Your search keyword '"Damond, Florence"' showing total 460 results

151. Impact of HIV-1 Genetic Diversity on Plasma HIV-1 RNA Quantification.

Author

François Rouet, Chaix, Marie-laure, Nerrienet, Eric, Ngo-Giang-Huong, Nicole, Plantier, Jean-Christophe, Burgard, Marianne, Peeters, Martine, Damond, Florence, Koumavi Ekouevi, Didier, Msellati, Philippe, Ferradini, Laurent, Rukobo, Sandra, Maréchal, Valérie, Schvachsa, Nilda, Wakrim, Lahcen, Rafalimanana, Christian, Rakotoambinina, Benjamin, Viard, Jean-Paul, Seigneurin, Jean-Marie, and Rouzioux, Christine

Published

2007

152. Impact of gaggenetic determinants on virological outcome to boosted lopinavir-containing regimen in HIV-2-infected patients

Author

Larrouy, Lucile, Vivot, Alexandre, Charpentier, Charlotte, Bénard, Antoine, Visseaux, Benoit, Damond, Florence, Matheron, Sophie, Chene, Geneviève, Brun-Vezinet, Françoise, and Descamps, Diane

Abstract

This study investigated the impact on virological outcome of the gagcleavage sites and the protease-coding region mutations in protease inhibitor-naive and protease inhibitor-experienced patients infected with HIV-2 receiving lopinavir (LPV) containing regimen.

Published

2013

153. Long-Lasting Persistence of Integrase Resistance Mutations in HIV-2-Infected Patients after Raltegravir Withdrawal

Author

Charpentier, Charlotte, Larrouy, Lucile, Matheron, Sophie, Damond, Florence, Delelis, Olivier, Mouscadet, Jean-François, Campa, Pauline, Chêne, Geneviève, Brun-Vézinet, Françoise, and Descamps, Diane

Abstract

Background Little is known in HIV-2 infection about the kinetics of disappearance of raltegravir (RAL)-resistant virus after RAL withdrawal.Methods RAL was interrupted in four highly antiretroviral- experienced HIV-2-infected patients exhibiting a virological failure when receiving RAL. Integrase gene was sequenced from plasma samples collected at the time of RAL failure and at further time points following RAL withdrawal.Results At the time of RAL withdrawal, virus exhibited different integrase resistance pathways: G140S/Q148R, E92Q/N155H, T97A/N155H and T97A/Y143C. In patient 1, the G140S/Q148R double-mutant was still detected at month (M)7 and at M11 after stopping RAL, but was no longer detected at M15. Regarding patient 2, the double- mutant E92Q/N155H was still present at M2 and M8 after stopping RAL, and was no longer detected at M12. In patient 3, RAL-resistant virus with T97A/N155H mutations were still present 1 month after stopping RAL, and were no longer detected at M14. Regarding patient 4, the mutant T97A/Y143C was still detected at M1 and M3 following RAL withdrawal. At M18 after RAL stop, integrase genotypic pattern evolved to T97A/Y143G.Conclusions Persistence of HIV-2 RAL-resistant mutants was observed in all the key genetic RAL resistance pathways. These findings have clinical implications especially in HIV-2-infected patients for whom therapeutic arsenal is limited compared to HIV-1, since the persistence of resistant mutants might compromise the possible efficacy of upcoming second-generation integrase inhibitors.

Published

2011

154. In vitroPhenotypic Susceptibility to Nucleoside Reverse Transcriptase Inhibitors of HIV-2 Isolates with the Q151M Mutation in the Reverse Transcriptase Gene

Author

Damond, Florence, Collin, Gilles, Matheron, Sophie, Peytavin, Gilles, Campa, Pauline, Delarue, Séverine, Taieb, Audrey, Bénard, Antoine, Chêne, Geneviève, Brun-Vézinet, Françoise, and Descamps, Diane

Abstract

In HIV-2 infection, many studies have reported a high frequency of selection of the Q151M mutation, but its impact on phenotypic susceptibility of HIV-2 isolates remains unclear. Four HIV-2 infected patients from the French ANRS HIV-2 cohort, with evidence of Q151M mutation in both plasma and available peripheral blood mononuclear cells (PBMCs) co-cultivated supernatants, were selected. In vitrophenotypic susceptibilities to different nucleoside reverse transcriptase inhibitors (NRTIs) were determined using a PBMC assay. In HIV-2 isolates, the Q151M mutation alone impacts only the phenotypic susceptibility to stavudine and abacavir. A decrease in susceptibility to all NRTIs was observed when Q151M was selected with V111I, a mutation of unknown impact on HIV-1 resistance. Clinical relevance of these phenotypic susceptibility results needs to be evaluated in HIV-2 treated patients.

