Your search keyword '"Vauloup-Fellous C"' showing total 11 results

1. Humoral Immune Response after Primary Rubella Virus Infection and after Vaccination

Author

Vauloup-Fellous, C., primary and Grangeot-Keros, L., additional

Published

2007

2. Diagnostic performance of real-time quantitative PCR in tear samples in various subtypes of herpes simplex keratitis.

Author

Hoarau G, Haigh O, Vauloup-Fellous C, Boucher R, Rouquette A, Faure P, Limam L, Labetoulle M, and Rousseau A

Subjects

Humans, Retrospective Studies, Real-Time Polymerase Chain Reaction, Tears, Keratitis, Herpetic diagnosis, Herpesvirus 1, Human genetics, Lacerations

Abstract

Diagnosis of herpes simplex keratitis (HSK) is mostly based on clinical findings, yet biological confirmation supports management of challenging cases. This study evaluated the place of real-time quantitative PCR (RT-qPCR) on tear samplings in the management of HSK. Clinical records of patients who underwent tear sampling tested by RT-qPCR for herpes simplex virus type 1 for an acute episode of corneal inflammation or defect between January 2013 and December 2021 were retrospectively reviewed, and results were compared to clinical diagnosis (i.e., HSK or not) based on biomicroscopic findings and medical history. Of 465 tested tear samples from 364 patients, a clinical diagnosis of active (ongoing) HSK was recorded in 240 cases, among which 76 were RT-qPCR positive (global sensitivity of 31.6%, specificity of 99.5%). Sensitivity of RT-qPCR was higher in epithelial (97.4%) and stromal keratitis with ulceration (48.7%), compared to other types of HSK (23.5% in keratouveitis, 13.6% in endotheliitis, 11.1% in postherpetic neurotrophic keratopathy, and 8.1% in stromal keratitis without ulceration). The highest viral loads were detected from epithelial and stromal keratitis with ulceration, while in HSK with no epithelial involvement, the viral load detected was 196-fold lower, on average. The proportion of clinically characterized HSK patients with negative tear samples was higher in patients receiving antiviral treatment ( P < 0.0001). RT-qPCR, performed on tear samples, can help in confirming diagnosis in case of presumed HSK, including clinical forms with no obvious epithelial involvement. The sensitivity of tear sampling is much higher whenever epithelial keratitis is present., Competing Interests: The authors declare no conflict of interest.

Published

2023

3. Evaluating 10 Commercially Available SARS-CoV-2 Rapid Serological Tests by Use of the STARD (Standards for Reporting of Diagnostic Accuracy Studies) Method.

Author

Dortet L, Ronat JB, Vauloup-Fellous C, Langendorf C, Mendels DA, Emeraud C, Oueslati S, Girlich D, Chauvin A, Afdjei A, Bernabeu S, Le Pape S, Kallala R, Rochard A, Verstuyft C, Fortineau N, Roque-Afonso AM, and Naas T

Subjects

Antibodies, Viral blood, COVID-19 blood, COVID-19 pathology, Diagnostic Tests, Routine methods, Female, Humans, Immunoassay, Immunoglobulin G blood, Immunoglobulin M blood, Male, Middle Aged, Practice Guidelines as Topic, Retrospective Studies, SARS-CoV-2 immunology, Sensitivity and Specificity, COVID-19 diagnosis, COVID-19 Serological Testing methods, Diagnostic Tests, Routine standards, SARS-CoV-2 isolation & purification

