Methods to prevent PCR amplification of DNA from non-viable virus were not successful for infectious laryngotracheitis virus

Bindari, Yugal Raj; Walkden‐Brown, Stephen W.; Gerber, Priscilla F.

doi:10.1371/journal.pone.0232571

Cited by 17 publications

(15 citation statements)

References 32 publications

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“…However, this was not supported by the findings in which infection was unsuccessful with dust or dust extracts collected from infected and clinically sick birds at 3, 7 and 14 dpe and given to 120 susceptible chicks in 6 isolators. This is in agreement with previous report by Bindari et al [ 36 ] that failed to infect cell cultures or chick embryos with qPCR positive dust extracts. These authors also found that spiking dust samples with cultured ILTV reduced the infectivity of the ILTV to chick embryos.…”

Section: Discussionsupporting

confidence: 94%

“…This is reinforced by experimental demonstration of airborne transmission of field and vaccine ILTV strains, potentially due to infective dust particles in the air [ 24 ]. In contrast, Bindari et al [ 36 ] were unable to isolate ILTV from ILTV PCR positive dust samples in either chick embryos or cell culture. Thus the role of poultry dust in the transmission of ILTV remains unresolved.…”

Section: Introductionmentioning

confidence: 99%

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Transmission of infectious laryngotracheitis virus vaccine and field strains: the role of degree of contact and transmission by whole blood, plasma and poultry dust

Yegoraw

Assen

Gerber

et al. 2021

Vet Res

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Understanding the mechanisms of transmission of infectious laryngotracheitis virus (ILTV) is critical to proper control as both vaccine and wild-type strains circulate within chicken flocks with potential adverse consequences. The relative efficiency of transmission by direct contact between chickens and airborne transmission has not been investigated. Furthermore, relatively high levels of ILTV DNA have been detected in poultry dust and blood but the infectivity of these is unknown. In this study, comparison of in-contact and airborne transmission of two vaccine and one field strain of ILTV revealed that all transmitted to 100% of in-contact birds by 6 days post-exposure (dpe). Airborne transmission without contact resulted in 100% transmission by 14 and 17 dpe for the wild-type and Serva vaccine virus but only 27% transmission by 21 dpe for the A20 vaccine virus. The infectivity of dust or extracts of dust and blood or plasma from infected chickens at various stages of infection was assessed by inoculation into susceptible chickens. There was no transmission by any of these materials. In conclusion, direct contact facilitated efficient ILTV transmission but the virus was unable to be transmitted by dust from infected chickens suggestive of a limited role in the epidemiology of ILTV.

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Section: Discussionsupporting

confidence: 94%

Section: Introductionmentioning

confidence: 99%

Transmission of infectious laryngotracheitis virus vaccine and field strains: the role of degree of contact and transmission by whole blood, plasma and poultry dust

Yegoraw

Assen

Gerber

et al. 2021

Vet Res

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“…These included propidium monoazide and immunomagnetic separation tested on laryngotracheitis virus and ethidium monoazide on avian influenza virus. (11,12) It is worth to report that we also tested on inactivated SARS-CoV-2 suspensions a porcine gastric mucine in situ capture RT-qPCR, a method that was originally implemented in our laboratory for human enteric viruses. (20) Although proper SARS-CoV-2 infectious controls could not be included, those experiments resulted in inconclusive outcomes (data not shown).…”

Section: Discussionmentioning

confidence: 99%

“…(10) However, the application of such techniques for enveloped viruses has not fully elucidated as it has failed for avian influenza virus (IAV) and infectious laryngotracheitis virus (ILTV) while it has recently been optimized for porcine epidemic diarrhea coronavirus. (11–13) Nonetheless, the implementation of this technique has not been explored for SARS-CoV-2.…”

Section: Introductionmentioning

confidence: 99%

Viability RT-PCR for SARS-CoV-2: a step forward to solve the infectivity quandary

