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15 results on '"Rebecca Hickman"'

1. Rapid, High-Throughput, Cost Effective Whole Genome Sequencing of SARS-CoV-2 Using a Condensed One Hour Library Preparation of the Illumina DNA Prep Kit

Author

Rebecca Hickman, Jason Nguyen, Tracy D. Lee, John R. Tyson, Robert Azana, Frankie Tsang, Linda Hoang, and Natalie Prystajecky

Abstract

The ongoing COVID-19 pandemic necessitates cost-effective, high-throughput, and timely genomic sequencing of SARS-CoV-2 viruses for outbreak investigations, identifying variants of concern (VoC), characterizing vaccine breakthrough infections, and public health surveillance. Additionally, the enormous demand of genomic sequencing on supply chains and the resulting shortages of laboratory supplies necessitate the use of low-reagent and low-consumable methods. Here, we report an optimized library preparation method where the same protocol can be used in a STAT scenario, from sample to sequencer in as little as eight hours, and a high-throughput scenario, where one technologist can perform 576 library preparations over the course of one 8-hour shift. This new method uses Freed et al.’s 1200 bp primer sets (Biol Methods Protoc 5:bpaa014, 2020, https://doi.org/10.1093/biomethods/bpaa014) and a modified and truncated Illumina DNA Prep workflow (Illumina, CA, USA). Compared to the original, application of this new method in hundreds of clinical specimens demonstrated equivalent results to the full-length DNA Prep workflow at 45% the cost, 15% of consumables required (such as pipet tips), 25% of manual hands-on time, and 15% of on-instrument time if performing on a liquid handler, with no compromise in sequence quality. Results suggest that this new method is a rapid, simple, cost-effective, and high-quality SARS-CoV-2 whole genome sequencing protocol.

Published
2022

2. Generating 1200bp tiled Amplicons for SARS-CoV2 Whole Genome Sequencing v2

Author

jason.nguyen not provided, Tracy Lee, Rebecca Hickman, Natalie Prystajecky, and John Tyson

Abstract

This procedure provides instructions for how to generate amplicons across the entire SARS-CoV-2 genome to be used for downstream whole genome sequencing applications, including Illumina MiSeq/NextSeq or Oxford Nanopore MinION sequencing platforms. The steps involved in this protocol were derived from version 3 of Freed et al protocol nCoV-2019 sequencing protocol (RAPID barcoding, 1200bp amplicon)V.3 available at https://dx.doi.org/10.17504/protocols.io.bgggjttw

Published
2022

3. Rapid, high throughput library preparation of SARS-CoV2 using Illumina’s DNA Prep Library Preparation Kit v3

Author

Jason Nguyen, Rebecca Hickman, Tracy Lee, Natalie Prystajecky, and John Tyson

Abstract

This procedure provides instructions on how to prepare DNA libraries for whole genome sequencing on an Illumina MiSeq or NextSeq using Illumina’s DNA Prep Library Preparation Kit scaled to half reaction volumes with modifications to the post-PCR procedures; tagmentation stop buffer and associated washes are removed and libraries are pooled post PCR then a single size selection is performed. This protocol is used to sequence SARS-CoV-2 using the cDNA/PCR protocol: https://dx.doi.org/10.17504/protocols.io.b3viqn4e

Published
2022

4. Rapid, high throughput library preparation of SARS-CoV2 using Illumina’s DNA Prep Library Preparation Kit v2

Author

Jason Nguyen, Rebecca Hickman, Tracy Lee, Natalie Prystajecky, and John Tyson

Abstract

This procedure provides instructions on how to prepare DNA libraries for whole genome sequencing on an Illumina MiSeq or NextSeq using Illumina’s DNA Prep Library Preparation Kit scaled to half reaction volumes with modifications to the post-PCR procedures; tagmentation stop buffer and associated washes are removed and libraries are pooled post PCR then a single size selection is performed.