Published

2005

155. High frequency of selection of K65R and Q151M mutations in HIV‐2 infected patients receiving nucleoside reverse transcriptase inhibitors containing regimen

Author

Descamps, Diane, Damond, Florence, Matheron, Sophie, Collin, Gilles, Campa, Pauline, Delarue, Severine, Pueyo, Sophie, Chêne, Genevieve, and Brun‐Vézinet, Francoise

Abstract

The objective of the study was to determine retrospectively which substitutions in the reverse transcriptase (RT) gene are selected in vivo during nucleoside RT inhibitors (NRTI) containing regimen in HIV‐2 infected subjects. Thirty‐four HIV‐2 patients having received NRTI‐containing regimen with available specimens and amplifiable RT gene were studied. Analyses of RT gene were undertaken after a median NRTI exposure of 51 months (range: 5–128). Mutations at positions known to be involved in HIV‐1 resistance were observed in 26/34 patients. Selection of Q151M mutation was observed in nine out of 34 isolates (26%) after a median NRTIs exposure of 41 months (range: 12–77). In 8/9 cases, Q151M mutation was associated with other substitutions at positions known to be involved in HIV‐1 resistance: K65R (n = 6), D67N (n = 1), N69S or T (n = 2), K70R (n = 3), M184V (n = 4), S215Y (n = 1). Compared with HIV‐1 infection, there is a high frequency of selection of Q151M mutation in HIV‐2 infected patients receiving various combinations of NRTIs. In these highly thymidine analogue pretreated patients, the selection of thymidine analogue mutations was low suggesting that the pathway to resistance is very different between these two viruses. J. Med. Virol. 74:197–201, 2004. © 2004 Wiley‐Liss, Inc.

Published

2004

156. Impact of Stavudine Phenotype and Thymidine Analogues Mutations on Viral Response to Stavudine plus Lamivudine in Altis 2 Anrs Trial

Author

Calvez, Vincent, Costagliola, Dominique, Descamps, Diane, Yvon, Anne, Collin, Gilles, Cécile, Agnès, Delaugerre, Constance, Damond, Florence, Marcelin, Anne-Geneviève, Matheron, Sophie, Simon, Anne, Valantin, Marc-Antoine, Katlama, Christine, and Brun-Vézinet, Françoise

Abstract

Objective Stavudine-based antiretroviral combinations are less effective in zidovudine-experienced patients than in naive subjects and recently, mutations have been described to be associated to the use of both stavudine and zidovudine. In the ALTIS 2 trial, it was shown that a combination of stavudine and lamivudine is less effective in zidovudine-experienced patients than in naive patients. We conducted a retrospective genotypic and phenotypic resistance study (expressed as stavudine phenotypic index, calculated by dividing the inhibitory concentrations 50% [IC50] by the mean value of the sensitive viruses) to evaluate the factors associated with decrease in plasma HIV-1 RNA.Design Associations with continuous variables were studied using non-parametric Spearman correlation coefficients. Associations with categorical variables were studied using non-parametric Mann–Whitney tests. Multivariate stepwise regression analyses were used to determine independent prognostic factors of the virological response.Results At baseline, most of the subjects harboured zidovudine-associated mutations in plasma and peripheral blood mononuclear cells. Zidovudine and stavudine IC50and IC90were strongly associated with response. It appears that a cut-off of stavudine phenotypic index of 1.8-fold of IC50, much lower than the usually used value, could be clinically significant for response to stavudine. In the multivariate analysis, the stepwise model with the higher multiple correlation coefficient (R2=0.742) included the presence of a 215 Y/F mutation, the number of previously used nucleoside analogues and a resistant stavudine phenotype.Conclusion These results argue for a phenotypic and genotypic cross resistance between stavudine and zidovudine. Modest increases of IC50and IC90for stavudine had an important impact on the virological response during the trial and plead for a new definition of the threshold value for stavudine phenotypic index.