Abstract

Numerous severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) rapid serological tests have been developed, but their accuracy has usually been assessed using very few samples, and rigorous comparisons between these tests are scarce. In this study, we evaluated and compared 10 commercially available SARS-CoV-2 rapid serological tests using the STARD (Standards for Reporting of Diagnostic Accuracy Studies) methodology. Two hundred fifty serum samples from 159 PCR-confirmed SARS-CoV-2 patients (collected 0 to 32 days after the onset of symptoms) were tested with rapid serological tests. Control serum samples ( n  = 254) were retrieved from pre-coronavirus disease (COVID) periods from patients with other coronavirus infections ( n   = 11), positivity for rheumatoid factors ( n   = 3), IgG/IgM hyperglobulinemia ( n   = 9), malaria ( n  = 5), or no documented viral infection ( n   = 226). All samples were tested using rapid lateral flow immunoassays (LFIAs) from 10 manufacturers. Only four tests achieved ≥98% specificity, with the specificities ranging from 75.7% to 99.2%. The sensitivities varied by the day of sample collection after the onset of symptoms, from 31.7% to 55.4% (days 0 to 9), 65.9% to 92.9% (days 10 to 14), and 81.0% to 95.2% (>14 days). Only three of the tests evaluated met French health authorities' thresholds for SARS-CoV-2 serological tests (≥90% sensitivity and ≥98% specificity). Overall, the performances varied greatly between tests, with only one-third meeting acceptable specificity and sensitivity thresholds. Knowledge of the analytical performances of these tests will allow clinicians and, most importantly, laboratorians to use them with more confidence; could help determine the general population's immunological status; and may help diagnose some patients with false-negative real-time reverse transcription-PCR (RT-PCR) results., (Copyright © 2021 American Society for Microbiology.)

Published

2021

4. Evaluation of a Rapid Diagnostic Assay for Detection of SARS-CoV-2 Antigen in Nasopharyngeal Swabs.

Author

Lambert-Niclot S, Cuffel A, Le Pape S, Vauloup-Fellous C, Morand-Joubert L, Roque-Afonso AM, Le Goff J, and Delaugerre C

Subjects

COVID-19, COVID-19 Testing, Coronavirus Infections virology, Humans, Pandemics, Pneumonia, Viral virology, Point-of-Care Testing, SARS-CoV-2, Sensitivity and Specificity, Antigens, Viral analysis, Betacoronavirus isolation & purification, Clinical Laboratory Techniques methods, Coronavirus Infections diagnosis, Immunoassay methods, Nasopharynx virology, Pneumonia, Viral diagnosis

Published

2020

5. True Measles Cases Undetected by Reverse Transcription-PCR (RT-PCR): Effect of Genetic Variability on Assay Sensitivity Needs To Be Regularly Surveyed.

Author

Dina J, Omnes J, Vauloup-Fellous C, Collet L, Hamel J, Antona D, Hübschen JM, Ben Mamou M, and Vabret A

Subjects

DNA Primers genetics, Epidemiological Monitoring, False Negative Reactions, France, Humans, Measles virology, Measles virus genetics, Measles virus isolation & purification, Molecular Diagnostic Techniques methods, Polymorphism, Single Nucleotide, RNA, Viral genetics, Reagent Kits, Diagnostic standards, Reverse Transcriptase Polymerase Chain Reaction methods, Reverse Transcription, Sensitivity and Specificity, Genetic Variation, Measles diagnosis, Molecular Diagnostic Techniques standards, Reverse Transcriptase Polymerase Chain Reaction standards

Published

2019

6. Assessing Immunity to Rubella Virus: a Plea for Standardization of IgG (Immuno)assays.

Author

Bouthry E, Furione M, Huzly D, Ogee-Nwankwo A, Hao L, Adebayo A, Icenogle J, Sarasini A, Revello MG, Grangeot-Keros L, and Vauloup-Fellous C

Subjects

Adult, Animals, Female, Humans, Pregnancy, Antibodies, Viral blood, Immunoassay standards, Immunoglobulin G blood, Pregnancy Complications, Infectious prevention & control, Rubella prevention & control, Rubella virus immunology

Abstract

Immunity to rubella virus (RV) is commonly determined by measuring specific immunoglobulin G (RV IgG). However, RV IgG results and their interpretation may vary, depending on the immunoassay, even though most commercial immunoassays (CIAs) have been calibrated against an international standard and results are reported in international units per milliliter. A panel of 322 sera collected from pregnant women that tested negative or equivocal for RV IgG in a prior test (routine screening) was selected. This panel was tested with two reference tests, immunoblotting (IB) and neutralization (Nt), and with 8 CIAs widely used in Europe. IB and Nt gave concordant results on 267/322 (82.9%) sera. Of these, 85 (26.4%) sera were negative and 182 (56.5%) sera were positive for both tests. All 85 IB/Nt-negative samples were classified as negative with all CIAs. Of the 182 IB/Nt-positive samples, 25.3 to 61.5% were classified as equivocal and 6 to 64.8% were classified as positive with the CIAs. Wide variations in titers in international units per milliliter were observed. In our series, more than half of the women considered susceptible to RV based on CIA results tested positive for RV antibodies by IB/Nt. Our data suggest that (i) sensitivity of CIAs could be increased by considering equivocal results as positive and (ii) the definition of immunity to RV as the 10-IU/ml usual cutoff as well as the use of quantitative results for clinical decisions may warrant reconsideration. A better standardization of CIAs for RV IgG determination is needed., (Copyright © 2016, American Society for Microbiology. All Rights Reserved.)

