Your search keyword '"Todd Cutts"' showing total 62 results

1. Inactivation Validation of Ebola, Marburg, and Lassa Viruses in AVL and Ethanol-Treated Viral Cultures

Author

Todd Cutts, Anders Leung, Logan Banadyga, and Jay Krishnan

Subjects

AVL, BSL-4, inactivation validation, Ebola virus, Lassa virus, lysis buffer, Microbiology, QR1-502

Abstract

High-consequence pathogens such as the Ebola, Marburg, and Lassa viruses are handled in maximum-containment biosafety level 4 (BSL-4) laboratories. Genetic material is often isolated from such viruses and subsequently removed from BSL-4 laboratories for a multitude of downstream analyses using readily accessible technologies and equipment available at lower-biosafety level laboratories. However, it is essential to ensure that these materials are free of viable viruses before removal from BSL-4 laboratories to guarantee sample safety. This study details the in-house procedure used for validating the inactivation of Ebola, Marburg, and Lassa virus cultures after incubation with AVL lysis buffer (Qiagen) and ethanol. This study’s findings show that no viable virus was detectable when high-titer cultures of Ebola, Marburg, and Lassa viruses were incubated with AVL lysis buffer for 10 min, followed by an equal volume of 95% ethanol for 3 min, using a method with a sensitivity of ≤0.8 log10 TCID50 as the limit of detection.

Published

2024

2. Standard hospital blanket warming cabinets can be utilized for complete moist heat SARS-CoV2 inactivation of contaminated N95 masks for re-use

Author

Anand Kumar, Samantha B. Kasloff, Todd Cutts, Anders Leung, Naresh Sharma, Gloria Vazquez-Grande, Tracy Drew, Denis Laframboise, Olivero Orofino, Joe Tanelli, and Jay Krishnan

Subjects

Medicine, Science

Abstract

Abstract Shortages of personal protective equipment for use during the SARS-CoV-2 pandemic continue to be an issue among health-care workers globally. Extended and repeated use of N95 filtering facepiece respirators without adequate decontamination is of particular concern. Although several methods to decontaminate and re-use these masks have been proposed, logistic or practical issues limit adoption of these techniques. In this study, we propose and validate the use of the application of moist heat (70 °C with humidity augmented by an open pan of water) applied by commonly available hospital (blanket) warming cabinets to decontaminate N95 masks. This report shows that a variety of N95 masks can be repeatedly decontaminated of SARS-CoV-2 over 6 h moist heat exposure without compromise of their filtering function as assessed by standard fit and sodium chloride aerosol filtration efficiency testing. This approached can easily adapted to provide point-of-care N95 mask decontamination allowing for increased practical utility of mask recycling in the health care setting.

Published

2021

3. Stability of SARS-CoV-2 on critical personal protective equipment

Author

Samantha B. Kasloff, Anders Leung, James E. Strong, Duane Funk, and Todd Cutts

Subjects

Medicine, Science

Abstract

Abstract The spread of COVID-19 in healthcare settings is concerning, with healthcare workers representing a disproportionately high percentage of confirmed cases. Although SARS-CoV-2 virus has been found to persist on surfaces for a number of days, the extent and duration of fomites as a mode of transmission, particularly in healthcare settings, has not been fully characterized. To shed light on this critical matter, the present study provides the first comprehensive assessment of SARS-CoV-2 stability on experimentally contaminated personal protective equipment (PPE) widely used by healthcare workers and the general public. Persistence of viable virus was monitored over 21 days on eight different materials, including nitrile medical examination gloves, reinforced chemical resistant gloves, N-95 and N-100 particulate respirator masks, Tyvek, plastic, cotton, and stainless steel. Unlike previous reports, viable SARS-CoV-2 in the presence of a soil load persisted for up to 21 days on experimentally inoculated PPE, including materials from filtering facepiece respirators (N-95 and N-100 masks) and a plastic visor. Conversely, when applied to 100% cotton fabric, the virus underwent rapid degradation and became undetectable by TCID50 assay within 24 h. These findings underline the importance of appropriate handling of contaminated PPE during and following use in high-risk settings and provide interesting insight into the potential utility of cotton in limiting COVID-19 transmission.

Published

2021

4. Mechanical Wiping Increases the Efficacy of Liquid Disinfectants on SARS-CoV-2

Author

Angela Sloan, Samantha B. Kasloff, and Todd Cutts

Subjects

SARS-CoV-2, biocide, disinfection, fomites, QCT-2, wiping, Microbiology, QR1-502

Abstract

High-touch environmental surfaces are acknowledged as potential sources of pathogen transmission, particularly in health care settings where infectious agents may be readily abundant. Methods of disinfecting these surfaces often include direct application of a chemical disinfectant or simply wiping the surface with a disinfectant pre-soaked wipe (DPW). In this study, we examine the ability of four disinfectants, ethanol (EtOH), sodium hypochlorite (NaOCl), chlorine dioxide (ClO2), and potassium monopersulfate (KMPS), to inactivate SARS-CoV-2 on a hard, non-porous surface, assessing the effects of concentration and contact time. The efficacy of DPWs to decontaminate carriers spiked with SARS-CoV-2, as well as the transferability of the virus from used DPWs to clean surfaces, is also assessed. Stainless steel carriers inoculated with approximately 6 logs of SARS-CoV-2 prepared in a soil load were disinfected within 5 min through exposure to 66.5% EtOH, 0.5% NaOCl, and 1% KMPS. The addition of mechanical wiping using DPWs impregnated with these biocides rendered the virus inactive almost immediately, with no viral transfer from the used DPW to adjacent surfaces. Carriers treated with 100 ppm of ClO2 showed a significant amount of viable virus remaining after 10 min of biocide exposure, while the virus was only completely inactivated after 10 min of treatment with 500 ppm of ClO2. Wiping SARS-CoV-2-spiked carriers with DPWs containing either concentration of ClO2 for 5 s left significant amounts of viable virus on the carriers. Furthermore, higher titers of infectious virus retained on the ClO2-infused DPWs were transferred to uninoculated carriers immediately after wiping. Overall, 66.5% EtOH, 0.5% NaOCl, and 1% KMPS appear to be highly effective biocidal agents against SARS-CoV-2, while ClO2 formulations are much less efficacious.

Published

2022

5. Impact of intensive care unit supportive care on the physiology of Ebola virus disease in a universally lethal non-human primate model

Author

Guillaume Poliquin, Duane Funk, Shane Jones, Kaylie Tran, Charlene Ranadheera, Mable Hagan, Kevin Tierney, Allen Grolla, Amrinder Dhaliwal, Alexander Bello, Anders Leung, Cory Nakamura, Darwyn Kobasa, Darryl Falzarano, Lauren Garnett, Hugues Fausther Bovendo, Heinz Feldmann, Murray Kesselman, Gregory Hansen, Jason Gren, George Risi, Mia Biondi, Todd Mortimer, Trina Racine, Yvon Deschambault, Sam Aminian, Jocelyn Edmonds, Ray Sourette, Mark Allan, Lauren Rondeau, Sharron Hadder, Christy Press, Christine DeGraff, Stephanie Kucas, Bradley W. M. Cook, B. J. Hancock, Anand Kumar, Reeni Soni, Darryl Schantz, Jarrid McKitrick, Bryce Warner, Bryan D. Griffin, Xiangguo Qiu, Gary P. Kobinger, Dave Safronetz, Derek Stein, Todd Cutts, James Kenny, Geoff Soule, Robert Kozak, Steven Theriault, Liam Menec, Robert Vendramelli, Sean Higgins, Guodong Liu, Niaz Md Rahim, Samantha Kasloff, Angela Sloan, Shihua He, Nikesh Tailor, Michael Gray, and James E. Strong

Subjects

Ebola, Supportive care, Fluid, NHP, Vasoactives, Hydrocortisone, Medical emergencies. Critical care. Intensive care. First aid, RC86-88.9

Abstract

Abstract Background There are currently limited data for the use of specific antiviral therapies for the treatment of Ebola virus disease (EVD). While there is anecdotal evidence that supportive care may be effective, there is a paucity of direct experimental data to demonstrate a role for supportive care in EVD. We studied the impact of ICU-level supportive care interventions including fluid resuscitation, vasoactive medications, blood transfusion, hydrocortisone, and ventilator support on the pathophysiology of EVD in rhesus macaques infected with a universally lethal dose of Ebola virus strain Makona C07. Methods Four NHPs were infected with a universally lethal dose Ebola virus strain Makona, in accordance with the gold standard lethal Ebola NHP challenge model. Following infection, the following therapeutic interventions were employed: continuous bedside supportive care, ventilator support, judicious fluid resuscitation, vasoactive medications, blood transfusion, and hydrocortisone as needed to treat cardiovascular compromise. A range of physiological parameters were continuously monitored to gage any response to the interventions. Results All four NHPs developed EVD and demonstrated a similar clinical course. All animals reached a terminal endpoint, which occurred at an average time of 166.5 ± 14.8 h post-infection. Fluid administration may have temporarily blunted a rise in lactate, but the effect was short lived. Vasoactive medications resulted in short-lived improvements in mean arterial pressure. Blood transfusion and hydrocortisone did not appear to have a significant positive impact on the course of the disease. Conclusions The model employed for this study is reflective of an intramuscular infection in humans (e.g., needle stick) and is highly lethal to NHPs. Using this model, we found that the animals developed progressive severe organ dysfunction and profound shock preceding death. While the overall impact of supportive care on the observed pathophysiology was limited, we did observe some time-dependent positive responses. Since this model is highly lethal, it does not reflect the full spectrum of human EVD. Our findings support the need for continued development of animal models that replicate the spectrum of human disease as well as ongoing development of anti-Ebola therapies to complement supportive care.

Published

2019

6. Simulated sunlight decreases the viability of SARS-CoV-2 in mucus

Author

Angela Sloan, Todd Cutts, Bryan D. Griffin, Samantha Kasloff, Zachary Schiffman, Mable Chan, Jonathan Audet, Anders Leung, Darwyn Kobasa, Derek R. Stein, David Safronetz, and Guillaume Poliquin

Subjects

Medicine, Science

Abstract

The novel coronavirus, SARS-CoV-2, has spread into a pandemic since its emergence in Wuhan, China in December of 2019. This has been facilitated by its high transmissibility within the human population and its ability to remain viable on inanimate surfaces for an extended period. To address the latter, we examined the effect of simulated sunlight on the viability of SARS-CoV-2 spiked into tissue culture medium or mucus. The study revealed that inactivation took 37 minutes in medium and 107 minutes in mucus. These times-to-inactivation were unexpected since they are longer than have been observed in other studies. From this work, we demonstrate that sunlight represents an effective decontamination method but the speed of decontamination is variable based on the underlying matrix. This information has an important impact on the development of infection prevention and control protocols to reduce the spread of this deadly pathogen.

Published

2021

7. Aerosol SARS-CoV-2 in hospitals and long-term care homes during the COVID-19 pandemic.

Author

Gary Mallach, Samantha B Kasloff, Tom Kovesi, Anand Kumar, Ryan Kulka, Jay Krishnan, Benoit Robert, Michaeline McGuinty, Sophia den Otter-Moore, Bashour Yazji, and Todd Cutts

Subjects

Medicine, Science

Abstract

BackgroundFew studies have quantified aerosol concentrations of SARS-CoV-2 in hospitals and long-term care homes, and fewer still have examined samples for viability. This information is needed to clarify transmission risks beyond close contact.MethodsWe deployed particulate air samplers in rooms with COVID-19 positive patients in hospital ward and ICU rooms, rooms in long-term care homes experiencing outbreaks, and a correctional facility experiencing an outbreak. Samplers were placed between 2 and 3 meters from the patient. Aerosol (small liquid particles suspended in air) samples were collected onto gelatin filters by Ultrasonic Personal Air Samplers (UPAS) fitted with ResultsIn total, 138 samples were collected from 99 rooms. RNA samples were positive in 9.1% (6/66) of samples obtained with the UPAS 2.5μm samplers, 13.5% (7/52) with the UPAS 10μm samplers, and 10.0% (2/20) samples obtained with the Coriolis samplers. Culturable virus was not recovered in any samples. Viral RNA was detected in 15.1% of the rooms sampled. There was no significant difference in viral RNA recovery between the different room locations or samplers. Method development experiments indicated minimal loss of SARS-CoV-2 viability via the personal air sampler operation.

