Your search keyword '"Ines, Ushiro-Lumb"' showing total 10 results

1. 6 The impact of COVID-19 on corneal transplantation in England

Author

Lewis Downward, Ines Ushiro-Lumb, Cathy Hopkinson, Ulrike Paulus, and Shaminie Shanmugaranjan

Subjects

Ophthalmology, RE1-994

Published

2022

2. The EHA Research Roadmap: Transfusion Medicine

Author

Simon J. Stanworth, Anneke Brand, Srini V. Kaveri, Hans Vrielink, Andreas Greinacher, Dragoslav Domanović, Marieke von Lindern, Shubha Allard, Jagadeesh Bayry, Milos Bohonek, Andreas Buser, Frans H. J. Claas, Folke Knutson, Miguel Lozano, Martin L. Olsson, France Pirenne, Paolo Rebulla, Cynthia So-Osman, Jean-Daniel Tissot, Ashley M. Toye, Ines Ushiro-Lumb, Emile van den Akker, and Sacha Zeerleder

Subjects

Diseases of the blood and blood-forming organs, RC633-647.5

Published

2022

3. Modulated Zika virus NS1 conjugate offers advantages for accurate detection of Zika virus specific antibody in double antigen binding and Ig capture enzyme immunoassays.

Author

Richard S Tedder, Steve Dicks, Samreen Ijaz, Nathalia Caroline Santiago de Souza, Anderson Vincente de Paula, Flavia Levy, Raquel Medialdea-Carrera, José Eduardo Levi, Claudio S Pannuti, Patrícia Carvalho de Sequeira, David W G Brown, and Ines Ushiro Lumb

Subjects

Medicine, Science

Abstract

The accurate diagnosis and seroprevalence investigations of Zika virus (ZKV) infections remain complex due to cross reactivity with other flaviviruses. Two assay formats, both using labelled Zika virus NS1 antigen as a revealing agent (a double antigen binding assay, DABA, and an immunoglobulin Ig capture assay, G capture) were initially developed and compared with the indirect EuroimmunZ assay for the detection of anti-Zika antibody. Of 147 pre-Zika period serum samples, 39 (27%) were reactive in the EuroimmunZ or the DABA assays, 28 sera concordantly so. Such false reactivity was influenced by the serotype of Dengue virus (DV) to which individuals had been exposed to. Thus, of sera from patients undergoing secondary Dengue virus infection of known serotype, 91%, 45% and 28% of Dengue virus serotype 2, 3 and 4 respectively were reactive in one or more of the three assays. A novel method of quenching false sero-reactivity was therefore developed for the DABA and G capture assays. Initial addition of a single homologous Dengue virus serotype 3 NS1Ag quench significantly ablated false reactivities in the pre-Zika period sera. An equipotent quadrivalent quench comprising homologous Dengue virus serotypes 1 to 4 NS1Ag was shown to be optimum yet retained sensitivity for the detection of specific anti-Zika antibody. Comparing DABA and G capture assays using quenched and unquenched conjugates in comparison with EuroimmunZ early in the course of PCR-confirmed infection indicated that a significant component of the apparent early anti-ZIKA antibody response is likely to be due to a Zika virus-driven anamnestic anti-Dengue virus response. The increased specificity provided by homologous antigen quenching is likely to provide a significant improvement in sero-diagnostics and to be of clinical value.

Published

2019

4. Screening for SARS‐CoV‐2 in potential deceased organ donors

Author

Jasvir Parmar, Ian Currie, John Forsythe, Dale Gardiner, Jonathon Olsburgh, Chris J. Callaghan, Ines Ushiro-Lumb, and Marius Berman

Subjects

donors and donation: donor‐derived infections, 2019-20 coronavirus outbreak, medicine.medical_specialty, Tissue and Organ Procurement, Coronavirus disease 2019 (COVID-19), Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), infectious disease, organ procurement and allocation, Case Report, 030230 surgery, clinical research/practice, 03 medical and health sciences, 0302 clinical medicine, editorial/personal viewpoint, lung transplantation/pulmonology, Internal medicine, Immunology and Allergy, Medicine, Humans, Pharmacology (medical), Infectious disease (athletes), donors and donation: deceased, Letter to the Editor, Transplantation, Lung donor, business.industry, Transmission (medicine), SARS-CoV-2, infection and infectious agents – viral, COVID-19, respiratory system, Tissue Donors, respiratory tract diseases, business