Published

2002

157. Development and Evaluation of a DNA Enzyme Immunoassay Method for envGenotyping of Subtypes A through G of Human Immunodeficiency Virus Type 1 Group M, with Discrimination of the Circulating Recombinant Forms CRF01_AE and CRF02_AG

Author

Plantier, Jean-Christophe, Vergne, Laurence, Damond, Florence, MBoup, Souleymane, MPoudi-NGole, Eitel, Buzelay, Laurence, Farfara, Isabelle, Brand, Denys, Peeters, Martine, Brun-Ve´zinet, Franc¸oise, Delaporte, Eric, and Barin, Francis

Abstract

ABSTRACTThe tools currently available for genetic subtyping of human immunodeficiency virus type 1 are laborious or can be used only for the analysis of a limited number of samples and/or subtypes. We developed and evaluated a molecular biology-based method using subtype-specific oligonucleotide probes for envgenotyping of subtypes A through G, CRF01_AE, and CRF02_AG. DNA enzyme immunoassay (DEIA) genotyping is based on nested PCR amplification of the 5' end of the envgene (proviral DNA), followed by subtype-specific hybridization and immunoenzymatic detection on microplates. DEIA genotyping was validated with a large number of samples (n= 128) collected in Europe (France; n= 47), West-Central Africa (Cameroon; n= 36), and West Africa (Senegal; n= 45). Three different formats, depending on the distribution of subtypes in the three countries, were developed. The results were compared with those obtained by sequencing of the V3-V5 region and phylogenetic analysis or an envheteroduplex mobility assay. Additional sequencing and phylogenetic analyses of the DEIA region (the first codon of the env coding sequence to the middle of conserved region C1 of gp120) were performed to investigate the reasons for discrepancies. Intense and highly specific reactions between the oligonucleotide probes and the corresponding samples were observed. Overall, correct identification was achieved for 107 of 128 samples (83.6%). One sample was not amplified, 10 (8%) were nontypeable (NT), and 10 (8%) were misidentified. Six of the 10 discordant samples were further investigated by phylogenetic analysis, which indicated that these samples corresponded to recombinants involving the env 5' end and the V3 and V5 regions of the two parental clades. Sequencing of NT samples showed numerous differences between sample and probe sequences, resulting in a lack of hybridization, and revealed the limitations of the selected probes in terms of specificity and sensitivity. We demonstrated the feasibility of DEIA genotyping: six subtypes plus the two most prevalent circulating recombinant forms were discriminated by using the 5' end of the envgene. This method can be adapted to the local situation by including only probes that correspond to the prevalent strains.

Published

2002

158. Prevalence of subtype-related polymorphisms associated with in vitro resistance to attachment inhibitor BMS-626529 in HIV-1 ‘non-B’-infected patients.

Author

Charpentier, Charlotte, Larrouy, Lucile, Visseaux, Benoit, Landman, Roland, Levittas, Marine, Storto, Alexandre, Damond, Florence, Yazdanpanah, Yazdan, Yeni, Patrick, Brun-Vézinet, Françoise, and Descamps, Diane

