Comparison of Pooling 11 or 5 Oropharyngeal Swabbings for Detecting Avian Influenza Virus by Real-Time Reverse Transcription–PCR in Broiler Chickens

Ladman, B. S.; Spackman, Erica; Gelb, Jack

doi:10.1637/9839-062011-resnote.1

Cited by 14 publications

(16 citation statements)

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“…On the potential effect of swab pooling, our findings for combined virus subtypes indicate that pooling up to 10 negative swabs with one positive swab reduced the viral antigen concentration and consequently the proportion of FluDETECT positive samples. This result is largely consistent with those of Ladman et al [11]. However, a study by Spackman et al [39] did not find differences in virus detection between a single swab from an inoculated bird, 5 swabs (1 from an inoculated bird, 4 from unexposed birds), or 11 swabs (1 from an inoculated bird and 10 from unexposed birds) by real time RT-PCR.…”

Section: Discussionsupporting

confidence: 91%

“…Its ability to detect the virus in pools of 11 was compared with that in individual pools of 5 or 6 and in combined pools of 5 or 6 for separate H5 and H7 subtypes as well as for merged H5 and H7 sample groups. Only samples with CT ≤ 35 were considered RT-PCR positive [11, 19] and in the comparison of virus positive proportions, Fisher’s exact test at significance level of p ≤ 0.05 was used [20]. …”

Section: Methodsmentioning

confidence: 99%

“…In other words, not only does swab-pooling increase testing throughput, it also reduces the number of tests needed to meet sample size requirements and consequently the testing costs. However, due to dilution, pooling may also significantly reduce test sensitivity and lead to missing low prevalence infections [10, 11]. …”

Section: Introductionmentioning

confidence: 99%

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Quantifying the effect of swab pool size on the detection of influenza A viruses in broiler chickens and its implications for surveillance

et al. 2018

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BackgroundTimely diagnosis of influenza A virus infections is critical for outbreak control. Due to their rapidity and other logistical advantages, lateral flow immunoassays can support influenza A virus surveillance programs and here, their field performance was proactively assessed.The performance of real-time polymerase chain reaction and two lateral flow immunoassay kits (FluDETECT and VetScan) in detecting low pathogenicity influenza A virus in oropharyngeal swab samples from experimentally inoculated broiler chickens was evaluated and at a flock-level, different testing scenarios were analyzed.ResultsFor real-time polymerase chain reaction positive individual-swabs, FluDETECT respectively detected 37% and 58% for the H5 and H7 LPAIV compared to 28% and 42% for VetScan. The mean virus titer in H7 samples was higher than for H5 samples. For real-time polymerase chain reaction positive pooled swabs (containing one positive), detections by FluDETECT were significantly higher in the combined 5- and 6-swab samples compared to 11-swab samples. FluDETECT detected 58%, 55.1% and 44.9% for the H7 subtype and 28.3%, 34.0% and 24.6% for the H5 in pools of 5, 6 and 11 respectively.In our testing scenario analysis, at low flock-level LPAIV infection prevalence, testing pools of 11 detected slightly more infections while at higher prevalence, testing pools of 5 or 6 performed better. For highly pathogenic avian influenza virus, testing pools of 11 (versus 5 or 6) detected up to 5% more infections under the assumption of similar sensitivity across pools and detected less by 3% when its sensitivity was assumed to be lower.ConclusionsMuch as pooling a bigger number of swab samples increases the chances of having a positive swab included in the sample to be tested, this study’s outcomes indicate that this practice may actually reduce the chances of detecting the virus since it may result into lowering the virus titer of the pooled sample. Further analysis on whether having more than one positive swab in a pooled sample would result in increased sensitivity for low pathogenicity avian influenza virus is needed.

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Section: Discussionsupporting

confidence: 91%

Section: Methodsmentioning

confidence: 99%

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Quantifying the effect of swab pool size on the detection of influenza A viruses in broiler chickens and its implications for surveillance

et al. 2018

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“…An upper limit of 11 swabs has been suggested based on the statistical calculation where 11 swabs from a flock (of 10,000 or more) should be sufficient to detect 25% infection rate with 95% confidence, which is the level of surveillance outlined by the NPIP. A previous study comparing 5 and 11 swabs for detection of LPAIV from broilers by rRT-PCR has been reported and found no difference [2]. Another study comparing a single swab with pools of 5 with samples from turkeys also found no difference [1] This study agrees with those results and adds a comparison with single swabs, five and 11 swab pools in one experiment and very importantly, data for VI.…”

Section: Discussionsupporting

confidence: 84%

“…Evaluations of swab pooling for AIV using only real-time (rRT-PCR), but not virus isolation have been reported [1,2]. Similarly, detection of AIV with wet versus dry swabs from Pekin ducks tested by rRT-PCR only has been compared [3].…”

Section: Introductionmentioning

confidence: 99%

Optimal specimen collection and transport methods for the detection of avian influenza virus and Newcastle disease virus

et al. 2013

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BackgroundActive and passive surveillance for avian influenza virus (AIV) and Newcastle disease virus (NDV) is widespread in commercial poultry worldwide, therefore optimization of sample collection and transport would be valuable to achieve the best sensitivity and specificity possible, and to develop the most accurate and efficient testing programs. A H7N2 low pathogenicity (LP) AIV strain was selected and used as an indicator virus because it is present in lower concentrations in swabbings and thus requires greater sensitivity for detection compared to highly pathogenic (HP) AIV. For similar reasons a mesogenic strain of NDV was selected. Using oro-pharyngeal and cloacal swabs collected from chickens experimentally exposed to the viruses we evaluated the effects of numerous aspects of sample collection and transport: 1) swab construction material (flocked nylon, non-flocked Dacron, or urethane foam), 2) transport media (brain heart infusion broth [BHI] or phosphate buffered saline [PBS]), 3) media volume (2 ml or 3.5 ml), 4) transporting the swab wet in the vial or removing the swab prior to transport, or transporting the swab dry with no media, and 5) single swabs versus pooling 5 or 11 swabs per vial.ResultsUsing real-time RT-PCR (rRT-PCR), virus isolation (VI) and commercial antigen detection immunoassays for AIV we observed statistically significant differences and consistent trends with some elements of sample collection and transport; media, dry transport and swab construction. Conversely, the number of swabs pooled (1, 5 or 11) and whether the swab was removed prior to transport did not impact virus detection. Similarly, with NDV detection by both VI and rRT-PCR was not affected by the numbers of swabs collected in a single vial (1, 5 or 11).ConclusionsWe observed that flocked and foam swabs were superior to non-flocked swabs, BHI media was better than PBS, and transporting swabs wet was better for virus recovery and detection than transporting them dry. There was no observable difference in detection whether the swab was removed prior to transport or left in the vial. Also, with both AIV and NDV, there was no observed difference in virus detection between pools of 1, 5 or 11 swabs.

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Diagnostics and surveillance methods

2016

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Comparison of Pooling 11 or 5 Oropharyngeal Swabbings for Detecting Avian Influenza Virus by Real-Time Reverse Transcription–PCR in Broiler Chickens

Cited by 14 publications

References 9 publications

Quantifying the effect of swab pool size on the detection of influenza A viruses in broiler chickens and its implications for surveillance

Quantifying the effect of swab pool size on the detection of influenza A viruses in broiler chickens and its implications for surveillance

Optimal specimen collection and transport methods for the detection of avian influenza virus and Newcastle disease virus

Diagnostics and surveillance methods

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