Abstract

We describe a case of proven transmission of SARS‐CoV‐2 from lung donor to recipient. The donor had no clinical history or findings suggestive of infection with SARS‐CoV‐2 and tested negative by reverse transcriptase polymerase chain reaction (RT‐PCR) on a nasopharyngeal (NP) swab obtained within 48 h of procurement. Lower respiratory tract testing was not performed. The recipient developed fever, hypotension, and pulmonary infiltrates on posttransplant day (PTD) 3, and RT‐PCR testing for SARS‐CoV‐2 on an NP swab specimen was non‐reactive, but positive on bronchoalveolar lavage (BAL) fluid. One thoracic surgeon present during the transplantation procedure developed COVID‐19. Sequence analysis of isolates from donor BAL fluid (obtained at procurement), the recipient, and the infected thoracic surgeon proved donor origin of recipient and health‐care worker (HCW) infection. No other organs were procured from this donor. Transplant centers and organ procurement organizations should perform SARS‐CoV‐2 testing of lower respiratory tract specimens from potential lung donors, and consider enhanced personal protective equipment for HCWs involved in lung procurement and transplantation.

Published

2021

5. Neutralising antibodies in Spike mediated SARS-CoV-2 adaptation

Author

Iatm Ferreira, Katherine Sharrocks, Cjr Illingworth, Aminu S Jahun, S Gayed, Richard A. Goldstein, Rawlings Datir, G. Barcenas-Morales, Chris Smith, John Bradley, Theodore Gouliouris, Kgc Smith, Petra Mlcochova, Dami A. Collier, Laura E. McCoy, Ines Ushiro Lumb, Myra Hosmillo, Anna Smielewska, Rainer Doffinger, E Blane, David D. Pollock, Jordan P. Skittrall, Nigel Temperton, Effrossyni Gkrania-Klotsas, MJ van Gils, Steven Kemp, Chloe Rees-Spear, Jag Briggs, Ravindra K. Gupta, Ian Goodfellow, Anita Chandra, Lourdes Ceron-Gutierrez, David J. Roberts, and Medical Microbiology

Subjects

Infectivity, education.field_of_study, Convalescent plasma, biology, medicine.drug_class, SARS-CoV-2, Population, Mutant, Wild type, COVID-19, Monoclonal antibody, evasion, Virology, Virus, Article, resistance, Viral replication, medicine, biology.protein, antibody escape, immune suppression, Antibody, mutation, education, neutralising antibodies

Abstract

SARS-CoV-2 Spike protein is critical for virus infection via engagement of ACE2, and amino acid variation in Spike is increasingly appreciated. Given both vaccines and therapeutics are designed around Wuhan-1 Spike, this raises the theoretical possibility of virus escape, particularly in immunocompromised individuals where prolonged viral replication occurs. Here we report chronic SARS-CoV-2 with reduced sensitivity to neutralising antibodies in an immune suppressed individual treated with convalescent plasma, generating whole genome ultradeep sequences by both short and long read technologies over 23 time points spanning 101 days. Although little change was observed in the overall viral population structure following two courses of remdesivir over the first 57 days, N501Y in Spike was transiently detected at day 55 and V157L in RdRp emerged. However, following convalescent plasma we observed large, dynamic virus population shifts, with the emergence of a dominant viral strain bearing D796H in S2 and ΔH69/ΔV70 in the S1 N-terminal domain NTD of the Spike protein. As passively transferred serum antibodies diminished, viruses with the escape genotype diminished in frequency, before returning during a final, unsuccessful course of convalescent plasma. In vitro, the Spike escape double mutant bearing ΔH69/ΔV70 and D796H conferred decreased sensitivity to convalescent plasma, whilst maintaining infectivity similar to wild type. D796H appeared to be the main contributor to decreased susceptibility, but incurred an infectivity defect. The ΔH69/ΔV70 single mutant had two-fold higher infectivity compared to wild type and appeared to compensate for the reduced infectivity of D796H. Consistent with the observed mutations being outside the RBD, monoclonal antibodies targeting the RBD were not impacted by either or both mutations, but a non RBD binding monoclonal antibody was less potent against ΔH69/ΔV70 and the double mutant. These data reveal strong selection on SARS-CoV-2 during convalescent plasma therapy associated with emergence of viral variants with reduced susceptibility to neutralising antibodies.