Subjects

ANTIVIRAL agents, AIDS, HIV, HIV infections, PATIENTS

Abstract

Objectives BMS-626529 is a member of the new drug class of HIV-1 attachment inhibitors currently in development. Mutations selected during in vitro experiments with BMS-626529 are located in the gp120 region: L116P, A204D, M426L, M434I-V506M and M475I. A differential antiviral activity of BMS-626529 was observed depending of the viral subtype. The aim of our study was to assess the prevalence of subtype-related polymorphisms previously described as being associated with in vitro resistance to BMS-626529 in patients infected with different HIV-1 ‘non-B’ subtypes. Patients and methods The prevalence of substitutions in gp120 was assessed in 85 HIV-infected patients (not previously treated with attachment inhibitors and infected with HIV-1 ‘non-B’ subtypes) by performing direct sequencing of the gp120 region. Results The most prevalent HIV-1 subtype was CRF02_AG (n = 46, 54%). The M426L substitution was found in virus from 10 patients (11.8%), mainly in subtypes D and CRF02_AG. The M434I substitution was found in virus from 11 patients (12.9%), mainly in subtypes CRF02_AG and CRF06_cpx. None of the CRF02_AG viruses harboured both M426L and M434I substitutions. Conclusions In our series, the M426L substitution in the gp120 region was detected in 46% and 7% of subtype D and CRF02_AG samples, respectively, and might affect the activity of BMS-626529 against these specific subtypes. Further studies are needed to better describe associations between HIV-1 ‘non-B’-subtype-related polymorphism profiles and the level of phenotypic resistance to attachment inhibitor BMS-626529. [ABSTRACT FROM PUBLISHER]

Published

2012

159. In-vitro phenotypic susceptibility of HIV-2 clinical isolates to the integrase inhibitor S/GSK1349572.

Author

Charpentier, Charlotte, Larrouy, Lucile, Collin, Gilles, Damond, Florence, Matheron, Sophie, Chêne, Geneviève, Nie, Ting, Schinazi, Raymond, Brun-Vézinet, Françoise, Descamps, Diane, and French ANRS HIV-2 Cohort (ANRS CO 05 VIH-2)

Published

2010

160. HIV-2 X4 tropism is associated with lower CD4cell count in treatment-experienced patients

Author

Visseaux, Benoit, Charpentier, Charlotte, Rouard, Caroline, Fagard, Catherine, Glohi, David, Tubiana, Roland, Damond, Florence, Brun-Vézinet, Françoise, Matheron, Sophie, and Descamps, Diane

Abstract

The distribution and evolution of X4R5 viral tropism during HIV-2 infection remains unknown. HIV-2 tropism was assessed in 83 antiretroviral-experienced patients with virological failure. Tropism was predicted as X4 in 58 of patients and was associated with a CD4cell count of less than 100cellsl, and with a higher number of drug resistance mutations. This high prevalence of X4 virus might compromise the use of CCR5 inhibitors, currently mostly considered in HIV-2 salvage therapy of highly pretreated patients.

Published

2014

161. Real-world data on long-acting intramuscular maintenance therapy with cabotegravir and rilpivirine mirror Phase 3 results.

Author

Serris, Alexandra, Ferre, Valentine Marie, Hingrat, Quentin Le, Bachelard, Antoine, Charpentier, Charlotte, Exarchopoulos, Marina, Damond, Florence, Phung, Bao-Chau, Landman, Roland, Yazdanpanah, Yazdan, Descamps, Diane, Joly, Véronique, Peytavin, Gilles, and Ghosn, Jade

Subjects

*INTRAMUSCULAR injections, *BODY mass index, *VIRAL load, *WEIGHT gain, *CLINICAL trials

Abstract

Introduction Cabotegravir, an integrase strand transfer inhibitor, and rilpivirine, an NNRTI, constitute the first long-acting (LA), injectable, two-drug ART regimen approved for the maintenance of virological suppression in persons living with HIV-1 (PLHIV). The aim of this study was to assess clinical effectiveness and tolerability of LA cabotegravir/rilpivirine in a real-world setting. Patients and methods We conducted a retrospective, single centre study, including all PLHIV receiving LA cabotegravir/rilpivirine as standard-of-care in our tertiary centre even if initiated in clinical trials. Results Between 2014 and 2022, 126 PLHIV initiated LA cabotegravir/rilpivirine. All were ART-experienced, and 98.4% had a viral load (VL) of <50 copies/mL before LA cabotegravir/rilpivirine initiation. Median BMI at cabotegravir/rilpivirine initiation was 24 IQR (23–28). During a median follow-up of 9 months IQR (7–24), 27 patients discontinued cabotegravir/rilpivirine: 5 because of virological failure, 6 for adverse events, 11 for personal reasons unrelated to treatment tolerance and 5 for other reasons. Virological failure was not associated with a higher BMI, nor with weight gain during LA intramuscular (IM) cabotegravir/rilpivirine treatment, inadequate cabotegravir and rilpivirine concentrations, VL blips or the use of oral lead-in (OLI) or not. No drug resistance-associated mutation emerged. Adverse events leading to treatment interruption were injection-site pain (n  = 3) and neuropsychological side effects (n  = 3). A correlation between BMI and both cabotegravir and rilpivirine concentrations at 1 month post-initiation of LA-IM cabotegravir/rilpivirine was observed, with no impact of OLI. Conclusions Data from this real-world cohort of PLHIV who received cabotegravir/rilpivirine LA injections suggest that this regimen is effective and well tolerated. Virological failures were not associated with the acquisition of resistance mutations. [ABSTRACT FROM AUTHOR]