Published

2016

7. Standardization of Assays That Detect Anti-Rubella Virus IgG Antibodies.

Author

Dimech W, Grangeot-Keros L, and Vauloup-Fellous C

Subjects

Humans, Antibodies, Viral blood, Enzyme-Linked Immunosorbent Assay methods, Enzyme-Linked Immunosorbent Assay standards, Immunoglobulin G blood, Rubella virus immunology

Abstract

Rubella virus usually causes a mild infection in humans but can cause congenital rubella syndrome (CRS). Vaccination programs have significantly decreased primary rubella virus infection and CRS; however, vaccinated individuals usually have lower levels of rubella virus IgG than those with natural infections. Rubella virus IgG is quantified with enzyme immunoassays that have been calibrated against the World Health Organization (WHO) international standard and report results in international units per milliliter. It is recognized that the results reported by these assays are not standardized. This investigation into the reasons for the lack of standardization found that the current WHO international standard (RUB-1-94) fails by three key metrological principles. The standard is not a pure analyte but is composed of pooled human immunoglobulin. It was not calibrated by certified reference methods; rather, superseded tests were used. Finally, no measurement uncertainty estimations have been provided. There is an analytical and clinical consequence to the lack of standardization of rubella virus IgG assays, which leads to misinterpretation of results. The current approach to standardization of rubella virus IgG assays has not achieved the desired results. A new approach is required., (Copyright © 2015, American Society for Microbiology. All Rights Reserved.)

Published

2016

8. Phylogenetic analysis of rubella viruses involved in congenital rubella infections in France between 1995 and 2009.

Author

Vauloup-Fellous C, Hübschen JM, Abernathy ES, Icenogle J, Gaidot N, Dubreuil P, Parent-du-Châtelet I, Grangeot-Keros L, and Muller CP

Subjects

Cluster Analysis, Female, France epidemiology, Humans, Molecular Epidemiology, Phylogeny, Pregnancy, RNA, Viral analysis, Rubella virus isolation & purification, Viral Envelope Proteins genetics, Amniotic Fluid virology, Rubella Syndrome, Congenital epidemiology, Rubella Syndrome, Congenital virology, Rubella virus genetics

Abstract

Rubella is an acute infectious disease that normally has a mild clinical course. However, infections during pregnancy, especially before week 12 of gestation (WG), can cause severe birth defects known as congenital rubella syndrome (CRS). The aim of this study was to perform genotyping and molecular characterization of rubella viruses involved in congenital infections in France over the past 15 years (1995 to 2009). Amniotic fluid (AF) specimens (n = 80) from pregnant women with congenital rubella infections (CRI) before week 20 of gestation, and a few other samples available from children/newborns with CRS (n = 26), were analyzed. The coding region of the rubella virus E1 gene was amplified directly from clinical specimens by reverse transcriptase PCR, and the resulting DNA fragments were sequenced. Sequences were assigned to genotypes by phylogenetic analysis with rubella virus reference sequences. Sufficient E1 gene sequences were obtained from 56 cases. Phylogenetic analysis of the sequences showed that at least five different genotypes (1E, 1G, 1B, 2B, and 1h) were present in France and were involved in congenital infections, with a strong predominance of genotype 1E (87%). This is one of the very few comprehensive studies of rubella viruses involved in CRI. The results indicated that over the past 15 years, multiple introductions of the dominant genotype E caused most of the CRI cases in France. A few sporadic cases were due to other genotypes (1B, 1G, 1h, 2B).