Published

2021

8. Decontamination of N95 masks for re-use employing 7 widely available sterilization methods.

Author

Anand Kumar, Samantha B Kasloff, Anders Leung, Todd Cutts, James E Strong, Kevin Hills, Frank X Gu, Paul Chen, Gloria Vazquez-Grande, Barret Rush, Sylvain Lother, Kimberly Malo, Ryan Zarychanski, and Jay Krishnan

Subjects

Medicine, Science

Abstract

The response to the COVID-19 epidemic is generating severe shortages of personal protective equipment around the world. In particular, the supply of N95 respirator masks has become severely depleted, with supplies having to be rationed and health care workers having to use masks for prolonged periods in many countries. We sought to test the ability of 7 different decontamination methods: autoclave treatment, ethylene oxide gassing (ETO), low temperature hydrogen peroxide gas plasma (LT-HPGP) treatment, vaporous hydrogen peroxide (VHP) exposure, peracetic acid dry fogging (PAF), ultraviolet C irradiation (UVCI) and moist heat (MH) treatment to decontaminate a variety of different N95 masks following experimental contamination with SARS-CoV-2 or vesicular stomatitis virus as a surrogate. In addition, we sought to determine whether masks would tolerate repeated cycles of decontamination while maintaining structural and functional integrity. All methods except for UVCI were effective in total elimination of viable virus from treated masks. We found that all respirator masks tolerated at least one cycle of all treatment modalities without structural or functional deterioration as assessed by fit testing; filtration efficiency testing results were mostly similar except that a single cycle of LT-HPGP was associated with failures in 3 of 6 masks assessed. VHP, PAF, UVCI, and MH were associated with preserved mask integrity to a minimum of 10 cycles by both fit and filtration testing. A similar result was shown with ethylene oxide gassing to the maximum 3 cycles tested. Pleated, layered non-woven fabric N95 masks retained integrity in fit testing for at least 10 cycles of autoclaving but the molded N95 masks failed after 1 cycle; filtration testing however was intact to 5 cycles for all masks. The successful application of autoclaving for layered, pleated masks may be of particular use to institutions globally due to the virtually universal accessibility of autoclaves in health care settings. Given the ability to modify widely available heating cabinets on hospital wards in well-resourced settings, the application of moist heat may allow local processing of N95 masks.

Published

2020

9. Deep-sequencing of Marburg virus genome during sequential mouse passaging and cell-culture adaptation reveals extensive changes over time

Author

Haiyan Wei, Jonathan Audet, Gary Wong, Shihua He, Xueyong Huang, Todd Cutts, Steven Theriault, Bianli Xu, Gary Kobinger, and Xiangguo Qiu

Subjects

Medicine, Science

Abstract

Abstract Marburg virus (MARV) has caused outbreaks of filoviral hemorrhagic fever since its discovery in 1967. The largest and deadliest outbreak occurred in Angola in 2005, with 252 cases and 227 deaths. In 2014, we developed a mouse-adapted MARV, Angola variant through serial passaging in mice. The mouse-adapted MARV exhibits many of the hallmarks of MARV disease in humans. By applying deep-sequencing to every passage of the virus, we are able to study virus evolution in this host with surprising precision. We show that two regions go through substantial changes: the intergenic region between NP and VP35, as well as the first 100 amino acids of the VP40 protein. Our results also reveal that there were profound changes during the production of the final virus stock in cell culture. Overall, our results show that a handful of regions carry most of the mutations acquired during the adaptation of the virus to a new host and that many mutations become fixed very early during the adaptation process.

Published

2017

10. Correction to: Impact of intensive care unit supportive care on the physiology of Ebola virus disease in a universally lethal non-human primate model

Author

Guillaume Poliquin, Duane Funk, Shane Jones, Kaylie Tran, Charlene Ranadheera, Mable Hagan, Kevin Tierney, Allen Grolla, Amrinder Dhaliwal, Alexander Bello, Anders Leung, Cory Nakamura, Darwyn Kobasa, Darryl Falzarano, Lauren Garnett, Hugues Fausther Bovendo, Heinz Feldmann, Murray Kesselman, Gregory Hansen, Jason Gren, George Risi, Mia Biondi, Todd Mortimer, Trina Racine, Yvon Deschambault, Sam Aminian, Jocelyn Edmonds, Ray Saurette, Mark Allan, Lauren Rondeau, Sharron Hadder, Christy Press, Christine DeGraff, Stephanie Kucas, Bradley W. M. Cook, B. J. Hancock, Anand Kumar, Reeni Soni, Daryl Schantz, Jarrid McKitrick, Bryce Warner, Bryan D. Griffin, Xiangguo Qiu, Gary P. Kobinger, Dave Safronetz, Derek Stein, Todd Cutts, James Kenny, Geoff Soule, Robert Kozak, Steven Theriault, Liam Menec, Robert Vendramelli, Sean Higgins, Logan Banadyga, Guodong Liu, Md Niaz Rahim, Samantha Kasloff, Angela Sloan, Shihua He, Nikesh Tailor, Alixandra Albietz, Brad Pickering, Gary Wong, Michael Gray, and James E. Strong

Subjects

Medical emergencies. Critical care. Intensive care. First aid, RC86-88.9

Abstract

Please note that four authors (Logan Banadyga, Alixandra Albietz, Brad Pickering, and Gary Wong) have been erroneously omitted from the author list in the published original article [1].

Published

2019

11. Bioaerosols and Transmission, a Diverse and Growing Community of Practice

Author

Samira Mubareka, Nicolas Groulx, Eric Savory, Todd Cutts, Steven Theriault, James A. Scott, Chad J. Roy, Nathalie Turgeon, Elizabeth Bryce, George Astrakianakis, Shelley Kirychuk, Matthieu Girard, Gary Kobinger, Chao Zhang, and Caroline Duchaine

Subjects

bioaerosols, microbes, virus, infections, viral dissemination, network, Public aspects of medicine, RA1-1270

Abstract

The transmission of infectious microbes via bioaerosols is of significant concern for both human and animal health. However, gaps in our understanding of respiratory pathogen transmission and methodological heterogeneity persist. New developments have enabled progress in this domain, and one of the major turning points has been the recognition that cross-disciplinary collaborations across spheres of human and animal health, microbiology, biophysics, engineering, aerobiology, infection control, public health, occupational health, and industrial hygiene are essential. Collaborative initiatives support advances in topics such as bioaerosol behavior, dispersion models, risk assessment, risk/exposure effects, and mitigation strategies in clinical, experimental, agricultural, and other field settings. There is a need to enhance the knowledge translation for researchers, stakeholders, and private partners to support a growing network of individuals and agencies to achieve common goals to mitigate inter- and intra-species pathogen transmission via bioaerosols.

Published

2019

12. Characterization of Ebola Virus Risk to Bedside Providers in an Intensive Care Environment

Author

Mia J. Biondi, Lauren Garnett, Alexander Bello, Duane Funk, Philippe Guillaume Poliquin, Shane Jones, Kevin Tierney, Kaylie Tran, Robert A. Kozak, Anders Leung, Allen Grolla, Cory Nakamura, Geoff Soule, Charlene Ranadheera, Mable Hagan, Amrinder Dhaliwal, Darwyn Kobasa, Darryl Falzarano, Hugues Fausther Bovendo, Heinz Feldmann, Murray Kesselman, Gregory Hansen, Jason Gren, Todd Mortimer, Trina Racine, Yvon Deschambault, Jocelyn Edmonds, Sam Aminian, Ray Saurette, Mark Allan, Lauren Rondeau, John Huynh, Sharron Hadder, Christy Press, Christine DeGraff, Stephanie Kucas, Julie Kubay, Kim Azanarsky, Bradley W. M. Cook, BJ Hancock, Anand Kumar, Reeni Soni, Daryl Schantz, Jarrid McKitrick, Bryce Warner, Bryan D. Griffin, Xiangguo Qiu, Gary P. Kobinger, Dave Safronetz, Heidi Wood, Derek R. Stein, Todd Cutts, Brad Pickering, James Kenny, Steven Theriault, Liam Menec, Robert Vendramelli, Sean Higgins, Logan Banadyga, Guodong Liu, Md Niaz Rahim, Samantha Kasloff, Angela Sloan, Shihua He, Nikesh Tailor, Alixandra Albietz, Gary Wong, Michael Gray, Friederike Feldmann, Andrea Marzi, George Risi, and James E. Strong

Subjects

Ebola, nosocomial infection, critical care, viral shedding, environmental contamination, Biology (General), QH301-705.5

Abstract

Background: The 2014–2016 Ebola outbreak in West Africa recapitulated that nosocomial spread of Ebola virus could occur and that health care workers were at particular risk including notable cases in Europe and North America. These instances highlighted the need for centers to better prepare for potential Ebola virus cases; including understanding how the virus spreads and which interventions pose the greatest risk. Methods: We created a fully equipped intensive care unit (ICU), within a Biosafety Level 4 (BSL4) laboratory, and infected multiple sedated non-human primates (NHPs) with Ebola virus. While providing bedside care, we sampled blood, urine, and gastric residuals; as well as buccal, ocular, nasal, rectal, and skin swabs, to assess the risks associated with routine care. We also assessed the physical environment at end-point. Results: Although viral RNA was detectable in blood as early as three days post-infection, it was not detectable in the urine, gastric fluid, or swabs until late-stage disease. While droplet spread and fomite contamination were present on a few of the surfaces that were routinely touched while providing care in the ICU for the infected animal, these may have been abrogated through good routine hygiene practices. Conclusions: Overall this study has helped further our understanding of which procedures may pose the highest risk to healthcare providers and provides temporal evidence of this over the clinical course of disease.

Published

2021

13. Efficacy of microbicides for inactivation of Ebola–Makona virus on a non-porous surface: a targeted hygiene intervention for reducing virus spread

Author

Samantha B Kasloff, Todd Cutts, Catherine Robertson, M. Khalid Ijaz, Steven Theriault, Joseph R. Rubino, and Raymond W. Nims

Subjects

0301 basic medicine, Sodium Hypochlorite, Surface Properties, media_common.quotation_subject, Disinfectant, 030106 microbiology, lcsh:Medicine, Diseases, In Vitro Techniques, Xylenes, medicine.disease_cause, Microbiology, Virus, Article, 03 medical and health sciences, chemistry.chemical_compound, Anti-Infective Agents, Cytopathogenic Effect, Viral, Hygiene, Chlorocebus aethiops, Environmental Microbiology, medicine, Animals, Humans, Chloroxylenol, lcsh:Science, Vero Cells, media_common, Cytopathic effect, Multidisciplinary, Ebola virus, Ethanol, Chemistry, lcsh:R, Health care, Hemorrhagic Fever, Ebola, Ebolavirus, Microbicides for sexually transmitted diseases, 030104 developmental biology, Sodium hypochlorite, Virus Inactivation, lcsh:Q, Porosity, Disinfectants, medicine.drug

Abstract

Microbicides play critical roles in infection prevention and control of Ebola virus by decontaminating high-touch environmental surfaces (HITES), interrupting the virus-HITES-hands nexus. We evaluated the efficacy of formulations containing different microbicidal actives for inactivating Ebola virus–Makona strain (EBOV/Mak) on stainless-steel carriers per ASTM E2197-11. Formulations of sodium hypochlorite (NaOCl) (0.05–1%), ethanol (70%), chloroxylenol (PCMX) (0.12–0.48% by weight) in hard water, and a ready-to-use disinfectant spray with 58% ethanol (EDS), were tested at contact times of 0, or 0.5 to 10 min at ambient temperature. EBOV/Mak was inactivated (> 6 log10) by 70% ethanol after contact times ≥ 2.5 min, by 0.5% and 1% NaOCl or EDS (> 4 log10) at contact times ≥ 5 min, and by 0.12–0.48% PCMX (> 4.2 log10) at contact times ≥ 5 min. Residual infectious virus in neutralized samples was assessed by passage on cells and evaluation for viral cytopathic effect. No infectious virus was detected in cells inoculated with EBOV/Mak exposed to NaOCl (0.5% or 1%), PCMX (0.12% to 0.48%), or EDS for ≥ 5 min. These results demonstrate ≥ 6 log10 inactivation of EBOV/Mak dried on prototypic surfaces by EDS or formulations of NaOCl (≥ 0.5%), PCMX (≥ 0.12%), or 70% ethanol at contact times ≥ 5 min.

Published

2020

14. Rechargeable Potent Anti‐Viral Cotton Grafted with a New Quaternized N‐Chloramine (Adv. Mater. Interfaces 35/2022)

Author

Sarah Currie, Todd Cutts, Samantha Kasloff, Weien Wang, Kimberly Holloway, Sarvesh Logsetty, Anand Kumar, Ayush Kumar, and Song Liu

Subjects

Mechanics of Materials, Mechanical Engineering

Published

2022

15. Standard hospital blanket warming cabinets can be utilized for complete moist heat SARS-CoV2 inactivation of contaminated N95 masks for re-use

Author

Jay Krishnan, Naresh Chand Sharma, Todd Cutts, Denis Laframboise, Tracy Drew, Anders Leung, Samantha B Kasloff, Joe Tanelli, Gloria Vazquez-Grande, Olivero Orofino, and Anand Kumar

Subjects

business.product_category, Time Factors, N95 Respirators, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Science, Point-of-Care Systems, Economic shortage, Diseases, Blanket, Article, Equipment Reuse, Humans, Respirator, Personal protective equipment, Decontamination, Biophysical methods, Multidisciplinary, Waste management, SARS-CoV-2, fungi, Biological techniques, Humidity, Human decontamination, Contamination, Hospitals, Viral infection, Environmental science, Medicine, Infectious diseases, Virus Inactivation, business, Microbiology techniques

Abstract

Shortages of personal protective equipment for use during the SARS-CoV-2 pandemic continue to be an issue among health-care workers globally. Extended and repeated use of N95 filtering facepiece respirators without adequate decontamination is of particular concern. Although several methods to decontaminate and re-use these masks have been proposed, logistic or practical issues limit adoption of these techniques. In this study, we propose and validate the use of the application of moist heat (70 °C with humidity augmented by an open pan of water) applied by commonly available hospital (blanket) warming cabinets to decontaminate N95 masks. This report shows that a variety of N95 masks can be repeatedly decontaminated of SARS-CoV-2 over 6 h moist heat exposure without compromise of their filtering function as assessed by standard fit and sodium chloride aerosol filtration efficiency testing. This approached can easily adapted to provide point-of-care N95 mask decontamination allowing for increased practical utility of mask recycling in the health care setting.