Published

2024

162. In Vitro Phenotypic Susceptibility of HIV-2 Clinical Isolates to CCR5 Inhibitors

Author

Visseaux, Benoit, Charpentier, Charlotte, Hurtado-Nedelec, Margarita, Storto, Alexandre, Antoine, Romain, Peytavin, Gilles, Damond, Florence, Matheron, Sophie, Brun-Vézinet, Françoise, and Descamps, Diane

Abstract

HIV-2 is naturally resistant to nonnucleoside reverse transcriptase inhibitors, to a fusion inhibitor, and to some of the protease inhibitors. Maraviroc is the first drug of the new anti-CCR5 drug class and is effective only on CCR5-tropic (R5) HIV-1. No previous studies concerning HIV-2 susceptibility to maraviroc have been reported yet. We developed a phenotypic maraviroc susceptibility test using a peripheral blood mononuclear cell (PBMC) model. We analyzed the maraviroc susceptibility of 13 R5 HIV-2, 2 X4R5 (dual) HIV-2, and 2 CXCR4-tropic (X4) HIV-2 clinical isolates. We also tested, with the same protocol, 1 X4 HIV-1 and 4 R5 HIV-1 clinical isolates. For the R5 HIV-2 clinical isolates, the 50% effective concentration (EC50) for maraviroc was 0.80 nM (interquartile range [IQR], 0.48 to 1.39 nM), similar to that observed for the R5 HIV-1 isolates. The median maximum percentage of inhibition in the R5 HIV-2 isolates was 93% (IQR, 84 to 98%), similar to that observed in the R5 HIV-1 isolates. As expected, both X4 HIV-1 and HIV-2 were highly resistant to maraviroc. Our study showed for the first time that maraviroc is active in vitro against R5 HIV-2. The new tools we developed will allow identification of HIV-2-infected patients eligible for CCR5 inhibitor use and management of virological failure when receiving a maraviroc-based regimen.

Published

2011

163. In VitroPhenotypic Susceptibility of HIV-2 Clinical Isolates to CCR5 Inhibitors

Author

Visseaux, Benoit, Charpentier, Charlotte, Hurtado-Nedelec, Margarita, Storto, Alexandre, Antoine, Romain, Peytavin, Gilles, Damond, Florence, Matheron, Sophie, Brun-Vézinet, Françoise, and Descamps, Diane

Abstract

ABSTRACTHIV-2 is naturally resistant to nonnucleoside reverse transcriptase inhibitors, to a fusion inhibitor, and to some of the protease inhibitors. Maraviroc is the first drug of the new anti-CCR5 drug class and is effective only on CCR5-tropic (R5) HIV-1. No previous studies concerning HIV-2 susceptibility to maraviroc have been reported yet. We developed a phenotypic maraviroc susceptibility test using a peripheral blood mononuclear cell (PBMC) model. We analyzed the maraviroc susceptibility of 13 R5 HIV-2, 2 X4R5 (dual) HIV-2, and 2 CXCR4-tropic (X4) HIV-2 clinical isolates. We also tested, with the same protocol, 1 X4 HIV-1 and 4 R5 HIV-1 clinical isolates. For the R5 HIV-2 clinical isolates, the 50% effective concentration (EC50) for maraviroc was 0.80 nM (interquartile range [IQR], 0.48 to 1.39 nM), similar to that observed for the R5 HIV-1 isolates. The median maximum percentage of inhibition in the R5 HIV-2 isolates was 93% (IQR, 84 to 98%), similar to that observed in the R5 HIV-1 isolates. As expected, both X4 HIV-1 and HIV-2 were highly resistant to maraviroc. Our study showed for the first time that maraviroc is active in vitroagainst R5 HIV-2. The new tools we developed will allow identification of HIV-2-infected patients eligible for CCR5 inhibitor use and management of virological failure when receiving a maraviroc-based regimen.

