241/0073-98552013721544 ◽

2013 ◽

Author(s):

Lucila Okuyama FUKASAWA ◽

Maria Gisele GONÇALVES ◽

Fabio Takenori HIGA ◽

Maristela Marques SALGADO ◽

Ana Paula Silva de LEMOS ◽

...

Keyword(s):

Real Time ◽

Meningococcal Disease ◽

Real Time Pcr ◽

False Negative ◽

Disease Diagnosis ◽

Rt Pcr ◽

Negative Results ◽

False Negative Results

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Evaluating real-time PCR for the quantification of distinct pathogens and indicator organisms in environmental samples

Water Science & Technology ◽

10.2166/wst.2004.0065 ◽

2004 ◽

Vol 50 (1) ◽

pp. 263-270 ◽

Cited By ~ 32

Author(s):

M. Lebuhn ◽

M. Effenberger ◽

G. Garcés ◽

A. Gronauer ◽

P.A. Wilderer

Keyword(s):

Nucleic Acid ◽

Real Time ◽

Real Time Pcr ◽

Environmental Samples ◽

False Negative ◽

Indicator Organisms ◽

Negative Results ◽

False Negative Results ◽

Methodological Bias ◽

Reliable Quantification

We evaluated quantitative real-time PCR (qPCR) and RTqPCR (for RNA species) for their ability to quantify microorganisms and viruses in problematic environmental samples such as cattle manure, digester material, wastewater and soil. Important developments included a standard spiking approach which compensated for methodological bias and allowed sample-to-sample comparison and reliable quantification. Programme CeTe was developed to calculate endogenous concentrations of target organisms (nucleic acid copies) for each sample separately from the generated standard curves. The approach also permitted assessment of the detection limit of the complete method, including extraction. It varied from sample to sample, due to different extraction efficiencies and variable co-extraction of PCR inhibitors. False negative results were thereby avoided. By using this approach we were able to optimise a DNA extraction protocol from the different tested sample types. Protocols for the extraction of RNA species from environmental samples were also optimised. DNA was (almost) not degraded after lethal shock (autoclaving) in the sterile environment. In contrast, the parallel selective cultivation and qPCR results for various microbial parameters from an anaerobic digester chain suggested that DNA from decaying organisms was readily recycled in metabolically active environments. It may, therefore, be used to determine viable organisms in samples exhibiting substantial metabolic turnover. It is proposed that our standard spiking approach, including data evaluation by the program CeTe, should be considered in future standardisation and norms for the quantification of nucleic acid containing organisms in environmental and product samples.

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