Published

2020

6. Modulated Zika virus NS1 conjugate offers advantages for accurate detection of Zika virus specific antibody in double antigen binding and Ig capture enzyme immunoassays

Author

Ines Ushiro Lumb, David W. Brown, Steve Dicks, Raquel Medialdea-Carrera, Richard S. Tedder, José Eduardo Levi, Anderson Vincente de Paula, Samreen Ijaz, Cláudio Sérgio Pannuti, Nathalia Caroline Santiago de Souza, Patrícia Carvalho de Sequeira, and Flavia Levy

Subjects

Serotype, RNA viruses, Physiology, Biosensing Techniques, 030204 cardiovascular system & hematology, Dengue virus, Viral Nonstructural Proteins, medicine.disease_cause, Pathology and Laboratory Medicine, Antibodies, Viral, Cross-reactivity, Biochemistry, DISEASE, Zika virus, Binding Analysis, 0302 clinical medicine, Antibody Specificity, Limit of Detection, Immune Physiology, INFECTION, Medicine and Health Sciences, ASSAY, 030212 general & internal medicine, Enzyme-Linked Immunoassays, Materials, Antigens, Viral, Cross Reactivity, Multidisciplinary, Immune System Proteins, biology, Chemistry, 3. Good health, Multidisciplinary Sciences, Solutions, Serology, Medical Microbiology, Viral Pathogens, Viruses, Physical Sciences, Science & Technology - Other Topics, Medicine, Antibody, Pathogens, Research Article, TRANSMISSION, General Science & Technology, Diluents, Science, 030231 tropical medicine, Immunology, Materials Science, Immunoglobulins, Cross Reactions, Research and Analysis Methods, Microbiology, Virus, Antibodies, 03 medical and health sciences, Antigen, medicine, Seroprevalence, Humans, Immunoassays, Microbial Pathogens, Chemical Characterization, Science & Technology, Flaviviruses, Organisms, Biology and Life Sciences, Proteins, Zika Virus, Dengue Virus, biology.organism_classification, Virology, Mixtures, biology.protein, Immunologic Techniques, Conjugate

Abstract

The accurate diagnosis and seroprevalence investigations of Zika virus (ZKV) infections remain complex due to cross reactivity with other flaviviruses. Two assay formats, both using labelled Zika virus NS1 antigen as a revealing agent (a double antigen binding assay, DABA, and an immunoglobulin Ig capture assay, IgG capture) were initially developed and compared with the indirect EuroimmunZ assay for the detection of anti-Zika antibody. Of 147 pre-Zika period serum samples, 39 (27%) were reactive in the EuroimmunZ or the DABA assays, 28 sera concordantly so. Such false reactivity was influenced by the serotype of Dengue virus (DV) to which individuals had been exposed to. Thus, of sera from patients undergoing secondary Dengue virus infection of known serotype, 91%, 45% and 28% of Dengue virus serotype 2, 3 and 4 respectively were reactive in one or more of the three assays. A novel method of quenching false sero-reactivity was therefore developed for the DABA and IgG capture assays. Initial addition of a single homologous Dengue virus serotype 3 NS1Ag quench significantly ablated false reactivities in the pre-Zika period sera. An equipotent quadrivalent quench comprising homologous Dengue virus serotypes 1 to 4 NS1Ag was shown to be optimum yet retained sensitivity for the detection of specific anti-Zika antibody. Comparing DABA and IgG capture assays using quenched and unquenched conjugates in comparison with EuroimmunZ early in the course of PCR-confirmed infection indicated that a significant component of the apparent early anti-ZIKA antibody response is likely to be due to a Zika virus-driven anamnestic anti-Dengue virus response. The increased specificity provided by homologous antigen quenching is likely to provide a significant improvement in sero-diagnostics and to be of clinical value.