Published

2021

16. Aerosol SARS-CoV-2 in hospitals and long-term care homes during the COVID-19 pandemic

Author

Michaeline McGuinty, Sophia den Otter-Moore, Todd Cutts, Ryan Kulka, Samantha B Kasloff, Gary Mallach, Benoit Robert, Tom Kovesi, Anand Kumar, Jay Krishnan, and Bashour Yazji

Subjects

RNA viruses, Veterinary medicine, Viral Diseases, Pulmonology, Coronaviruses, Air Microbiology, Medical Conditions, Animal Products, Chlorocebus aethiops, Materials, Pathology and laboratory medicine, Multidisciplinary, Agriculture, Medical microbiology, Method development, Hospitals, Infectious Diseases, Vesicular Stomatitis Virus, Physical Sciences, Viruses, Medicine, RNA, Viral, SARS CoV 2, Pathogens, Protein target, Research Article, Coronavirus disease 2019 (COVID-19), SARS coronavirus, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Science, Materials Science, complex mixtures, Microbiology, Rhabdoviruses, Respiratory Disorders, Animals, Humans, Viral rna, Hospital ward, Close contact, Vero Cells, Aerosols, Medicine and health sciences, Biology and life sciences, SARS-CoV-2, Significant difference, fungi, Organisms, Viral pathogens, COVID-19, Covid 19, Long-Term Care, Aerosol, Microbial pathogens, Health Care, Health Care Facilities, Mixtures, Respiratory Infections, Environmental science, Gelatin

Abstract

BackgroundFew studies have quantified aerosol concentrations of SARS-CoV-2 in hospitals and long-term care homes, and fewer still have examined samples for viability. This information is needed to clarify transmission risks beyond close contact.MethodsWe deployed particulate air samplers in rooms with COVID-19 positive patients in hospital ward and ICU rooms, rooms in long-term care homes experiencing outbreaks, and a correctional facility experiencing an outbreak. Samplers were placed between 2 and 3 meters from the patient. Aerosol (small liquid particles suspended in air) samples were collected onto gelatin filters by Ultrasonic Personal Air Samplers (UPAS) fitted with 3), and with a Coriolis Biosampler over 10 minutes (total 1.5m3). Samples were assayed for viable SARS-CoV-2 virus and for the viral genome by multiplex PCR using the E and N protein target sequences. We validated the sampling methods by inoculating gelatin filters with viable vesicular stomatitis virus (VSV), and with three concentrations of viable SARS-CoV-2, operating personal samplers for 16hrs, and quantifying viable virus recovery by TCID50 assay.ResultsIn total, 138 samples were collected from 99 rooms. RNA samples were positive in 9.1% (6/66) of samples obtained with the UPAS 2.5µm samplers, 13.5% (7/52) with the UPAS 10µm samplers, and 10.0% (2/20) samples obtained with the Coriolis samplers. Culturable virus was not recovered in any samples. Viral RNA was detected in 10.9% of the rooms sampled. There was no significant difference in viral RNA recovery between the different room locations or samplers. Method development experiments indicated minimal loss of SARS-CoV-2 viability via the personal air sampler operation.Key FindingsAlthough a subset of aerosol samples exhibited detectable SARS-CoV-2 RNA at low titres, the presence of viable SARS-CoV-2 virus in aerosols appears to be infrequent at >2m distance.

Published

2021

17. In vitro efficacy of topical ophthalmic antiseptics against SARS-CoV-2

Author

Tina Felfeli, Todd Cutts, Sherif El-Defrawy, Samantha B Kasloff, Jay Krishnan, and Tony Mazzulli

Subjects

medicine.medical_specialty, Coronavirus disease 2019 (COVID-19), experimental & laboratory, Contact time, business.industry, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), public health, COVID-19, tears, Antiseptic solutions, RE1-994, infection, Ophthalmology, Editorial, Internal medicine, Healthy individuals, Chlorhexidine gluconate, medicine, Tears, business, Healthcare providers

Abstract

Shedding of SARS-CoV-2 in tears of patients with COVID-19 has been reported,1 2 which could serve as a source of infection for healthy individuals, including healthcare providers. The current standard antiseptic solutions used in ophthalmology in the setting of inoffice procedures and operating rooms include povidone-iodine (PVI) 5% and chlorhexidine gluconate (CHX) 0.1% or 0.05%, which are at concentrations that are lower than those used in other surgical specialties. Although laboratory and clinical studies to date have aimed to evaluate the virucidal benefits of routine PVI use for ophthalmic surgeries,3 currently there are no established guidelines regarding the optimal contact time and efficacy of varying dilutions as well as comparisons with other formulations such as CHX. Rigorous evaluation of the efficacy of virucidal agents for disinfecting ocular surface of potentially infected patients with SARS-CoV-2 is critical in mitigating the risk of transmission. In the current study, we evaluated the virucidal efficacy and contact times for commonly used ophthalmic concentrations of PVI and CHX against SARS-CoV-2 using Vero E6 cells as indicator cell lines for residual viable virus based on previously established methodologies (online supplemental appendix).4–6 PVI (5% weight per volume, w/v) and CHX (0.05% and 0.1% w/v) were tested at full strength. Fifty microlitres of ophthalmic formulations …

Published

2021

18. Efficacy Testing of Personal Protective Filters on Biosafety Level 4 Positive Pressure Suits

Author

Samantha B Kasloff, Todd Cutts, Anders Leung, Jay Krishnan, Gabriel Lightly, Laura Landry, and Greg Fey

Subjects

Biosafety level 4, 0303 health sciences, 030306 microbiology, business.industry, Health, Toxicology and Mutagenesis, Public Health, Environmental and Occupational Health, Positive pressure, Original Articles, 030501 epidemiology, Management, Monitoring, Policy and Law, medicine.disease, Biocontainment, Positive pressure breathing, 03 medical and health sciences, Medicine, Medical emergency, 0305 other medical science, business, Personal protective equipment, Biotechnology

Abstract

Introduction: Positive pressure breathing air-fed protective suits from three vendors are commonly used in biosafety level 4 (BSL-4) laboratories: they are Dover Chemturion suits (ILC Dover, DE), Delta suits (Honeywell Safety, NC), and HVO suits (HVO-ISSI-Deutschland GmbH, Germany). To address the potential risk of infectious agents being introduced through the supplied breathing air stream, some suit manufacturers incorporate protective filters on the suits themselves. However, these integrated filters are not amenable to in situ testing for efficacy verification. We have been using external filters from Matheson USA on the positive pressure suits since our BSL-4 laboratories were commissioned two decades ago. As part of our BSL-4 protective suit management program, we test these filters before them being put into use, and annually thereafter. In the past few years, we have observed these filters failing at a higher rate, as high as two out of three of the new filters tested at one point. Objective: The purpose of this study was to procure personal protective filters from other sources and validate their efficacy long-term. Methods: Filters from Respirex, HVO, and Honeywell were validated for filter integrity and filter loading. Results: Respirex filters performed well during the initial testing and periodic testing thereafter. Regular testing of the Respirex filters has now been ongoing for 30 months with continued successful performance. Conclusion: Filters from Respirex are a suitable option to protect personnel wearing positive pressure suits in BSL-4 laboratories.

Published

2021

19. Effectiveness of Dettol Antiseptic Liquid for Inactivation of Ebola Virus in Suspension

Author

Todd Cutts, Steven Theriault, Joseph R. Rubino, Raymond W. Nims, and M. Khalid Ijaz

Subjects

0301 basic medicine, Serial dilution, medicine.drug_class, lcsh:Medicine, Xylenes, medicine.disease_cause, Virus, Article, 03 medical and health sciences, Ebola virus, 0302 clinical medicine, Antiseptic, Suspensions, Chlorocebus aethiops, medicine, Animals, Humans, lcsh:Science, Vero Cells, Cytopathic effect, Multidisciplinary, Chemistry, lcsh:R, Outbreak, Hemorrhagic Fever, Ebola, Antivirals, Ebolavirus, Virology, Titer, 030104 developmental biology, Vero cell, Anti-Infective Agents, Local, Virus Inactivation, lcsh:Q, 030217 neurology & neurosurgery

Abstract

The efficacy of Dettol Antiseptic Liquid (DAL) for inactivating Ebola virus (Makona C07 variant) (EBOV/Mak) within an organic load in suspension was evaluated per ASTM E1052-11. Three DAL lots were evaluated at dilutions of 1:10, 1:20, and 1:40, with contact times of 0.5, 1, 5, and 10 min. Approximately 7 log10 tissue culture infectious dose50 (TCID50) of EBOV/Mak was exposed to DAL at ambient temperature. Each dilution tested reduced the infectious EBOV/Mak titer by ~5 log10 within one min. Detectable virus was still present after an 0.5-min exposure, but each DAL dilution caused >4 log10 reduction within this time. Detection of virus below the limit of detection of the TCID50 assay was assessed by inoculating flasks of Vero E6 cells with undiluted neutralized sample and evaluating the cultures for cytopathic effect after 14 days incubation. No infectious virus was detected with this non-quantitative method in samples subjected to DAL for 5 or 10 min, regardless of the dilution evaluated. The rapid and substantial inactivation of EBOV/Mak by DAL suggests that use of this hygiene product could help prevent the spread of Ebola virus disease during outbreaks.

Published

2019

20. Correction for Cutts et al., 'Inactivating Zaire Ebolavirus in Whole-Blood Thin Smears Used for Malaria Diagnosis'

Author

Todd Cutts, P. Guillaume Poliquin, Bradley W. M. Cook, Steven Theriault, and James E. Strong

Subjects

Microbiology (medical), Zaire ebolavirus, Microbial Viability, Time Factors, business.industry, Methanol, medicine.disease_cause, medicine.disease, Ebolavirus, Virology, Malaria, Disinfection, Blood, parasitic diseases, Medicine, Humans, Parasitology, business, Author Correction, Whole blood, Disinfectants

Abstract

Malaria is an important mimic or coinfection in potential Ebolavirus disease patients. Here, we evaluated the efficacy of the 100% methanol-inactivating Zaire Ebolavirus Makona variant for malaria thin-smear preparation. We determined that 100% methanol completely inactivated the virus after 15 min.

Published

2021

21. Decontamination of N95 Respirators using Moist Heat Delivered by Hospital Blanket Warming Cabinets: A Widely Available Method for N95 Re-Processing

Author

Jay Krishnan, Gloria Vazquez-Grande, Samantha B Kasloff, Joe Tanelli, Tracy Drew, Denis Laframboise, Anand Kumar, Anders Leung, Olivero Orofino, Naresh Chand Sharma, and Todd Cutts

Subjects

business.product_category, Waste management, Environmental science, Human decontamination, Blanket, Respirator, business

Abstract

Shortages of personal protective equipment for use during the SARS-CoV-2 pandemic continue to be an issue among health-care workers globally. Extended and repeated use of N95 filtering facepiece respirators without adequate decontamination is of particular concern. Although several methods to decontaminate and re-use these masks have been proposed, logistic or practical issues limit adoption of these techniques. In this study, we propose and validate the use of the application of moist heat (70oC with humidity augmented by an open pan of water) applied by commonly available hospital (blanket) warming cabinets to decontaminate N95 masks. This report shows that a variety of N95 masks can be repeatedly decontaminated of SARS-CoV-2 over 6 hours moist heat exposure without compromise of their filtering function as assessed by standard fit and sodium chloride aerosol filtration efficiency testing. This approached can easily adapted to provide point-of-care N95 mask decontamination allowing for increased practical utility of mask recycling in the health care setting.

Published

2021

22. Stability of SARS-CoV-2 on critical personal protective equipment

Author

Todd Cutts, Anders Leung, Duane J. Funk, Samantha B Kasloff, and James E. Strong

Subjects

0301 basic medicine, 2019-20 coronavirus outbreak, business.product_category, Coronavirus disease 2019 (COVID-19), Surface Properties, Science, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), 030106 microbiology, Policy and public health in microbiology, Article, 03 medical and health sciences, 0302 clinical medicine, Viral genetics, Virology, Environmental health, Medicine, 030212 general & internal medicine, Respirator, Personal Protective Equipment, Personal protective equipment, Multidisciplinary, SARS-CoV-2, business.industry, Limiting, Healthcare settings, RNA, Viral, business, Porosity

Abstract

The spread of COVID-19 in healthcare settings is concerning, with healthcare workers representing a disproportionately high percentage of confirmed cases. Although SARS-CoV-2 virus has been found to persist on surfaces for a number of days, the extent and duration of fomites as a mode of transmission, particularly in healthcare settings, has not been fully characterized. To shed light on this critical matter, the present study provides the first comprehensive assessment of SARS-CoV-2 stability on experimentally contaminated personal protective equipment (PPE) widely used by healthcare workers and the general public. Persistence of viable virus was monitored over 21 days on eight different materials, including nitrile medical examination gloves, reinforced chemical resistant gloves, N-95 and N-100 particulate respirator masks, Tyvek, plastic, cotton, and stainless steel. Unlike previous reports, viable SARS-CoV-2 in the presence of a soil load persisted for up to 21 days on experimentally inoculated PPE, including materials from filtering facepiece respirators (N-95 and N-100 masks) and a plastic visor. Conversely, when applied to 100% cotton fabric, the virus underwent rapid degradation and became undetectable by TCID50 assay within 24 h. These findings underline the importance of appropriate handling of contaminated PPE during and following use in high-risk settings and provide interesting insight into the potential utility of cotton in limiting COVID-19 transmission.