Published

2011

164. Hot Spots of Integrase Genotypic Changes Leading to HIV-2 Resistance to Raltegravir

Author

Charpentier, Charlotte, Roquebert, Bénédicte, Delelis, Olivier, Larrouy, Lucile, Matheron, Sophie, Tubiana, Roland, Karmochkine, Marina, Duval, Xavier, Chêne, Geneviève, Storto, Alexandre, Collin, Gilles, Bénard, Antoine, Damond, Florence, Mouscadet, Jean-François, Brun-Vézinet, Françoise, and Descamps, Diane

Abstract

ABSTRACTWe studied seven heavily pretreated HIV-2-infected patients exhibiting a virological failure while receiving a salvage raltegravir-containing regimen. At the time of virological failure, different resistance genetic pathways were observed: T97A-Y143C, Q148K, Q148R, G140S-Q148R, E92Q-Y143R-N155H, and T97A-N155H. Thus, despite a 40% difference in integrase genes between HIV-1 and HIV-2, the genetic pathways leading to raltegravir resistance are similar.

Published

2010

165. Transmitted drug resistance in French HIV-2-infected patients

Author

Charpentier, Charlotte, Visseaux, Benoit, Bénard, Antoine, Peytavin, Gilles, Damond, Florence, Roy, Céline, Taieb, Audrey, Chêne, Geneviève, Matheron, Sophie, Brun-Vézinet, Francoise, Descamps, Diane, Michelet, Christian, Laboratoire de Virologie, Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-AP-HP - Hôpital Bichat - Claude Bernard [Paris], Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP), Epidémiologie et Biostatistique [Bordeaux], Université Bordeaux Segalen - Bordeaux 2-Institut de Santé Publique, d'Épidémiologie et de Développement (ISPED)-Institut National de la Santé et de la Recherche Médicale (INSERM), Service de pharmacie, Service des maladies infectieuses et tropicales, Université Paris Diderot - Paris 7 (UPD7)-AP-HP - Hôpital Bichat - Claude Bernard [Paris], Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP), Institut de recherche en santé, environnement et travail (Irset), Université d'Angers (UA)-Université de Rennes 1 (UR1), Université de Rennes (UNIV-RENNES)-Université de Rennes (UNIV-RENNES)-École des Hautes Études en Santé Publique [EHESP] (EHESP)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Structure Fédérative de Recherche en Biologie et Santé de Rennes ( Biosit : Biologie - Santé - Innovation Technologique ), ANRS CO5 HIV-2 Cohort, Assistance publique - Hôpitaux de Paris (AP-HP) (APHP)-AP-HP - Hôpital Bichat - Claude Bernard [Paris], Assistance publique - Hôpitaux de Paris (AP-HP) (APHP)-AP-HP - Hôpital Bichat - Claude Bernard [Paris]-Université Paris Diderot - Paris 7 (UPD7), Assistance publique - Hôpitaux de Paris (AP-HP) (AP-HP)-Université Paris Diderot - Paris 7 (UPD7), and Université d'Angers (UA)-Université de Rennes (UR)-École des Hautes Études en Santé Publique [EHESP] (EHESP)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Structure Fédérative de Recherche en Biologie et Santé de Rennes ( Biosit : Biologie - Santé - Innovation Technologique )

Subjects

medicine.medical_treatment, Immunology, Human immunodeficiency virus (HIV), HIV Infections, Drug resistance, medicine.disease_cause, 03 medical and health sciences, 0302 clinical medicine, Drug Resistance, Viral, Prevalence, medicine, Humans, Immunology and Allergy, 030212 general & internal medicine, 0303 health sciences, Protease, 030306 microbiology, business.industry, Survey research, HIV Protease Inhibitors, Virology, Reverse transcriptase, Confidence interval, 3. Good health, Infectious Diseases, [SDV.TOX]Life Sciences [q-bio]/Toxicology, HIV-2, Cohort, RNA, Viral, Reverse Transcriptase Inhibitors, France, business

Abstract

International audience; We report the first transmitted drug resistance survey study in HIV-2-infected patients living in France. The prevalence of transmitted drug resistance was 5.0% (95% confidence interval, 0.1-9.9) with mutations detected only in protease, not in reverse transcriptase. In this series, 10% of patients displayed X4/dual-mixed viruses. These findings classified the rate of transmitted drug resistance in the HIV-2 French Cohort as low prevalence.