Published

2019

7. Antibody-based assay discriminates Zika virus infection from other flaviviruses

Author

Fausto Baldanti, Stefano Jaconi, Steve Dicks, Patricia Siqueira, Luisa Barzon, Damaris Collado, Davide Corti, Karin Stettler, Elisabetta Cameroni, José Victor Zambrana, Richard S. Tedder, Eva Harris, A.M. Bispo de Filippis, David W. G. Brown, Xia Jin, Francesca Rovida, Elena Percivalle, Saira Saborio, Ines Ushiro-Lumb, Samreen Ijaz, Angel Balmaseda, Maria Zambon, and Raquel Medialdea-Carrera

Subjects

0301 basic medicine, viruses, serology, Viral Nonstructural Proteins, Dengue virus, Antibodies, Viral, medicine.disease_cause, DISEASE, Serology, Zika virus, CHIKUNGUNYA, Dengue, 0302 clinical medicine, Monoclonal, Diagnosis, Pandemic, URINE, Flavivirus Infections, Viral, Prospective Studies, Child, PEDIATRIC DENGUE COHORT, REVERSE TRANSCRIPTION-PCR, Multidisciplinary, Zika Virus Infection, Antibodies, Monoclonal, virus diseases, Biological Sciences, TRAVELERS, Blocking, Vaccination, Multidisciplinary Sciences, Flavivirus, Infectious Diseases, Child, Preschool, Science & Technology - Other Topics, ELISA, Infection, Biotechnology, Adolescent, 030231 tropical medicine, Enzyme-Linked Immunosorbent Assay, Cross Reactions, Biology, DIAGNOSIS, Sensitivity and Specificity, Antibodies, Diagnosis, Differential, Vaccine Related, 03 medical and health sciences, Rare Diseases, Zika, Biodefense, MD Multidisciplinary, medicine, Humans, Seroprevalence, Antibodies, Blocking, Preschool, TIME RT-PCR, Science & Technology, Prevention, Zika Virus, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, dengue, flaviviruses, Virology, SPECIMENS, Vector-Borne Diseases, Emerging Infectious Diseases, Good Health and Well Being, 030104 developmental biology, Differential, Immunology, RNA, Immunization

Abstract

Zika virus (ZIKV) is a mosquito-borne flavivirus that emerged recently as a global health threat, causing a pandemic in the Americas. ZIKV infection mostly causes mild disease, but is linked to devastating congenital birth defects and Guillain-Barré syndrome in adults. The high level of cross-reactivity among flaviviruses and their cocirculation has complicated serological approaches to differentially detect ZIKV and dengue virus (DENV) infections, accentuating the urgent need for a specific and sensitive serological test. We previously generated a ZIKV nonstructural protein 1 (NS1)-specific human monoclonal antibody, which we used to develop an NS1-based competition ELISA. Well-characterized samples from RT-PCR-confirmed patients with Zika and individuals exposed to other flavivirus infections or vaccination were used in a comprehensive analysis to determine the sensitivity and specificity of the NS1 blockade-of-binding (BOB) assay, which was established in laboratories in five countries (Nicaragua, Brazil, Italy, United Kingdom, and Switzerland). Of 158 sera/plasma from RT-PCR-confirmed ZIKV infections, 145 (91.8%) yielded greater than 50% inhibition. Of 171 patients with primary or secondary DENV infections, 152 (88.9%) scored negative. When the control group was extended to patients infected by other flaviviruses, other viruses, or healthy donors (n = 540), the specificity was 95.9%. We also analyzed longitudinal samples from DENV-immune and DENV-naive ZIKV infections and found inhibition was achieved within 10 d postonset of illness and maintained over time. Thus, the Zika NS1 BOB assay is sensitive, specific, robust, simple, low-cost, and accessible, and can detect recent and past ZIKV infections for surveillance, seroprevalence studies, and intervention trials.

Published

2017

8. Chlamydia trachomatis variant not detected by plasmid based nucleic acid amplification tests: molecular characterisation and failure of single dose azithromycin

Author

Helen Lee, Claude‐Edouard-E. Michel, Sarah Alexander, Ines Ushiro-Lumb, Beng Tin Goh, Catherine A Ison, Jose Paolo V. Magbanua, and Aura Aguirre‐Andreasen

Subjects

Sexually transmitted disease, Adult, DNA, Bacterial, Male, Chlamydia trachomatis, Dermatology, Biology, Azithromycin, medicine.disease_cause, Polymerase Chain Reaction, Microbiology, law.invention, 03 medical and health sciences, 0302 clinical medicine, law, medicine, Nucleic Acid Amplification Tests, Humans, Chlamydiaceae, 030212 general & internal medicine, Treatment Failure, Polymerase chain reaction, Antibacterial agent, 0303 health sciences, Chlamydia, 030306 microbiology, Urethritis, Nucleic acid amplification technique, Chlamydia Infections, medicine.disease, biology.organism_classification, Virology, 3. Good health, Anti-Bacterial Agents, Infectious Diseases, New Variant, Nucleic Acid Amplification Techniques