Published

2021

23. Decontamination of Common Healthcare Facility Surfaces Contaminated with SARS-CoV-2 using Peracetic Acid Dry Fogging

Author

Jay Krishnan, David Safronetz, Todd Cutts, and Samantha B Kasloff

Subjects

Microbiology (medical), Fogging, Surface Properties, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), 030501 epidemiology, Article, 03 medical and health sciences, chemistry.chemical_compound, Peracetic acid, Intensive care, Equipment Reuse, Medicine, Peracetic Acid, Decontamination, Infectious virus, 0303 health sciences, SARS-CoV-2, 030306 microbiology, business.industry, COVID-19, General Medicine, Human decontamination, biochemical phenomena, metabolism, and nutrition, Contamination, Computer keyboard, Pulp and paper industry, Dry fogging, Infectious Diseases, chemistry, Fumigation, Environmental science, Health Facilities, 0305 other medical science, business, Disinfectants

Abstract

BackgroundThe SARS-Cov-2 pandemic has highlighted the urgent need for safe and effective surface decontamination methods, particularly in healthcare settings.MethodsThe effectiveness of peracetic acid (PAA) dry fogging in decontaminating common healthcare setting surfaces was evaluated after experimentally contaminating nine surfaces (stainless steel, latex painted wood, unsealed hardwood, melamine countertop, vinyl flooring, clear plastic, faux leather, computer keyboard button and smartphone touch screen) with more than 106 TCID50 of SARS-CoV-2.ResultsWhen fumigated with PAA dry fog for an hour, no infectious SARS-CoV-2 virus was recovered from experimentally inoculated coupons of representing nine different surface types. In contrast, high titer recovery of infectious virus was demonstrated for corresponding untreated drying controls of the same materials.ConclusionStandard surface decontaminating processes, including sprays and wipes, are laborious and often cannot completely decontaminate sensitive electronic equipment. The ease of use, low cost and overall effectiveness of a PAA dry fogging suggest it should be considered for decontaminating settings, particularly intensive care units where severely ill SARS-CoV-2 patients are cared for.

Published

2020

24. Simulated sunlight decreases the viability of SARS-CoV-2

Author

Jonathan Audet, Bryan D. Griffin, Samantha B Kasloff, Todd Cutts, Zachary Schiffman, Mable Chan, Angela Sloan, Darwyn Kobasa, Anders Leung, Guillaume Poliquin, and Derek R. Stein

Subjects

Sunlight, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Environmental science, skin and connective tissue diseases, Virology

Abstract

The novel coronavirus, SARS-CoV-2, has spread into a pandemic since its emergence in Wuhan, China in December of 2019. This has been facilitated by its high transmissibility within the human population and its ability to remain viable on inanimate surfaces for an extended period. To address the latter, we examined the ability of sunlight to degrade SARS-CoV-2 on stainless steel. All assays were performed using a solar simulator at the equivalent of one air mass (i.e. equatorial sun at its Zenith). Heat-controlled experiments were conducted at approximately 34% relative humidity (RH); otherwise, RH decreased with sunlight exposure until a constant temperature was maintained. When initially suspended in tissue culture medium, the virus was rendered non-viable after two hours of sunlight exposure. However, when suspended in an organic matrix designed to mimic bodily secretions, three hours of continuous sunlight was required for complete degradation. From this work, we demonstrate that sunlight represents an effective decontamination method but the speed of decontamination is variable based on the underlying matrix. This information has an important impact on the development of infection prevention and control protocols to reduce the spread of this deadly pathogen.

Published

2020

25. Kyasanur Forest disease virus non-mouse animal models: a pilot study

Author

Darwyn Kobasa, Steven Theriault, Todd Cutts, Aidan M. Nikiforuk, Bradley W. M. Cook, K. Tierny, and University of Manitoba

Subjects

0301 basic medicine, Guinea Pigs, 030106 microbiology, Datasets as Topic, lcsh:Medicine, Pilot Projects, Spleen, Data Note, Virus Replication, Severity of Illness Index, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Cricetinae, medicine, Hamster, Ferret, Animals, Animal model, Kyasanur Forest disease virus, lcsh:Science (General), lcsh:QH301-705.5, Tropism, biology, Infectious dose, Flavivirus, lcsh:R, Ferrets, General Medicine, biology.organism_classification, medicine.disease, Guinea pig, Virology, Tick-borne, Kyasanur Forest Disease, Disease Models, Animal, Viral Tropism, 030104 developmental biology, medicine.anatomical_structure, Viral replication, lcsh:Biology (General), Tissue tropism, Viral load, Kyasanur forest disease, lcsh:Q1-390

Abstract

Objectives Mouse models have delivered variable recapitulation of Kyasanur Forest disease (KFD) pathology and consistently demonstrated neurological involvement which may be a limited feature of human disease. With the purpose of more accurately modelling human disease progression we infected several small-mammalian models: guinea pigs, hamsters and ferrets with a titered infectious dose of Kyasanur Forest disease virus (KFDV). Clinical indicators of disease severity were observed for seventeen days, on day eighteen a visual post-mortem analysis of visceral organs was conducted. Viral load in selected tissues was measured to infer disease signs and the establishment of viral replication. Data description Daily monitoring did not reveal any observable signs of illness; weight loss was minimal across species and gross pathology did not indicate severe viral infection. Tissue specific tropism and establishment of viral infection was monitored by quantitative real-time polymerase chain reaction (qRT-PCR). No viral replication was detected in ferrets (n = 0/3), but was present in the spleen of guinea pigs (n = 3/3) and the brain of hamsters (n = 3/3). Low levels of viral RNA were detected in multiple hamster tissues (kidney, liver, lung and spleen) suggesting the possibility of viral tropism and possible adaptation to the host. No serological tests were performed.

Published

2020

26. Stability of SARS-CoV-2 on Critical Personal Protective Equipment

Author

James E. Strong, Todd Cutts, Samantha B Kasloff, and Duane J. Funk

Subjects

Toxicology, business.product_category, Coronavirus disease 2019 (COVID-19), business.industry, Tyvek, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Healthcare settings, Medicine, Limiting, Respirator, business, Personal protective equipment

Abstract

The spread of COVID-19 in healthcare settings is concerning, with healthcare workers representing a disproportionately high percentage of confirmed cases. Although SARS-CoV-2 virus has been found to persist on surfaces for a number of days, the extent and duration of fomites as a mode of transmission, particularly in healthcare settings, has not been fully characterized. To shed light on this critical matter, the present study provides the first comprehensive assessment of SARS-CoV-2 stability on experimentally contaminated personal protective equipment (PPE) widely used by healthcare workers and the general public. Persistence of viable virus was monitored over 21 days on eight different materials, including nitrile medical examination gloves, reinforced chemical resistant gloves, N-95 and N-100 particulate respirator masks, Tyvek®, plastic, cotton, and stainless steel. Unlike previous reports, viable SARS-CoV-2 in the presence of a soil load persisted for up to 21 days on experimentally inoculated PPE, including materials from filtering facepiece respirators (N-95 and N-100 masks) and a plastic visor. Conversely, when applied to 100% cotton fabric, the virus underwent rapid degradation and became undetectable in less than 24 hours. These findings underline the importance of appropriate handling of contaminated PPE during and following use in high-risk settings and provide interesting insight into the potential utility of cotton, including cotton masks, in limiting COVID-19 transmission.

Published

2020

27. N95 Mask Decontamination using Standard Hospital Sterilization Technologies

Author

Jay Krishnan, Samantha B Kasloff, Ryan Zarychanski, Kevin Hills, James E. Strong, Gloria Vazquez-Grande, Anders Leung, Todd Cutts, Sylvain A. Lother, Barret Rush, and Anand Kumar

Subjects

business.product_category, Fogging, Waste management, Human decontamination, Sterilization (microbiology), Autoclave, chemistry.chemical_compound, chemistry, Peracetic acid, Environmental science, Respirator, business, Hydrogen peroxide, Personal protective equipment

Abstract

The response to the COVID-19 epidemic is generating severe shortages of personal protective equipment around the world. In particular, the supply of N95 respirator masks has become severely depleted, with supplies having to be rationed and health care workers having to use masks for prolonged periods in many countries. We sought to test the ability of 5 different decontamination methods: autoclave treatment, ethylene oxide gassing, low temperature hydrogen peroxide gas plasma treatment, vaporous hydrogen peroxide exposure and peracetic acid dry fogging to decontaminate a variety of different N95 masks of experimental contamination with SARS-CoV-2 or Vesicular stomatitis virus as a surrogate. In addition, we sought to determine whether masks would tolerate repeated cycles of decontamination while maintaining structural and functional integrity. We found that one cycle of treatment with all modalities was effective in decontamination and was associated with no structural or functional deterioration. Vaporous hydrogen peroxide, peracetic acid dry fogging and autoclave treatments were associated with no loss of structural or functional integrity to a minimum of 10 cycles for the mask models tested. The molded N95 masks however tolerated only 1 cycle of autoclaving. The successful application of autoclaving for layered fabric, pleated masks may be of particular use to institutions globally due to the virtually universal accessibility of autoclaves in health care settings.

Published

2020

28. Simulated sunlight decreases the viability of SARS-CoV-2 in mucus

Author

Bryan D. Griffin, Darwyn Kobasa, Angela Sloan, Todd Cutts, Anders Leung, Derek R. Stein, Jonathan Audet, Guillaume Poliquin, Mable Chan, Samantha B Kasloff, David Safronetz, and Zachary Schiffman

Subjects

RNA viruses, Light, Coronaviruses, Physiology, medicine.disease_cause, Mathematical and Statistical Techniques, Pathogen, Pathology and laboratory medicine, Decontamination, Virus Testing, Coronavirus, education.field_of_study, Multidisciplinary, Microbial Viability, Physics, Electromagnetic Radiation, Statistics, Medical microbiology, Body Fluids, Viruses, Physical Sciences, Sunlight, Regression Analysis, Medicine, Solar Radiation, SARS CoV 2, Pathogens, Anatomy, Research Article, Ultraviolet radiation, 2019-20 coronavirus outbreak, SARS coronavirus, Science, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Population, Linear Regression Analysis, Biology, Research and Analysis Methods, Microbiology, Diagnostic Medicine, medicine, Humans, Statistical Methods, Saliva, education, Medicine and health sciences, Biology and life sciences, SARS-CoV-2, Organisms, Viral pathogens, COVID-19, Mucus, Microbial pathogens, Virus Inactivation, Ultraviolet B, Mathematics

Abstract

The novel coronavirus, SARS-CoV-2, has spread into a pandemic since its emergence in Wuhan, China in December of 2019. This has been facilitated by its high transmissibility within the human population and its ability to remain viable on inanimate surfaces for an extended period. To address the latter, we examined the effect of simulated sunlight on the viability of SARS-CoV-2 spiked into tissue culture medium or mucus. The study revealed that inactivation took 37 minutes in medium and 107 minutes in mucus. These times-to-inactivation were unexpected since they are longer than have been observed in other studies. From this work, we demonstrate that sunlight represents an effective decontamination method but the speed of decontamination is variable based on the underlying matrix. This information has an important impact on the development of infection prevention and control protocols to reduce the spread of this deadly pathogen.