Published
2022

5. Mutations in emerging variant of concern lineages disrupt genomic sequencing of SARS-CoV-2 clinical specimens

Author

Jason Nguyen, Linda Hoang, Natalie Prystajecky, Tracy D. Lee, Kevin S. Kuchinski, John R. Tyson, Agatha N. Jassem, and Rebecca Hickman

Subjects
viral genomics, Microbiology (medical), 2019-20 coronavirus outbreak, Lineage (genetic), Coronavirus disease 2019 (COVID-19), Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Infectious and parasitic diseases, RC109-216, Computational biology, Genome, Viral, Biology, Genome, Article, 03 medical and health sciences, 0302 clinical medicine, Humans, 030304 developmental biology, 0303 health sciences, Laboratory methods, amplicon sequencing, British Columbia, SARS-CoV-2, Genomic sequencing, COVID-19, General Medicine, Genomics, 3. Good health, genomic surveillance, Infectious Diseases, Mutation, Amplicon sequencing, variant of concern, 030217 neurology & neurosurgery
Abstract

Mutations in emerging severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) lineages can interfere with laboratory methods used to generate viral genome sequences for public health surveillance. We identified 20 mutations that are widespread in variant of concern lineages and affect widely used sequencing protocols by the ARTIC network and Freed et al. Three of these mutations disrupted sequencing of P.1 lineage specimens during a recent outbreak in British Columbia, Canada. We provide laboratory validation of protocol modifications that restored sequencing performance. The study findings indicate that genomic sequencing protocols require immediate updating to address emerging mutations. This work also suggests that routine monitoring and protocol updates will be necessary as SARS-CoV-2 continues to evolve. The bioinformatic and laboratory approaches used here provide guidance for this kind of assay maintenance.

Published
2021

6. Mutations in emerging variant of concern lineages disrupt genomic sequencing of SARS-CoV-2 clinical specimens

Author

Jason Nguyen, Rebecca Hickman, Tracy D. Lee, Natalie Prystajecky, John R. Tyson, Agatha N. Jassem, Kevin S. Kuchinski, and Linda Hoang

Subjects
Genetics, Laboratory methods, 2019-20 coronavirus outbreak, Lineage (genetic), Coronavirus disease 2019 (COVID-19), Genomic sequencing, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Biology, Genome
Abstract

Mutations in emerging SARS-CoV-2 lineages can interfere with the laboratory methods used to generate high-quality genome sequences for COVID-19 surveillance. Here, we identify 46 mutations in current variant of concern lineages affecting the widely used laboratory protocols for SARS-CoV-2 genomic sequencing by Freed et al. and the ARTIC network. We provide laboratory data showing how three of these mutations disrupted sequencing of P.1 lineage specimens during a recent outbreak in British Columbia, Canada, and we also demonstrate how we modified the Freed et al. protocol to restore performance.

Published
2021

7. Uses of maritime heritage: the twenty-first-century life of the Newport Medieval Ship

Author

Rebecca Hickman

Subjects
Cultural Studies, History, 060102 archaeology, 05 social sciences, Museology, Geography, Planning and Development, Twenty-First Century, 06 humanities and the arts, Conservation, Ancient history, Tourism, Leisure and Hospitality Management, 0502 economics and business, 0601 history and archaeology, 050212 sport, leisure & tourism
Abstract

This paper explores the contemporary uses of maritime heritage as an identity-building and place-marketing tool by examining the case of the Newport Medieval Ship, a fifteenth-century merchant vess...

Published
2019

8. Naturally acquired antibody against Haemophilus influenzae type a in pediatric saliva

Author

Adriana Cabrera, Eli B. Nix, Rebecca Hickman, James E.A. Zlosnik, Marina Ulanova, and Manish Sadarangani

Subjects
Haemophilus Infections, Immunology, Humans, Infant, Immunology and Allergy, Child, Saliva, Antibodies, Bacterial, Haemophilus influenzae, Immunoglobulin A
Abstract

We developed a salivary assay for the detection of naturally acquired IgA antibody against Haemophilus influenzae type a (Hia) capsular polysaccharide in healthy Indigenous children from Northwestern Ontario, Canada. Hia-specific IgA antibody was detected in the saliva of 93% of Indigenous children aged 2-7 years.