Abstract

Objective: To characterise a Chlamydia trachomatis variant strain from a patient with non-gonococcal urethritis (NGU) whose first void urine (FVU) displayed discrepant C trachomatis test results and describe the clinical response to treatment. Methods: The FVU specimen was assayed with an immune based Chlamydia Rapid Test (CRT) and various nucleic acid amplification tests (NAATs) to establish C trachomatis infection. Sequencing of the major outer membrane protein gene (omp1 also known as ompA) was undertaken to identify the serovar of the variant strain. Polymerase chain reaction (PCR) analysis was also conducted to determine whether the strain harboured deletions in the cryptic plasmid or was plasmid free. Results: The FVU specimen was strongly reactive in CRT but negative with the plasmid based Amplicor PCR (Roche) and ProbeTec ET (Becton-Dickinson) assays. However, NAATs for 16S RNA (Aptima Combo 2, GenProbe), omp1 (RealArt CT PCR, Artus and in-house NAATs) or the outer membrane complex B protein gene (omcB) established C trachomatis infection. Sequencing of omp1 showed that the variant belonged to serovar I. PCR analysis indicated that the variant was plasmid free. The patient did not respond to single dose azithromycin treatment but subsequently responded to a course of doxycycline. Conclusions: A pathogenic plasmid free C trachomatis variant was identified. Clinicians should be alerted to the possibility of undetected C trachomatis infection caused by such variants and the potential of azithromycin failure in patients with recurrent chlamydial NGU. The occurrence of this variant is rare and should not form the basis for judgment of the performance or usefulness of plasmid based NAATs for C trachomatis detection.

Published

2007

9. Improving hepatitis C services across the UK: response to a walk-in HCV testing service

Author

R.F.C. D'Souza, Graham R. Foster, E. M. Alstead, Michael Glynn, and Ines Ushiro-Lumb

Subjects

Service (business), medicine.medical_specialty, education.field_of_study, Letter, Outpatient Clinics, Hospital, Walk-in, business.industry, Hepatitis C virus, Population, Gastroenterology, End stage liver disease, Hepatitis C, Hepatitis C, Chronic, medicine.disease, medicine.disease_cause, Health Services Accessibility, Internal medicine, Immunology, London, medicine, Humans, education, business

Abstract

The Department of Health (DH) estimates that approximately 0.4% of the UK population are chronically infected with hepatitis C virus (HCV) (that is, 200 000 people). As few as 10% of these individuals, who are at risk of end stage liver disease, are thought to be aware of their infection. Clearly action is required to identify and treat these patients with current drugs (pegylated interferons …

Published

2004

10. Evaluation of Roche Cobas Taqman Quantitative HIV-1 RNA PCR against other HIV-1 commercial viral load tests to examine potential under-quantification

Author

Adele V. Lee, Iain Reeves, Anthony R. Oliver, H Noble, Ines Ushiro-Lumb, Jane Anderson, S Limb, Guy Baily, X Couto-Parada, Duncan A. Clark, and Chloe Orkin

Subjects

business.industry, Cobas taqman, Human immunodeficiency virus (HIV), Public Health, Environmental and Occupational Health, RNA, medicine.disease_cause, Virology, Hiv 1 rna, Virological response, Infectious Diseases, Pcr test, Cobas amplicor, Medicine, business, Viral load

Abstract

Background HIV-1 RNA quantification underpins the monitoring of virological response to antiviral therapy, achievement of viral suppression and early identification of viral escape. Most laboratories use commercial HIV-1 RNA viral load tests and the genetic diversity of HIV-1 requires that these are applicable across all subtypes. We introduced the Roche Cobas Ampliprep/Cobas Taqman (CAP/CTM) Real Time Quantitative HIV-1 RNA PCR into diagnostic service after conducting a favourable comparative evaluation of 191 samples with the Roche Cobas Amplicor v1.5 PCR assay [1]. However, concerns were raised when in subsequent routine use we identified 10 patients where there was significant under-quantification (details will be presented, five subtyped all non-B). A separate study reported that Roche CTM was under-quantifying a significant number of samples across a range of subtypes compared to Amplicor [2]. We have undertaken a larger evaluation of CAP/CTM versus Roche Amplicor and have included evaluation of a subset against the Abbott quantitative HIV-1 RNA real-time PCR test.