Cuevas-Ferrando

Randazzo

Pérez-Cataluña

et al. 2021

Preprint

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Background: Isolation, contact tracing and restrictions on social movement are being globally implemented to prevent and control onward spread of SARS-CoV-2, even though the infection risk modelled on RNA detection by RT-qPCR remains biased as viral shedding and infectivity are not discerned. Thus, we aimed to develop a rapid viability RT-qPCR procedure to infer SARS-CoV-2 infectivity in clinical specimens and environmental samples. Methods: We screened monoazide dyes and platinum compounds as viability molecular markers on five SARS-CoV-2 RNA targets. A platinum chloride-based viability RT-qPCR was then optimized using genomic RNA, and inactivated SARS-CoV-2 particles inoculated in buffer, stool, and urine. Our results were finally validated in nasopharyngeal swabs from persons who tested positive for COVID-19 and in wastewater samples positive for SARS-CoV-2 RNA. Findings: We established a rapid viability RT-qPCR that selectively detects potentially infectious SARS-CoV-2 particles in complex matrices. In particular, the confirmed positivity of nasopharyngeal swabs following the viability procedure suggests their potential infectivity, while the complete prevention of amplification in wastewater indicated either non-infectious particles or free RNA. Interpretation: The viability RT-qPCR approach provides a more accurate ascertainment of the infectious viruses detection and it may complement analyses to foster risk-based investigations for the prevention and control of new or re-occurring outbreaks with a broad application spectrum. Fundings: This work was supported by Spanish Scientific Research Council (CSIC), Generalitat Valenciana, and MICINN co-founded by AEI/FEDER, UE.

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“…In addition, dust has also been shown to be useful for the monitoring of pathogens that are primarily transmitted by feather dander such as Marek's disease virus ( Walkden-Brown et al, 2013 ). Respiratory pathogens such as infectious laryngotracheitis virus ( Ahaduzzaman et al, 2019 ), Newcastle disease virus and infectious bronchitis virus ( Tran et al, 2020 ) are detectable in dust samples using PCR although it is not clear whether this represents infective virus from the respiratory tract or inactivated viral nucleic acids present in excreta following passage through the gut ( Bindari et al, 2020 ; Yegoraw et al, 2020 ). It can be expected that pathogens originating in litter material (e.g., litter derived Aspergillus fumigatus ) will also be well represented in dust, however, it should be noted that the proportion of bedding in dust declined to low levels over time as observed in this study.…”

Section: Discussionmentioning

confidence: 99%

Characterization of poultry house dust using chemometrics and scanning electron microscopy imaging

et al. 2021

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Poultry house dust is composed of fine particles which likely originate from a diverse range of materials such as feed, litter, excreta, and feathers. Little is known about the contribution of these sources to broiler house airborne dust so the present study was designed to identify the relative contributions of these sources. Samples of feed, excreta, feather, and bedding, known mixtures of these and settled dust from 28 broiler chicken flocks were tested for the concentration of 18 chemical elements. A chemometrics approach (the application of multivariate statistical techniques to chemical analysis data) was used to identify the primary source material in broiler chicken house dust samples. Scanning electron microscopy ( SEM ) was also used to analyze dust sample particulates based on examination of source materials. Excreta was found to be the main component of broiler chicken house dust, both by SEM and chemometric analysis. SEM of experimental flock dust between 7 and 35 days of age ( d ) revealed that the contribution of excreta to dust increased with age from 60% at 7 d to 95% at 28 d ( P < 0.001). The proportion of bedding and feed in dust declined with age while the contribution of feather material remained low throughout. This study demonstrates that excreta provides the bulk of the material in poultry dust samples with bedding material, feed and feather material providing lower proportions. The relative contributions of these materials to dust varies with age of birds at dust collection. Additional research is required to determine the health and diagnostic implications of this variation.

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Methods to prevent PCR amplification of DNA from non-viable virus were not successful for infectious laryngotracheitis virus

Cited by 17 publications

References 32 publications

Transmission of infectious laryngotracheitis virus vaccine and field strains: the role of degree of contact and transmission by whole blood, plasma and poultry dust

Transmission of infectious laryngotracheitis virus vaccine and field strains: the role of degree of contact and transmission by whole blood, plasma and poultry dust

Viability RT-PCR for SARS-CoV-2: a step forward to solve the infectivity quandary

Characterization of poultry house dust using chemometrics and scanning electron microscopy imaging

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