Published
2022

9. Rapid, high throughput library preparation of SARS-CoV2 using Illumina’s DNA Prep Library Preparation Kit v1

Author

Jason Nguyen, Rebecca Hickman, Tracy Lee, Natalie Prystajecky, and John Tyson

Abstract

This procedure provides instructions on how to prepare DNA libraries for whole genome sequencing on an Illumina MiSeq or NextSeq using Illumina’s DNA Prep Library Preparation Kit scaled to half reaction volumes with modifications to the post-PCR procedures; tagmentation stop buffer and associated washes are removed and libraries are pooled post PCR then a single size selection is performed.

Published
2021

10. Generating 1200bp tiled Amplicons for SARS-CoV2 Whole Genome Sequencing v1

Author

jason.nguyen not provided, Tracy Lee, Rebecca Hickman, Natalie Prystajecky, and John Tyson

Abstract

This procedure provides instructions for how to generate amplicons across the entire SARS-CoV-2 genome to be used for downstream whole genome sequencing applications, including Illumina MiSeq/NextSeq or Oxford Nanopore MinION sequencing platforms. The steps involved in this protocol were derived from version 3 of Freed et al protocol nCoV-2019 sequencing protocol (RAPID barcoding, 1200bp amplicon)V.3 available at https://dx.doi.org/10.17504/protocols.io.bgggjttw

Published
2021

11. Epidemiology of

Author

James E A, Zlosnik, Deborah A, Henry, Trevor J, Hird, Rebecca, Hickman, Maureen, Campbell, Adriana, Cabrera, Giulio, Laino Chiavegatti, Mark A, Chilvers, and Manish, Sadarangani

Subjects
Canada, Cystic Fibrosis, Burkholderia, Incidence, Humans, Burkholderia Infections
Published
2020

12. Vaccine Effectiveness Against Lineage-matched and -mismatched Influenza B Viruses Across 8 Seasons in Canada, 2010–2011 to 2017–2018

Author

Catharine Chambers, Danuta M. Skowronski, Yan Li, Jonathan B. Gubbay, Suzana Sabaiduc, Christine Martineau, Gaston De Serres, Hugues Charest, Tracy Chan, Anne-Luise Winter, Steven J. Drews, Kevin Fonseca, Mel Krajden, James A. Dickinson, Caren Rose, Martin Petric, Agatha N. Jassem, Rebecca Hickman, and Nathalie Bastien

Subjects
Adult, Male, 0301 basic medicine, Microbiology (medical), Trivalent influenza vaccine, Canada, cross-protection, Lineage (genetic), Adolescent, Databases, Factual, Cross Protection, 030106 microbiology, Young Adult, 03 medical and health sciences, Immunogenicity, Vaccine, 0302 clinical medicine, Vaccine strain, influenza vaccine effectiveness, Influenza, Human, Humans, Medicine, 030212 general & internal medicine, Child, Vaccine Potency, Aged, Influenza B viruses, business.industry, Influenzavirus B, repeat vaccination, Infant, Middle Aged, influenza B virus, Virology, 3. Good health, Vaccination, Infectious Diseases, Immunization, Influenza Vaccines, Child, Preschool, Epidemiological Monitoring, Female, Brief Reports, Seasons, business, lineage
Abstract

Vaccine effectiveness (VE) against influenza B was derived separately for Victoria and Yamagata lineages across 8 seasons (2010–2011 to 2017–2018) in Canada when trivalent influenza vaccine was predominantly used. VE was ≥50% regardless of lineage match to circulating viruses, except when the vaccine strain was unchanged from the prior season.

Published
2018

13. Influenza Vaccine Effectiveness by A(H3N2) Phylogenetic Subcluster and Prior Vaccination History: 2016-2017 and 2017-2018 Epidemics in Canada

Author

Steven J. Drews, Suzana Sabaiduc, Gaston De Serres, Macy Zou, Yan Li, Rebecca Hickman, Mel Krajden, Tracy Chan, Catharine Chambers, Romy Olsha, Agatha N. Jassem, Danuta M. Skowronski, Nathalie Bastien, Siobhan Leir, Caren Rose, James A. Dickinson, Hugues Charest, Anne-Luise Winter, and Jonathan B. Gubbay