Published

2021

29. Impact of intensive care unit supportive care on the physiology of Ebola virus disease in a universally lethal non-human primate model

Author

Michael Gray, Shane Jones, Niaz Rahim, Samantha B Kasloff, Alexander Bello, Ray Saurette, Jarrid McKitrick, Charlene Ranadheera, Heinz Feldmann, Lauren Garnett, Kevin Tierney, Todd Cutts, Amrinder Dhaliwal, Steven Theriault, Darwyn Kobasa, Angela Sloan, Jason Gren, Nikesh Tailor, Cory Nakamura, Lauren Rondeau, James Kenny, Robert Vendramelli, Guodong Liu, Brad S. Pickering, Xiangguo Qiu, D Safronetz, Robert A. Kozak, B.J. Hancock, Jocelyn Edmonds, Mia J. Biondi, Yvon Deschambault, Reeni Soni, Sharron Hadder, Stephanie Kucas, James E. Strong, Liam Menec, Bradley W. M. Cook, Kaylie Tran, George Risi, Geoff Soule, Christy Press, Sam Aminian, Logan Banadyga, Gary P. Kobinger, Darryl Falzarano, Gary Wong, Sean Higgins, Daryl Schantz, Christine DeGraff, Bryan D. Griffin, Hugues Fausther Bovendo, Shihua He, Duane J. Funk, Anand Kumar, Anders Leung, Mable Hagan, Mark F. Allan, Trina Racine, Todd Mortimer, Murray Kesselman, Allen Grolla, Gregory Hansen, Alixandra Albietz, Bryce M. Warner, Derek R. Stein, Guillaume Poliquin, and University of Manitoba

Subjects

medicine.medical_specialty, Vasoactives, Hydrocortisone, MEDLINE, NHP, Disease, Critical Care and Intensive Care Medicine, medicine.disease_cause, Pathophysiology, law.invention, 03 medical and health sciences, 0302 clinical medicine, law, medicine, 030212 general & internal medicine, Intensive care medicine, 030304 developmental biology, 0303 health sciences, Ebola virus, Non human primate, business.industry, Research, Published Erratum, lcsh:Medical emergencies. Critical care. Intensive care. First aid, Correction, lcsh:RC86-88.9, Intensive care unit, 3. Good health, Ventilatory support, Ebola, Fluid, business, Supportive care

Abstract

BackgroundThere are currently limited data for the use of specific antiviral therapies for the treatment of Ebola virus disease (EVD). While there is anecdotal evidence that supportive care may be effective, there is a paucity of direct experimental data to demonstrate a role for supportive care in EVD. We studied the impact of ICU-level supportive care interventions including fluid resuscitation, vasoactive medications, blood transfusion, hydrocortisone, and ventilator support on the pathophysiology of EVD in rhesus macaques infected with a universally lethal dose of Ebola virus strain Makona C07.MethodsFour NHPs were infected with a universally lethal dose Ebola virus strain Makona, in accordance with the gold standard lethal Ebola NHP challenge model. Following infection, the following therapeutic interventions were employed: continuous bedside supportive care, ventilator support, judicious fluid resuscitation, vasoactive medications, blood transfusion, and hydrocortisone as needed to treat cardiovascular compromise. A range of physiological parameters were continuously monitored to gage any response to the interventions.ResultsAll four NHPs developed EVD and demonstrated a similar clinical course. All animals reached a terminal endpoint, which occurred at an average time of 166.5 ± 14.8 h post-infection. Fluid administration may have temporarily blunted a rise in lactate, but the effect was short lived. Vasoactive medications resulted in short-lived improvements in mean arterial pressure. Blood transfusion and hydrocortisone did not appear to have a significant positive impact on the course of the disease.ConclusionsThe model employed for this study is reflective of an intramuscular infection in humans (e.g., needle stick) and is highly lethal to NHPs. Using this model, we found that the animals developed progressive severe organ dysfunction and profound shock preceding death. While the overall impact of supportive care on the observed pathophysiology was limited, we did observe some time-dependent positive responses. Since this model is highly lethal, it does not reflect the full spectrum of human EVD. Our findings support the need for continued development of animal models that replicate the spectrum of human disease as well as ongoing development of anti-Ebola therapies to complement supportive care.

Published

2019

30. Hand hygiene: virucidal efficacy of a liquid hand wash product against Ebola virus

Author

M.K. Ijaz, E. Bruning, J.R. Rubino, Steven Theriault, R.W. Nims, and Todd Cutts

Subjects

Hand washing, Hand wash, Liquid hand wash, Ebola virus inactivation, Contact time, viruses, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), media_common.quotation_subject, medicine.disease_cause, lcsh:Infectious and parasitic diseases, Hygiene, medicine, lcsh:RC109-216, Original Research Article, media_common, Coronavirus, Ebola virus, business.industry, lcsh:Public aspects of medicine, lcsh:RA1-1270, Ebola virus (Makona C07 variant), Virology, Titer, Prevention of spread of infectious agents including high-risk viruses, business, Emerging/re-emerging viruses, Hand hygiene

Abstract

Summary Background Hand washing is an important targeted hygiene intervention for limiting the spread of infectious agents, including the Ebola virus, which continues to re-emerge. We have assessed the virucidal efficacy of a commercially available liquid hand wash product (LHW) for inactivating Ebola virus. Methods The ASTM E1052-11 Standard was used to evaluate the efficacy of an LHW containing the microbicidal active salicylic acid for inactivating Ebola virus - Makona variant suspended in an organic load. Three concentrations (12.5%, 25%, 50%) of three lots of LHW prepared in 440 ppm hard water were evaluated at room temperature for 20, 30, and 60 s contact time. Results A 25% solution of the LHW caused 4.5 log10 and 4.8 log10 reduction in Ebola virus titer within 20 and 30 s, respectively. The efficacy of a 12.5% LHW solution was lower (1.9 and 2.0 log10 reduction in titer within 20 and 30 s, respectively). The efficacy of the 50% LHW solution could not be measured, due to inability to sufficiently neutralize the LHW at the end of exposure. Conclusion These results suggest the potential utility of an appropriately formulated liquid hand wash agent during Ebola virus disease outbreaks for use within healthcare, community, and home settings. Such an LHW should also be effective against other enveloped viruses, such as the pandemic coronavirus SARS-CoV-2.

Published

2021

31. Characterization of Ebola Virus Risk to Bedside Providers in an Intensive Care Environment

Author

Logan Banadyga, Darryl Falzarano, Hugues Fausther Bovendo, Shihua He, Christine DeGraff, Todd Mortimer, Lauren Rondeau, Daryl Schantz, Guodong Liu, Mark F. Allan, Yvon Deschambault, Anders Leung, Sean Higgins, Steven Theriault, Murray Kesselman, Gary P. Kobinger, George Risi, Darwyn Kobasa, Sharron Hadder, Cory Nakamura, Duane J. Funk, Friederike Feldmann, Bradley W. M. Cook, Shane Jones, Reeni Soni, Gregory Hansen, Philippe Guillaume Poliquin, Ray Saurette, Alixandra Albietz, Heidi Wood, Bryce M. Warner, Todd Cutts, Anand Kumar, Mable Hagan, Samantha B Kasloff, Heinz Feldmann, Robert Vendramelli, Bryan D. Griffin, Stephanie Kucas, James E. Strong, Niaz Rahim, James Kenny, John Huynh, Charlene Ranadheera, Andrea Marzi, D Safronetz, Xiangguo Qiu, Kaylie Tran, Allen Grolla, Kevin Tierney, Michael Gray, Jocelyn Edmonds, Sam Aminian, Geoff Soule, Amrinder Dhaliwal, Nikesh Tailor, Derek R. Stein, Gary Wong, B.J. Hancock, Julie Kubay, Kimberly Azanarsky, Alexander Bello, Angela Sloan, Jason Gren, Lauren Garnett, Brad S. Pickering, Mia J. Biondi, Robert A. Kozak, Christy Press, Jarrid McKitrick, Trina Racine, and Liam Menec

Subjects

0301 basic medicine, Microbiology (medical), viral shedding, medicine.medical_specialty, environmental contamination, viruses, media_common.quotation_subject, Disease, medicine.disease_cause, Microbiology, Article, law.invention, 03 medical and health sciences, 0302 clinical medicine, Hygiene, law, Virology, Intensive care, Health care, Medicine, 030212 general & internal medicine, Viral shedding, Intensive care medicine, lcsh:QH301-705.5, media_common, Ebola virus, business.industry, virus diseases, Outbreak, Intensive care unit, 3. Good health, critical care, 030104 developmental biology, lcsh:Biology (General), nosocomial infection, Ebola, business

Abstract

Background: The 2014–2016 Ebola outbreak in West Africa recapitulated that nosocomial spread of Ebola virus could occur and that health care workers were at particular risk including notable cases in Europe and North America. These instances highlighted the need for centers to better prepare for potential Ebola virus cases, including understanding how the virus spreads and which interventions pose the greatest risk. Methods: We created a fully equipped intensive care unit (ICU), within a Biosafety Level 4 (BSL4) laboratory, and infected multiple sedated non-human primates (NHPs) with Ebola virus. While providing bedside care, we sampled blood, urine, and gastric residuals, as well as buccal, ocular, nasal, rectal, and skin swabs, to assess the risks associated with routine care. We also assessed the physical environment at end-point. Results: Although viral RNA was detectable in blood as early as three days post-infection, it was not detectable in the urine, gastric fluid, or swabs until late-stage disease. While droplet spread and fomite contamination were present on a few of the surfaces that were routinely touched while providing care in the ICU for the infected animal, these may have been abrogated through good routine hygiene practices. Conclusions: Overall this study has helped further our understanding of which procedures may pose the highest risk to healthcare providers and provides temporal evidence of this over the clinical course of disease.

Published

2021

32. Decontamination of N95 masks for re-use employing 7 widely available sterilization methods

Author

Barret Rush, Kevin Hills, Kimberly Malo, Gloria Vazquez-Grande, Paul Z. Chen, Samantha B Kasloff, Anders Leung, Sylvain A. Lother, James E. Strong, Jay Krishnan, Todd Cutts, Frank X. Gu, Ryan Zarychanski, and Anand Kumar

Subjects

Ethylene Oxide, RNA viruses, business.product_category, Plasma Gases, Light, Sanitization, Coronaviruses, 02 engineering and technology, Respirators, Autoclave, law.invention, chemistry.chemical_compound, Medical Conditions, law, Peracetic acid, Medicine and Health Sciences, Public and Occupational Health, Respirator, Decontamination, Pathology and laboratory medicine, Virus Testing, 0303 health sciences, Multidisciplinary, Physics, Oxides, Human decontamination, Medical microbiology, 021001 nanoscience & nanotechnology, Pulp and paper industry, Peroxides, Equipment Sterilization, Physical sciences, Chemistry, Infectious Diseases, Vesicular Stomatitis Virus, Viruses, Medicine, Engineering and Technology, SARS CoV 2, Pathogens, 0210 nano-technology, Research Article, Biotechnology, Equipment Preparation, Ultraviolet radiation, Materials science, Infectious Disease Control, SARS coronavirus, N95 Respirators, Ultraviolet Rays, Science, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Bioengineering, Research and Analysis Methods, Microbiology, Rhabdoviruses, 03 medical and health sciences, Electromagnetic radiation, Diagnostic Medicine, Equipment Reuse, Humans, Peracetic Acid, Personal protective equipment, Filtration, Biology and life sciences, SARS-CoV-2, 030306 microbiology, Organisms, Viral pathogens, Chemical Compounds, COVID-19, Hydrogen Peroxide, Vesiculovirus, Microbial pathogens, Health Care, Autoclaving, chemistry, Medical Devices and Equipment, Preventive Medicine, Ultraviolet C, business

Abstract

The response to the COVID-19 epidemic is generating severe shortages of personal protective equipment around the world. In particular, the supply of N95 respirator masks has become severely depleted, with supplies having to be rationed and health care workers having to use masks for prolonged periods in many countries. We sought to test the ability of 7 different decontamination methods: autoclave treatment, ethylene oxide gassing (ETO), low temperature hydrogen peroxide gas plasma (LT-HPGP) treatment, vaporous hydrogen peroxide (VHP) exposure, peracetic acid dry fogging (PAF), ultraviolet C irradiation (UVCI) and moist heat (MH) treatment to decontaminate a variety of different N95 masks following experimental contamination with SARS-CoV-2 or vesicular stomatitis virus as a surrogate. In addition, we sought to determine whether masks would tolerate repeated cycles of decontamination while maintaining structural and functional integrity. All methods except for UVCI were effective in total elimination of viable virus from treated masks. We found that all respirator masks tolerated at least one cycle of all treatment modalities without structural or functional deterioration as assessed by fit testing; filtration efficiency testing results were mostly similar except that a single cycle of LT-HPGP was associated with failures in 3 of 6 masks assessed. VHP, PAF, UVCI, and MH were associated with preserved mask integrity to a minimum of 10 cycles by both fit and filtration testing. A similar result was shown with ethylene oxide gassing to the maximum 3 cycles tested. Pleated, layered non-woven fabric N95 masks retained integrity in fit testing for at least 10 cycles of autoclaving but the molded N95 masks failed after 1 cycle; filtration testing however was intact to 5 cycles for all masks. The successful application of autoclaving for layered, pleated masks may be of particular use to institutions globally due to the virtually universal accessibility of autoclaves in health care settings. Given the ability to modify widely available heating cabinets on hospital wards in well-resourced settings, the application of moist heat may allow local processing of N95 masks.

Published

2020

33. Inactivation ofZaire ebolavirusVariant Makona in Human Serum Samples Analyzed by Enzyme-Linked Immunosorbent Assay

Author

Todd Cutts, Xiangguo Qiu, Allen Grolla, Steven Theriault, Shane Jones, and Bradley W. M. Cook

Subjects

0301 basic medicine, Zaire ebolavirus, Hot Temperature, 030106 microbiology, Enzyme-Linked Immunosorbent Assay, Antibodies, Viral, medicine.disease_cause, Immunoglobulin G, Virus, Disease Outbreaks, 03 medical and health sciences, Chlorocebus aethiops, medicine, Animals, Humans, Immunology and Allergy, Antigens, Viral, Vero Cells, Ebola virus, biology, Infectious dose, Outbreak, Hemorrhagic Fever, Ebola, Ebolavirus, Virology, Africa, Western, Titer, 030104 developmental biology, Infectious Diseases, Immunoglobulin M, Democratic Republic of the Congo, biology.protein, Virus Inactivation

Abstract

Personnel deployed to remote areas during infectious disease outbreaks have limited access to mechanical and chemical inactivation resources. The inactivation of infectious agents present in diagnostic samples is critical to ensure the safety of personnel and the containment of the disease. We evaluated the efficacy of thermal inactivation (exposure to 56°C for 1 hour) and chemical inactivation with 0.5% Tween-20 against a high titer of Ebola virus (species Zaire ebolavirus) variant Makona in spiked human serum samples. No surviving virus was revealed by a 50% tissue culture infective dose assay after the combined treatment under laboratory conditions. In-field use of this inactivation protocol during the 2013-2016 West Africa Ebola outbreaks demonstrated readily detectable levels of immunoglobulin G and/or immunoglobulin M in human plasma samples after treatment.