Published

2010

9. Evaluation of different cytomegalovirus (CMV) DNA PCR protocols for analysis of dried blood spots from consecutive cases of neonates with congenital CMV infections.

Author

Soetens O, Vauloup-Fellous C, Foulon I, Dubreuil P, De Saeger B, Grangeot-Keros L, and Naessens A

Subjects

Adult, Cytomegalovirus genetics, Cytomegalovirus Infections virology, DNA, Viral analysis, Female, Humans, Infant, Newborn, Sensitivity and Specificity, Urine virology, Blood virology, Blood Specimen Collection methods, Cytomegalovirus isolation & purification, Cytomegalovirus Infections congenital, Cytomegalovirus Infections diagnosis, DNA, Viral isolation & purification, Polymerase Chain Reaction methods

Abstract

Two protocols for the extraction of cytomegalovirus (CMV) DNA and two methods for the amplification of CMV DNA in dried blood spots were evaluated for the retrospective diagnosis of congenital CMV infection. During the period from 1996 to 2006, a urine screening program detected 76 congenitally infected neonates. Stored Guthrie cards with blood from 55 cases and 12 controls were tested. Two spots of dried blood were cut from each card and evaluated in two centers. CMV DNA was extracted from a whole single spot. Center 1 used phenol-chloroform extraction and ethanol precipitation followed by a conventional PCR. Center 2 used the NucliSens easyMAG automated DNA/RNA extraction platform (bioMérieux) followed by a real-time PCR. For evaluation of the extraction method, DNA extracted from each blood spot was evaluated by the amplification method used by the collaborating center. The sensitivities were 66% for center 1 and 73% for center 2. None of the controls were positive. A sensitivity as high as 82% could be obtained by combining the most sensitive extraction method (the phenol-chloroform procedure) with the most sensitive PCR method (real-time PCR). The detection rate was not influenced by the duration of storage of the spots. The sensitivity was higher with blood from congenitally infected cases due to a primary maternal CMV infection, regardless of the protocol used. However, the difference reached significance only for the least-sensitive protocol (P = 0.036).

Published

2008

10. Development of a rapid and convenient method for determination of rubella virus-specific immunoglobulin G avidity.

Author

Vauloup-Fellous C, Ursulet-Diser J, and Grangeot-Keros L

Subjects

Antibodies, Viral blood, Humans, Immunoglobulin G blood, Immunoglobulin M blood, Immunoglobulin M immunology, Rubella virology, Antibodies, Viral immunology, Antibody Affinity, Enzyme-Linked Immunosorbent Assay methods, Immunoglobulin G immunology, Rubella immunology, Rubella virus immunology

Abstract

We describe here a rapid and semiautomated method for the determination of rubella virus immunoglobulin G (IgG) avidity with the VIDAS instrument. A total of 153 serum samples from persons with naturally acquired rubella virus infections (n = 98), from vaccinated persons (n = 44), and from patients with autoantibodies (n = 11) were included in this study. The rubella virus-specific IgG avidity assay we developed for the VIDAS instrument was evaluated by comparison with an in-house method. Results obtained with the VIDAS instrument allow considering this method valuable to help confirm or exclude acute primary infection or recent vaccination.

Published

2007

11. Evaluation of cytomegalovirus (CMV) DNA quantification in dried blood spots: retrospective study of CMV congenital infection.

Author

Vauloup-Fellous C, Ducroux A, Couloigner V, Marlin S, Picone O, Galimand J, Loundon N, Denoyelle F, Grangeot-Keros L, and Leruez-Ville M

Subjects

Child, Preschool, Cytomegalovirus genetics, Humans, Infant, Infant, Newborn, Retrospective Studies, Sensitivity and Specificity, Viral Load, Cytomegalovirus isolation & purification, Cytomegalovirus Infections congenital, Cytomegalovirus Infections diagnosis, DNA, Viral blood, Polymerase Chain Reaction methods

Abstract

We compared two protocols for extracting DNA from dried blood spots for cytomegalovirus (CMV) DNA detection and quantification by real-time PCR. Both extraction methods were reliable for the retrospective diagnosis of CMV congenital infection. Quantification of CMV DNA was valuable after normalization of viral loads with albumin gene PCR amplification results.

Published

2007