Subjects
Canada, Influenza vaccine, Hemagglutinin (influenza), Vaccine Efficacy, Disease cluster, Antigen, Influenza, Human, Immunology and Allergy, Medicine, Humans, Clade, Epidemics, Phylogeny, Phylogenetic tree, biology, business.industry, Influenza A Virus, H3N2 Subtype, Vaccination, Influenza a, Virology, Infectious Diseases, Influenza Vaccines, biology.protein, Seasons, business
Abstract

Background The influenza A(H3N2) vaccine was updated from clade 3C.3a in 2015–2016 to 3C.2a for 2016–2017 and 2017–2018. Circulating 3C.2a viruses showed considerable hemagglutinin glycoprotein diversification and the egg-adapted vaccine also bore mutations. Methods Vaccine effectiveness (VE) in 2016–2017 and 2017–2018 was assessed by test-negative design, explored by A(H3N2) phylogenetic subcluster and prior season’s vaccination history. Results In 2016–2017, A(H3N2) VE was 36% (95% confidence interval [CI], 18%–50%), comparable with (43%; 95% CI, 24%–58%) or without (33%; 95% CI, −21% to 62%) prior season’s vaccination. In 2017–2018, VE was 14% (95% CI, −8% to 31%), lower with (9%; 95% CI, −18% to 30%) versus without (45%; 95% CI, −7% to 71%) prior season’s vaccination. In 2016–2017, VE against predominant clade 3C.2a1 viruses was 33% (95% CI, 11%–50%): 18% (95% CI, −40% to 52%) for 3C.2a1a defined by a pivotal T135K loss of glycosylation; 60% (95% CI, 19%–81%) for 3C.2a1b (without T135K); and 31% (95% CI, 2%–51%) for other 3C.2a1 variants (with/without T135K). VE against 3C.2a2 viruses was 45% (95% CI, 2%–70%) in 2016–2017 but 15% (95% CI, −7% to 33%) in 2017–2018 when 3C.2a2 predominated. VE against 3C.2a1b in 2017–2018 was 37% (95% CI, −57% to 75%), lower at 12% (95% CI, −129% to 67%) for a new 3C.2a1b subcluster (n = 28) also bearing T135K. Conclusions Exploring VE by phylogenetic subcluster and prior vaccination history reveals informative heterogeneity. Pivotal mutations affecting glycosylation sites, and repeat vaccination using unchanged antigen, may reduce VE.

Published
2019

14. Early season co-circulation of influenza A(H3N2) and B(Yamagata): interim estimates of 2017/18 vaccine effectiveness, Canada, January 2018

Author

Nathalie Bastien, Mel Krajden, Yan Li, Jonathan B. Gubbay, James A. Dickinson, Steven J. Drews, Catharine Chambers, Danuta M. Skowronski, Rebecca Hickman, Gaston De Serres, Hugues Charest, Anne-Luise Winter, Agatha N. Jassem, and Tracy Chan

Subjects
0301 basic medicine, medicine.medical_specialty, Epidemiology, influenza virus, 03 medical and health sciences, 0302 clinical medicine, Antigen, Virology, Interim, genomics, medicine, 030212 general & internal medicine, vaccine effectiveness, business.industry, Public Health, Environmental and Occupational Health, virus diseases, Influenza a, mid-season, Influenza, Confidence interval, Vaccination, vaccine-preventable diseases, vaccines and immunisation, 030104 developmental biology, Immunization, Vaccine-preventable diseases, business, Rapid Communication
Abstract

Using a test-negative design, we assessed interim vaccine effectiveness (VE) for the 2017/18 epidemic of co-circulating influenza A(H3N2) and B(Yamagata) viruses. Adjusted VE for influenza A(H3N2), driven by a predominant subgroup of clade 3C.2a viruses with T131K + R142K + R261Q substitutions, was low at 17% (95% confidence interval (CI): −14 to 40). Adjusted VE for influenza B was higher at 55% (95% CI: 38 to 68) despite prominent use of trivalent vaccine containing lineage-mismatched influenza B(Victoria) antigen, suggesting cross-lineage protection.

Published
2018

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