Published

2016

34. Development of a subgenomic clone system for Kyasanur Forest disease virus

Author

Darwyn Kobasa, Steven Theriault, Deborah A. Court, Bradley W. M. Cook, Todd Cutts, and Aidan M. Nikiforuk

Subjects

0301 basic medicine, medicine.medical_specialty, Hemorrhagic Fevers, Viral, Clone (cell biology), Genome, Viral, Disease, Virus Replication, Antiviral Agents, Microbiology, Genome, Encephalitis Viruses, Tick-Borne, 03 medical and health sciences, Genes, Reporter, Molecular genetics, medicine, Luciferases, Subgenomic mRNA, Genetics, biology, Transmission (medicine), Flavivirus, biology.organism_classification, medicine.disease, Virology, High-Throughput Screening Assays, 030104 developmental biology, Infectious Diseases, Insect Science, Replicon, Parasitology, Kyasanur forest disease

Abstract

Emerging tropical viruses pose an increasing threat to public health because social, economic and environmental factors such as global trade and deforestation allow for their migration into previously unexposed populations and ecological niches. Among such viruses, Kyasanur Forest disease virus (KFDV) deserves particular recognition because it causes hemorrhagic fever. This work describes the completion of an antiviral testing platform (subgenomic system) for KFDV that could be used to quickly and safely screen compounds capable of inhibiting KFDV replication without the requirement for high containment, as the structural genes have been replaced with a luciferase reporter gene precluding the generation of infectious particles. The coordination of KFDV kinetics with the replication characteristics of the subgenomic system has provided additional insight into the timing of flavivirus replication events, as the genetically engineered KFDV genome began replication as early as 2 h post cellular entry. Possession of such antiviral testing platforms by public health agencies should accelerate the testing of antiviral drugs against emerging or recently emerged viruses mitigating the effects of their disease and transmission.

Published

2016

35. Development and Characterization of a Guinea Pig-Adapted Sudan Virus

Author

Todd Cutts, Jill Graham, Jonathan Audet, Andrea Kroeker, Anders Leung, Gary P. Kobinger, Gary Wong, Carissa Embury-Hyatt, Xiangguo Qiu, Darwyn Kobasa, Haiyan Wei, and Shihua He

Subjects

0301 basic medicine, Guinea Pigs, Immunology, Adaptation, Biological, Spleen, Viremia, Biology, medicine.disease_cause, Microbiology, Median lethal dose, Virus, Lethal Dose 50, 03 medical and health sciences, Virology, medicine, Animals, Ebolavirus, Ebola virus, Lethal dose, Outbreak, Hemorrhagic Fever, Ebola, medicine.disease, Survival Analysis, Disease Models, Animal, 030104 developmental biology, medicine.anatomical_structure, Liver, Insect Science, Pathogenesis and Immunity

Abstract

Infections with Sudan virus (SUDV), a member of the genus Ebolavirus , result in a severe hemorrhagic fever with a fatal outcome in over 50% of human cases. The paucity of prophylactics and therapeutics against SUDV is attributed to the lack of a small-animal model to screen promising compounds. By repeatedly passaging SUDV within the livers and spleens of guinea pigs in vivo , a guinea pig-adapted SUDV variant (SUDV-GA) uniformly lethal to these animals, with a 50% lethal dose (LD 50 ) of 5.3 × 10 −2 50% tissue culture infective doses (TCID 50 ), was developed. Animals infected with SUDV-GA developed high viremia and died between 9 and 14 days postinfection. Several hallmarks of SUDV infection, including lymphadenopathy, increased liver enzyme activities, and coagulation abnormalities, were observed. Virological analyses and gross pathology, histopathology, and immunohistochemistry findings indicate that SUDV-GA replicates in the livers and spleens of infected animals similarly to SUDV infections in nonhuman primates. These developments will accelerate the development of specific medical countermeasures in preparation for a future disease outbreak due to SUDV. IMPORTANCE A disease outbreak due to Ebola virus (EBOV), suspected to have emerged during December 2013 in Guinea, with over 11,000 dead and 28,000 infected, is finally winding down. Experimental EBOV vaccines and treatments were administered to patients under compassionate circumstances with promising results, and availability of an approved countermeasure appears to be close. However, the same range of experimental candidates against a potential disease outbreak caused by other members of the genus Ebolavirus , such as Sudan virus (SUDV), is not readily available. One bottleneck contributing to this situation is the lack of a small-animal model to screen promising drugs in an efficient and economical manner. To address this, we have generated a SUDV variant (SUDV-GA) that is uniformly lethal to guinea pigs. Animals infected with SUDV-GA develop disease similar to that of SUDV-infected humans and monkeys. We believe that this model will significantly accelerate the development of life-saving measures against SUDV infections.

Published

2016

36. Intensive Supportive Care Alone Does Not Impact Survival in a Lethal Non-Human Primate Model of Ebola Virus Disease

Author

Alexander Bello, Charlene Ranadheera, Heinz Feldmann, Geoff Soule, Yvon Deschambault, Jason Gren, Jocelyn Edmonds, Trina Racine, Sam Aminian, Anders Leung, Amrinder Dhaliwal, Kevin Tierney, Xiangguo Qiu, Sharron Hadder, Hugues Fausther Bovendo, Mia J. Biondi, Robert A. Kozak, Stephanie Kucas, James E. Strong, Allen Grolla, Darwyn Kobasa, Steven Theriault, Cory Nakamura, Christy Press, Jarrid McKitrick, George F. Risi, Lauren Rondeau, Derek R. Stein, Mable Hagan, Bradley W. M. Cook, Anand Kumar, Darryl Schantz, Reeni Soni, Murray Kesselman, James Kenny, Todd Mortimer, Shane Jones, D Safronetz, B.J. Hancock, Christine DeGraff, Kaylie Tran, Ray Saurette, Darryl Falzarano, Duane J. Funk, Gary P. Kobinger, Mark F. Allan, Todd Cutts, Guillaume Poliquin, and Gregory Hansen

Subjects

Fluid administration, Resuscitation, medicine.medical_specialty, Non human primate, Ebola virus, Blood transfusion, business.industry, medicine.medical_treatment, Clinical course, Conflict of interest, Disease, medicine.disease_cause, medicine, Intensive care medicine, business

Abstract

Introduction: There are currently no licensed treatments for Ebola Virus Disease, making supportive care the only viable option. While there is anecdotal evidence that this is effective, the paucity of experimental data to demonstrate the role of supportive care in EVD has limited its use. We hypothesized that supportive care would enhance survival in a non-human primate (NHP) model of EVD. Methods: Three NHPs were infected with Ebola virus strain Makona and provided continuous bedside supportive care, including ventilatory support, fluid resuscitation, vasoactive medications, blood transfusion and hydrocortisone as needed to treat cardiovascular compromise. Findings: All three NHPs developed EVD and demonstrated a very similar clinical course and ultimately reached a terminal endpoint at an average time of 160 ± 8·7 hours post infection, which is similar to caged animals (144-192 hours). Fluid administration may have temporarily blunted a rise in lactate but the effect was short lived. Vasoactive medications, blood transfusion and hydrocortisone did not appear to have an impact. Interpretation: Supportive care did not impact survival length in a high stringency NHP EVD disease model. Our findings help support the need for the development and use of specific anti-Ebola therapies. Funding Statement: Funding was provided by the Canadian Institutes of Health Research and the Government of Canada. Declaration of Interests: None of the authors had a conflict of interest with regard to this study. Ethics Approval Statement: The study protocol was reviewed and approved by the institutional Animal Care Committee, in accordance with Canadian Council on Animal Care (CCAC) guidelines.

Published

2018

37. Ebola Virus Transmission in Guinea Pigs

Author

Gary Wong, Brad Collignon, Xiangguo Qiu, Gary P. Kobinger, Todd Cutts, Carissa Embury-Hyatt, Jenna Aviles, Jason S. Richardson, and Jason Gren

Subjects

Guinea Pigs, Respiratory System, Immunology, Biology, medicine.disease_cause, Microbiology, Median lethal dose, Virus, Virology, Disease Transmission, Infectious, medicine, Animals, Viral shedding, Ebolavirus, Ebola virus, Transmission (medicine), Hemorrhagic Fever, Ebola, Survival Analysis, Virus Shedding, Mucosal Infection, Disease Models, Animal, medicine.anatomical_structure, Insect Science, Pathogenesis and Immunity, Respiratory tract

Abstract

Ebola virus (EBOV) transmission is currently poorly characterized and is thought to occur primarily by direct contact with infectious material; however transmission from swine to nonhuman primates via the respiratory tract has been documented. To establish an EBOV transmission model for performing studies with statistical significance, groups of six guinea pigs (gps) were challenged intranasally (i.n.) or intraperitoneally (i.p.) with 10,000 times the 50% lethal dose (LD 50 ) of gp-adapted EBOV, and naive gps were then introduced as cage mates for contact exposure at 1 day postinfection (p.i.). The animals were monitored for survival and clinical signs of disease and quantitated for virus shedding postexposure. Changes in the duration of contact of naive gps with infected animals were evaluated for their impact on transmission efficiency. Transmission was more efficient from i.n.- than from i.p.-challenged gps, with 17% versus 83% of naive gps surviving exposure, respectively. Virus shedding was detected beginning at 3 days p.i. from both i.n.- and i.p.-challenged animals. Contact duration positively correlated with transmission efficiency, and the abrogation of direct contact between infected and naive animals through the erection of a steel mesh was effective at stopping virus spread, provided that infectious animal bedding was absent from the cages. Histopathological and immunohistochemical findings show that i.n.-infected gps display enhanced lung pathology and EBOV antigen in the trachea, which supports increased virus transmission from these animals. The results suggest that i.n.-challenged gps are more infectious to naive animals than their systemically infected counterparts and that transmission occurs through direct contact with infectious materials, including those transported through air movement over short distances. IMPORTANCE Ebola is generally thought to be spread between humans though infectious bodily fluids. However, a study has shown that Ebola can be spread from pigs to monkeys without direct contact. Further studies have been hampered, because an economical animal model for Ebola transmission is not available. To address this, we established a transmission model in guinea pigs and determined the mechanisms behind virus spread. The survival data, in addition to microscopic examination of lung and trachea sections, show that mucosal infection of guinea pigs is an efficient model for Ebola transmission. Virus spread is increased with longer contact times with an infected animal and is possible without direct contact between an infected and a naive host but can be stopped if infectious materials are absent. These results warrant consideration for the development of future strategies against Ebola transmission and for a better understanding of the parameters involved in virus spread.

Published

2015

38. Inactivating Zaire Ebolavirus in Whole-Blood Thin Smears Used for Malaria Diagnosis

Author

James E. Strong, Steven Theriault, P. Guillaume Poliquin, Bradley W. M. Cook, and Todd Cutts

Subjects

0301 basic medicine, Microbiology (medical), Ebolavirus, Disinfection methods, Zaire ebolavirus, Biology, medicine.disease_cause, medicine.disease, Virology, Virus, 03 medical and health sciences, 030104 developmental biology, parasitic diseases, medicine, Coinfection, Malaria, Whole blood

Abstract

Malaria is an important mimic or coinfection in potential Ebolavirus disease patients. Here, we evaluated the efficacy of the 100% methanol-inactivating Zaire Ebolavirus Makona variant for malaria thin-smear preparation. We determined that 100% methanol completely inactivated the virus after 15 min.

Published

2016

39. Deep-sequencing of Marburg virus genome during sequential mouse passaging and cell-culture adaptation reveals extensive changes over time

Author

Bianli Xu, Xiangguo Qiu, Jonathan Audet, Todd Cutts, Xueyong Huang, Haiyan Wei, Shihua He, Gary P. Kobinger, Gary Wong, and Steven Theriault

Subjects

0301 basic medicine, Science, Adaptation, Biological, Genome, Viral, Biology, Genome, Article, Deep sequencing, Virus, Marburg virus, Mice, Viral Proteins, 03 medical and health sciences, Intergenic region, VP40, Animals, Marburg Virus Disease, Serial Passage, Cells, Cultured, Genetics, Multidisciplinary, High-Throughput Nucleotide Sequencing, Outbreak, Viral Load, Virology, 030104 developmental biology, Marburgvirus, Viral evolution, Medicine, RNA, Viral

Abstract

Marburg virus (MARV) has caused outbreaks of filoviral hemorrhagic fever since its discovery in 1967. The largest and deadliest outbreak occurred in Angola in 2005, with 252 cases and 227 deaths. In 2014, we developed a mouse-adapted MARV, Angola variant through serial passaging in mice. The mouse-adapted MARV exhibits many of the hallmarks of MARV disease in humans. By applying deep-sequencing to every passage of the virus, we are able to study virus evolution in this host with surprising precision. We show that two regions go through substantial changes: the intergenic region between NP and VP35, as well as the first 100 amino acids of the VP40 protein. Our results also reveal that there were profound changes during the production of the final virus stock in cell culture. Overall, our results show that a handful of regions carry most of the mutations acquired during the adaptation of the virus to a new host and that many mutations become fixed very early during the adaptation process.

Published

2017

40. Challenge of Liquid Stressed Protective Materials and Environmental Persistence of Ebola Virus

Author

Todd Cutts, Bradley W. M. Cook, Steven Theriault, and Aidan M. Nikiforuk

Subjects

0301 basic medicine, Zaire ebolavirus, Veterinary medicine, Science, viruses, Climate, Environment, medicine.disease_cause, Virus, Article, West africa, Disease Outbreaks, 03 medical and health sciences, 0302 clinical medicine, medicine, Humans, 030212 general & internal medicine, Personal protective equipment, Personal Protective Equipment, Infectious virus, Ebolavirus, Multidisciplinary, Ebola virus, business.industry, Outbreak, Hemorrhagic Fever, Ebola, Virology, 3. Good health, Africa, Western, 030104 developmental biology, Medicine, business

Abstract

After the largest Ebola virus outbreak in history, experts have attempted to answer how the Zaire ebolavirus species emerged in West Africa and caused chains of human-to-human transmission. The widespread and untimely infection of Health Care Workers (HCW) in the affected countries accelerated spread of the virus within the community. Among the reasons attributed to this trend, it must be considered that HCW were exposed to the virus in their occupational environment. The contribution of environmental conditions to the spread of Ebola in West Africa was examined by investigating the effect of temperature/humidity on the virus’s environmental persistence and by modeling if saturation (liquid stress) allows for penetration of Ebola virus through personal protective equipment (PPE). Ebola-Makona virus persisted on PPE and materials found in outbreak settings for less than 72 hours at 27 °C and 80% relative humidity (RH). A difference in virus penetration was observed between dry (5%, 1/21 tests) and saturated (33%, 7/21 tests) samples of PPE. Infectious virus particles penetrated through saturated coupons of Tyvek Micro Clean, Tychem QC, whole surgical masks and N95 respirators. These findings suggest inclusion of saturation or similar liquid stress simulation in protective equipment testing standards.

Published

2017

41. Establishment and Characterization of a Lethal Mouse Model for the Angola Strain of Marburg Virus

Author

Gary Wong, Todd Cutts, Xiangguo Qiu, Stephanie A. Booth, Jonathan Audet, Gary P. Kobinger, and Yulian Niu

Subjects

Molecular Sequence Data, Immunology, Adaptation, Biological, Filoviridae, Viremia, Mice, SCID, medicine.disease_cause, Microbiology, Median lethal dose, Virus, Lethal Dose 50, Marburg virus, Serial passage, Virology, Filoviridae Infections, medicine, Animals, Serial Passage, Mice, Inbred BALB C, Ebola virus, biology, Sequence Analysis, DNA, Viral Load, biology.organism_classification, medicine.disease, Survival Analysis, Mice, Inbred C57BL, Disease Models, Animal, Blood, Liver, Insect Science, Pathogenesis and Immunity, RNA, Viral, Viral load

Abstract

Infections with Marburg virus (MARV) and Ebola virus (EBOV) cause severe hemorrhagic fever in humans and nonhuman primates (NHPs) with fatality rates up to 90%. A number of experimental vaccine and treatment platforms have previously been shown to be protective against EBOV infection. However, the rate of development for prophylactics and therapeutics against MARV has been lower in comparison, possibly because a small-animal model is not widely available. Here we report the development of a mouse model for studying the pathogenesis of MARV Angola (MARV/Ang), the most virulent strain of MARV. Infection with the wild-type virus does not cause disease in mice, but the adapted virus (MARV/Ang-MA) recovered from liver homogenates after 24 serial passages in severe combined immunodeficient (SCID) mice caused severe disease when administered intranasally (i.n.) or intraperitoneally (i.p.). The median lethal dose (LD 50 ) was determined to be 0.015 50% TCID 50 (tissue culture infective dose) of MARV/Ang-MA in SCID mice, and i.p. infection at a dose of 1,000× LD 50 resulted in death between 6 and 8 days postinfection in SCID mice. Similar results were obtained with immunocompetent BALB/c and C57BL/6 mice challenged i.p. with 2,000× LD 50 of MARV/Ang-MA. Virological and pathological analyses of MARV/Ang-MA-infected BALB/c mice revealed that the associated pathology was reminiscent of observations made in NHPs with MARV/Ang. MARV/Ang-MA-infected mice showed most of the clinical hallmarks observed with Marburg hemorrhagic fever, including lymphopenia, thrombocytopenia, marked liver damage, and uncontrolled viremia. Virus titers reached 10 8 TCID 50 /ml in the blood and between 10 6 and 10 10 TCID 50 /g tissue in the intestines, kidney, lungs, brain, spleen, and liver. This model provides an important tool to screen candidate vaccines and therapeutics against MARV infections. IMPORTANCE The Angola strain of Marburg virus (MARV/Ang) was responsible for the largest outbreak ever documented for Marburg viruses. With a 90% fatality rate, it is similar to Ebola virus, which makes it one of the most lethal viruses known to humans. There are currently no approved interventions for Marburg virus, in part because a small-animal model that is vulnerable to MARV/Ang infection is not available to screen and test potential vaccines and therapeutics in a quick and economical manner. To address this need, we have adapted MARV/Ang so that it causes illness in mice resulting in death. The signs of disease in these mice are reminiscent of wild-type MARV/Ang infections in humans and nonhuman primates. We believe that this will be of help in accelerating the development of life-saving measures against Marburg virus infections.

Published

2014

42. The Disinfection Characteristics of Ebola Virus Outbreak Variants

Author

Anders Leung, Todd Cutts, Aidan M. Nikiforuk, Darwyn Kobasa, Steven Theriault, and Bradley W. M. Cook

Subjects

0301 basic medicine, Zaire ebolavirus, Sodium Hypochlorite, Contact time, viruses, 030106 microbiology, Microbial Sensitivity Tests, Biology, medicine.disease_cause, Article, Disease Outbreaks, 03 medical and health sciences, chemistry.chemical_compound, medicine, Humans, Infection control, Infectious virus, Infectivity, Multidisciplinary, Ebola virus, Ethanol, Virion, Outbreak, Hemorrhagic Fever, Ebola, Ebolavirus, Virology, 3. Good health, Disinfection, Africa, Western, chemistry, Sodium hypochlorite, RNA, Viral, Disinfectants

Abstract

The recent Ebola virus outbreak in West Africa has forced experts to re-evaluate their understanding of how to best disinfect areas contaminated with infectious bodily fluids. Recent research has found that Ebola virus remains viable in blood for 7–10 days making appropriate disinfection crucial to infection control. We sought to determine if the three most important outbreak variants of Zaire ebolavirus (Mayinga, Kikwit and Makona) exhibit separate phenotypes when challenged with a range of sodium hypochlorite (NaOCl) concentrations or 70% ethanol (EtOH) at average West African temperature. The time dependent killing of Ebola virus was evaluated by measuring infectious virus and viral RNA (vRNA), to determine if RNA detection is a viable method for decontamination measurement in areas without high containment laboratory access. Makona was less susceptible to weaker concentrations of NaOCl (0.05 and 0.1%) than Mayinga and Kikwit. At the recommended concentration of NaOCl (≥0.5%) all of the variants were inert after 5 minutes of contact time. Similarly, all variants were inactivated by 70% EtOH after 2.5 minutes, only Makona was detected at 1 minute. In multiple instances, high amounts of vRNA was detected in the absence of infectious virus, suggesting that it does not serve as an accurate measure of remaining infectivity after cleansing.

Published

2016

43. Reduction of Neuraminidase Activity Exacerbates Disease in 2009 Pandemic Influenza Virus-Infected Mice

Author

Anders Leung, Brad Collignon, Todd Cutts, Steven Theriault, Carissa Embury-Hyatt, Mable Hagan, Darwyn Kobasa, and Charlene Ranadheera

Subjects

0301 basic medicine, Oseltamivir, Exacerbation, Swine, viruses, Immunology, Hemagglutinin (influenza), Virulence, Neuraminidase, Biology, medicine.disease_cause, Virus Replication, Microbiology, Antiviral Agents, Virus, Cell Line, Madin Darby Canine Kidney Cells, 03 medical and health sciences, chemistry.chemical_compound, Mice, Viral Proteins, Dogs, Influenza A Virus, H1N1 Subtype, Orthomyxoviridae Infections, Virology, Vaccines and Antiviral Agents, Influenza A virus, medicine, Viral neuraminidase, Animals, Enzyme Inhibitors, Pandemics, Mice, Inbred BALB C, Ferrets, virus diseases, Disease Models, Animal, 030104 developmental biology, chemistry, Insect Science, biology.protein, Female

Abstract

During the first wave of the 2009 pandemic, caused by a H1N1 influenza virus (pH1N1) of swine origin, antivirals were the only form of therapeutic available to control the proliferation of disease until the conventional strain-matched vaccine was produced. Oseltamivir is an antiviral that inhibits the sialidase activity of the viral neuraminidase (NA) protein and was shown to be effective against pH1N1 viruses in ferrets. Furthermore, it was used in humans to treat infections during the pandemic and is still used for current infections without reported complication or exacerbation of illness. However, in an evaluation of the effectiveness of oseltamivir against pH1N1 infection, we unexpectedly observed an exacerbation of disease in virus-infected mice treated with oseltamivir, transforming an otherwise mild illness into one with high morbidity and mortality. In contrast, an identical treatment regime alleviated all signs of illness in mice infected with the pathogenic mouse-adapted virus A/WSN/33 (H1N1). The worsened clinical outcome with pH1N1 viruses occurred over a range of oseltamivir doses and treatment schedules and was directly linked to a reduction in NA enzymatic activity. Our results suggest that the suppression of NA activity with antivirals may exacerbate disease in a host-dependent manner by increasing replicative fitness in viruses that are not optimally adapted for replication in that host. IMPORTANCE Here, we report that treatment of pH1N1-infected mice with oseltamivir enhanced disease progression, transforming a mild illness into a lethal infection. This raises a potential pitfall of using the mouse model for evaluation of the therapeutic efficacy of neuraminidase inhibitors. We show that antiviral efficacy determined in a single animal species may not represent treatment in humans and that caution should be used when interpreting the outcome. Furthermore, increased virulence due to oseltamivir treatment was the effect of a shift in the hemagglutinin (HA) and neuraminidase (NA) activity balance. This is the first study that has demonstrated that altering the HA/NA activity balance by reduction in NA activity can result in an increase in virulence in any animal model from nonpathogenic to lethal and the first to demonstrate a situation in which treatment with a NA activity inhibitor has an effect opposite to the intended therapeutic effect of ameliorating the infection.

Published

2016

44. Limited Effects of Type I Interferons on Kyasanur Forest Disease Virus in Cell Culture

Author

Charlene Ranadheera, Bradley W. M. Cook, Todd Cutts, Steven Theriault, Deborah A. Court, Aidan M. Nikiforuk, and Darwyn Kobasa

Subjects

RNA viruses, 0301 basic medicine, Cytotoxicity, Dengue virus, Pathology and Laboratory Medicine, Toxicology, medicine.disease_cause, Biochemistry, Cricetinae, Chlorocebus aethiops, Medicine and Health Sciences, biology, Immunogenicity, lcsh:Public aspects of medicine, Flavivirus, Infectious Diseases, Vesicular Stomatitis Virus, Medical Microbiology, Vesicular stomatitis virus, Viral Pathogens, Viruses, Interferon Type I, Biological Cultures, Pathogens, Research Article, lcsh:Arctic medicine. Tropical medicine, lcsh:RC955-962, Research and Analysis Methods, Microbiology, Antiviral Agents, Rhabdoviruses, Vesicular stomatitis Indiana virus, Encephalitis Viruses, Tick-Borne, 03 medical and health sciences, Virology, medicine, Animals, Humans, Microbial Pathogens, Vero Cells, Flaviviruses, Organisms, Public Health, Environmental and Occupational Health, Biology and Life Sciences, Proteins, Outbreak, lcsh:RA1-1270, Cell Cultures, Dengue Virus, biology.organism_classification, medicine.disease, Viral Replication, Kyasanur Forest Disease, 030104 developmental biology, Viral replication, A549 Cells, Cell culture, Immunology, Interferons, Japanese Encephalitis Virus, Kyasanur forest disease

Abstract

Background The tick-borne flavivirus, Kyasanur Forest disease virus (KFDV) causes seasonal infections and periodic outbreaks in south-west India. The current vaccine offers poor protection with reported issues of coverage and immunogenicity. Since there are no approved prophylactic therapeutics for KFDV, type I IFN-α/β subtypes were assessed for antiviral potency against KFDV in cell culture. Methodology/Principal Findings The continued passage of KFDV-infected cells with re-administered IFN-α2a treatment did not eliminate KFDV and had little effect on infectious particle production whereas the IFN-sensitive, green fluorescent protein-expressing vesicular stomatitis virus (VSV-GFP) infection was controlled. Further evaluation of the other IFN-α/β subtypes versus KFDV infection indicated that single treatments of either IFN-αWA and IFN-αΚ appeared to be more effective than IFN-α2a at reducing KFDV titres. Concentration-dependent analysis of these IFN-α/β subtypes revealed that regardless of subtype, low concentrations of IFN were able to limit cytopathic effects (CPE), while significantly higher concentrations were needed for inhibition of virion release. Furthermore, expression of the KFDV NS5 in cell culture before IFN addition enabled VSV-GFP to overcome the effects of IFN-α/β signalling, producing a robust infection. Conclusions/Significance Treatment of cell culture with IFN does not appear to be suitable for KFDV eradication and the assay used for such studies should be carefully considered. Further, it appears that the NS5 protein is sufficient to permit KFDV to bypass the antiviral properties of IFN. We suggest that other prophylactic therapeutics should be evaluated in place of IFN for treatment of individuals with KFDV disease., Author Summary Since 1957 Kyasanur Forest disease virus (KFDV) has caused seasonal infections and periodic outbreaks in south-west India. It is estimated that nearly 500 people acquire KFDV annually and 3–5% of those infected succumb to the disease. The vaccine strategy is complicated by the lack of coverage, compliance and efficacy, highlighted by the fact that less than half of the target population received the recommended three dose-regimen. Besides the prevention of tick bites and vaccination, there are no approved antivirals for KFDV infection. Based on these observations, the commonly-used-IFN-α2a was assessed and was not capable of limiting KFDV virus titres. Further characterization of the other IFN-α/β subtypes used at different concentrations revealed that KFDV replication was insensitive to all subtypes, even though signs of cellular damage were reduced. Thus, infectious titre, rather than monolayer staining or cytopathic effect (CPE) monitoring, is more reliable for IFN analyses. The capability of KFDV to overcome the antiviral properties of IFN was attributed to the NS5 protein. Thus, other treatment options need to be evaluated for patients suffering with Kyasanur Forest disease.

Published

2016

45. Comparative Inactivation Studies ofListeria Monocytogenesat Room and Refrigeration Temperatures

Author

Bree-Ann A. Carruthers, Steven Theriault, Todd Cutts, and Christy-Lynn Cross

Subjects

Health, Toxicology and Mutagenesis, Disinfectant, digestive, oral, and skin physiology, Public Health, Environmental and Occupational Health, food and beverages, Refrigeration, Outbreak, Human decontamination, Management, Monitoring, Policy and Law, Biology, medicine.disease_cause, Microbiology, Listeria monocytogenes, medicine, Refrigeration temperature, Pathogen, Biotechnology

Abstract

Listeria monocytogenes is an important food-borne pathogen which has been associated with disease outbreaks from contaminated ready-to-eat meat products due to the improper decontamination of the e...

Published

2012

46. A Study of the Effectiveness of the Containment Level-4 (CL-4) Chemical Shower in Decontaminating Dover Positive-Pressure Suits

Author

Todd Cutts, Steven Theriault, Natasha Klaponski, and Diane Gordon

Subjects

Engineering, Shower, Containment, Waste management, business.industry, Health, Toxicology and Mutagenesis, Public Health, Environmental and Occupational Health, Environmental engineering, Human decontamination, Management, Monitoring, Policy and Law, business, Personal protective equipment, Biotechnology

Abstract

Objectives: The decontamination or physical removal of contaminants from personal protective equipment upon exit from high containment laboratories is crucial to maintain containment and safety of ...

Published

2011

47. The interaction between thymine DNA glycosylase and nuclear receptor coactivator 3 is required for the transcriptional activation of nuclear hormone receptors

Author

Alina Radziwon, Shirley Chiang, Tanya Burch, Runtao He, Todd Cutts, Xuguang Li, Craig Brusnyk, Gary Van Domselaar, Jessica Piper, Megan R. Edwards, Jingxin Cao, and Kevin Dick

Subjects

Transcriptional Activation, medicine.medical_treatment, Amino Acid Motifs, Clinical Biochemistry, Receptors, Cytoplasmic and Nuclear, Estrogen receptor, Biology, Nuclear Receptor Coactivator 3, Cell Line, Tumor, Two-Hybrid System Techniques, Protein Interaction Mapping, medicine, Humans, Receptor, Molecular Biology, Cell Biology, General Medicine, Thymine DNA Glycosylase, Nuclear receptor coactivator 1, Steroid hormone, Nuclear receptor, Biochemistry, Nuclear receptor coactivator 3, Mutagenesis, Site-Directed, Nuclear receptor coactivator 2, Thymine-DNA glycosylase

Abstract

The T:G mismatch specific DNA glycosylase (TDG) is known as an important enzyme in repairing damaged DNA. Recent studies also showed that TDG interacts with a p160 protein, steroid receptor coactivator 1 or nuclear receptor coactivator 1 (SRC1), and is involved in transcriptional activation of the estrogen receptor. However, whether other members of the p160 family are also involved in TDG-interaction and signal transduction regulation remains to be seen. In this study, we employed the mammalian two-hybrid system to investigate the interaction between TDG and another member of the p160 family, nuclear receptor coactivator 3 (NCoA-3). We found that a DXXD motif from aa 294-297 within TDG was responsible for the TDG-NCoA-3 interaction, we also found that a LLXXXL motif (X means any amino acid) from aa 1029-1037 (LLRNSL) and a merged LLXXL motif (LLDQLHTLL) from aa 1053-1061 in NCoA-3 were important for the TDG-NCoA-3 interactions. Mutation of the two aspartic acids (aa 294 and 297) into two alanines in TDG significantly affected the interaction and subsequent transcriptional activation of several steroid hormone receptors including, estrogen-, androgen- and progesterone- receptors in Huh7 cells. We also identified that mutations of NCoA-3 at either leucines 1029-1030 or 1053-1054 (replaced by alanines) also reduced the interaction activity between TDG and NCoA1. These data indicated that the TDG-NCoA-3 interaction is important for broad range activation of steroid hormone nuclear receptors, and may also contribute significantly to further understanding of TDG-related nuclear receptor regulation.

Published

2009

48. Influenza virus emitted by naturally-infected hosts in a healthcare setting

Author

Andrea Granados, Jonathan B. Gubbay, Adriana Peci, Samira Mubareka, Ilyse Darwish, James A. Scott, Todd Cutts, George Astrakianakis, and Ushma Naik

Subjects

Adult, Male, Middle East respiratory syndrome coronavirus, viruses, Air Microbiology, Pilot Projects, medicine.disease_cause, Virus, Article, Exposure, Virology, Influenza, Human, Influenza A virus, Medicine, Humans, Transmission, Viral rna, Community Health Services, Aged, Bioaerosol, Aged, 80 and over, business.industry, Transmission (medicine), Healthcare, Middle Aged, Influenza A virus subtype H5N1, Influenza B virus, Infectious Diseases, Influenza virus RNA, Female, business, Influenza virus

Abstract

Highlights • This pilot study examined the viral content of bioaerosols emitted by patients with laboratory-confirmed influenza. • Nine out of fifteen patients emitted variable amounts of viral RNA. • Patients with influenza may emit virus into the air which disperses >1 m and may reach the breathing zone of a healthcare worker., Background The emergence of novel respiratory viruses such as avian influenza A(H7N9) virus and the Middle East Respiratory Syndrome Coronavirus (MERS-CoV) highlights the importance of understanding determinants of transmission to healthcare workers (HCWs) and the public. Objectives We aim to determine the viral content of the air emitted by symptomatic inpatients or long-term care residents with laboratory-confirmed influenza virus infection (emitters), and in the breathing zones of healthcare workers who attend to them. Design A prospective pilot study of patients with laboratory-confirmed influenza virus infection was undertaken. Air within 1 m of the patient was sampled using a high volume air sampler. In addition, a lower volume air sampler was placed 1 m from the patient. Viral RNA was recovered from the samplers and submitted for quantitative real time PCR. In addition, personal button samplers were provided to HCWs. Results The air emitted by 15 participants with laboratory-confirmed influenza virus infection was sampled. Of the patients infected with influenza A, viral RNA was recovered from the air emitted by 9/12 patients using the low-volume sampler; no viral RNA was detected from air emitted by patients with influenza B (n = 3). Influenza virus RNA was recovered from one HCW’s sampler. Conclusions Patients with respiratory virus infection emit virus into the air which disperses to >1 m and may reach the breathing zone of a HCW. This pilot study highlights the feasibility and importance of conducting a larger-scale study to identify determinants of exposure and transmission from patient to HCW.

Published

2015

49. Evaluating environmental persistence and disinfection of the Ebola virus Makona variant

Author

Philip Guillaume Poliquin, Steven Theriault, Bradley W. M. Cook, Deborah A. Court, Aidan M. Nikiforuk, James E. Strong, and Todd Cutts

Subjects

filovirus, Time Factors, Contact time, Sodium Hypochlorite, Molecular Sequence Data, lcsh:QR1-502, Biology, medicine.disease_cause, outbreak management, lcsh:Microbiology, Article, Persistence (computer science), Microbiology, chemistry.chemical_compound, Ebola virus, Makona, Virology, medicine, Environmental Microbiology, Food science, Disinfection methods, Ethanol, Microbial Viability, biosafety, Sequence Analysis, DNA, Ebolavirus, Disinfection, Infectious Diseases, chemistry, Sodium hypochlorite, environment, Disinfectants

Abstract

Background: The current disease outbreak caused by the Ebola virus Makona variant (EBOV/Mak) has led to unprecedented morbidity and lethality given its geographic reach and sustained transmission. Sodium hypochlorite and ethanol are well-accepted decontamination agents, however little published evidence supports the selection of appropriate concentrations and contact times. The present study addresses the environmental robustness of EBOV/Mak and evaluates the effectiveness of sodium hypochlorite and ethanol as disinfectants. Methods: EBOV/Mak was suspended in a simulated organic soil load and dried onto surfaces. Viability was measured at 1 hour, 24 hours, 72 hours, and 192 hours. For the evaluation of disinfectants, EBOV/Mak in a simulated organic soil was dried onto stainless steel carriers and disinfected with 0.01% (v/v), 0.1% (v/v), 0.5% (v/v) and 1% (v/v) sodium hypochlorite solutions or 67% (v/v) ethanol at contact times of 1, 5 or 10 minutes. Results: EBOV/Mak persisted longer on steel and plastic surfaces (192 hours) than cotton (&lt, 24 hours). Dilute sodium hypochlorite (0.01% and 0.1%) showed little antiviral action, whereas 0.5% and 1% sodium hypochlorite solutions demonstrated recoverable virus at one minute but sterilized surfaces in five minutes. Disinfection with 67% ethanol did not fully clear infectious virions from 3/9 carriers at 1 minute but sterilized all carriers at 5 and 10 minutes. Conclusions: Sodium hypochlorite and ethanol effectively decontaminate EBOV/Mak suspended in a simulated organic load, however, selection of concentration and contact time proves critical.

Published

2015

50. Potent and selective inhibition of SARS coronavirus replication by aurintricarboxylic acid

Author

Maya Traykova-Adonova, Todd Cutts, Yvon Deschambaul, Xuguang Li, Runtao He, Anton Adonov, Jody D. Berry, Elsie Grudesky, Jingxin Cao, and Michael Drebot

Subjects

Drug, viruses, media_common.quotation_subject, Biophysics, Biology, Selective inhibition, Severe Acute Respiratory Syndrome, Virus Replication, medicine.disease_cause, Coronavirus, SARS-CoV, Antiviral Agents, Sensitivity and Specificity, Biochemistry, Article, Microbiology, chemistry.chemical_compound, Chlorocebus aethiops, Aurintricarboxylic acid, medicine, Asian country, Animals, Vero Cells, Molecular Biology, Inhibition, media_common, Coronavirus, SARS, Dose-Response Relationship, Drug, Aurintricarboxylic Acid, fungi, Reproducibility of Results, Cell Biology, Virology, Dose–response relationship, Severe acute respiratory syndrome-related coronavirus, chemistry, Vero cell, Severe acute respiratory syndrome coronavirus, Cell Division

Abstract

The severe acute respiratory syndrome virus (SARS) is a coronavirus that instigated regional epidemics in Canada and several Asian countries in 2003. The newly identified SARS coronavirus (SARS-CoV) can be transmitted among humans and cause severe or even fatal illnesses. As preventive vaccine development takes years to complete and adverse reactions have been reported to some veterinary coronaviral vaccines, anti-viral compounds must be relentlessly pursued. In this study, we analyzed the effect of aurintricarboxylic acid (ATA) on SARS-CoV replication in cell culture, and found that ATA could drastically inhibit SARS-CoV replication, with viral production being 1000-fold less than that in the untreated control. Importantly, when compared with IFNs alpha and beta, viral production was inhibited by more than 1000-fold as compared with the untreated control. In addition, when compared with IFNs alpha and beta, ATA was approximately 10 times more potent than IFN alpha and 100 times more than interferon beta at their highest concentrations reported in the literature previously. Our data indicated that ATA should be considered as a candidate anti-SARS compound for future clinical evaluation.

Published

2004