166. Immunovirological Response to Triple Nucleotide Reverse-Transcriptase Inhibitors and Ritonavir-Boosted Protease Inhibitors in Treatment-Naive HIV-2-Infected Patients: The ACHIEV2E Collaboration Study Group

Author

Benard, Antoine, van Sighem, Ard, Taieb, Audrey, Valadas, Emilia, Ruelle, Jean, Soriano, Vicente, Calmy, Alexandra, Balotta, Claudia, Damond, Florence, Brun-Vezinet, Françoise, Chene, Geneviève, Matheron, Sophie, Benard, Antoine, van Sighem, Ard, Taieb, Audrey, Valadas, Emilia, Ruelle, Jean, Soriano, Vicente, Calmy, Alexandra, Balotta, Claudia, Damond, Florence, Brun-Vezinet, Françoise, Chene, Geneviève, and Matheron, Sophie

Abstract

This European inter-cohort collaboration shows poorer immunological and virological responses with triple NRTI compared to PI/r-containing cART in treatment-naïve HIV-2-infected patients, regardless of baseline CD4 cell count. PI/r-containing cART should be recommended as first-line antiretroviral regimens in HIV-2 infection

167. Response to Hønge et al.: Comment on Gautheret-Dejean et al.: Performance of Rapid Tests for Discrimination Between HIV-1 and/or HIV-2 Infections.

Author

Gautheret‐Dejean, Agnès, Bocobza, Jonathan, Brunet, Sylvie, Damond, Florence, Plantier, Jean‐Christophe, and Barin, Francis

Published

2016

168. Salvage Therapy Including Foscarnet and Ibalizumab for Multidrug-Resistant Human Immunodeficiency Virus Type 2 Infection.

Author

Bachelard, Antoine, Hingrat, Quentin Le, Ferré, Valentine-Marie, Lê, Minh, Peytavin, Gilles, Damond, Florence, Charpentier, Charlotte, Goudot, Guillemette Fremont, Bouille, Jeanne Goupil de, Lariven, Sylvie, Delobel, Pierre, Yazdanpanah, Yazdan, Descamps, Diane, Matheron, Sophie, Ghosn, Jade, and group, for the ANRS CO05 VIH-2 cohort study

Subjects

*THERAPEUTIC use of monoclonal antibodies, *KIDNEY function tests, *PATIENT compliance, *VIRAL load, *RESEARCH funding, *SALVAGE therapy, *SCIENTIFIC observation, *DRUG resistance in microorganisms, *CD4 lymphocyte count, *MULTIDRUG resistance, *HIV infections, *TREATMENT effectiveness, *BLOOD cell count, *DESCRIPTIVE statistics, *ANTIVIRAL agents, *COMBINED modality therapy, *RESEARCH, *BLOOD plasma, *ANTI-HIV agents, *DRUGS, *GENETIC mutation, *TIME, *LIVER function tests, *DRUG tolerance

Abstract

We evaluated Ibalizumab (IBA)-containing standardized optimized salvage regimen (with or without a 4-week foscarnet induction) in individuals harboring multidrug-resistant human immunodeficiency virus type 2 (HIV-2). Nine were included; 2 achieved virological suppression after foscarnet induction with a sustained suppression at Week 24 after IBA initiation, and an additional individual at Week 24 after Ibalizumab initiation. [ABSTRACT FROM AUTHOR]

Published

2024

169. Future of Antiretroviral Drugs and Evolution of HIV-1 Drug Resistance.

Author

Charpentier, Charlotte, Le Hingrat, Quentin, Ferré, Valentine Marie, Damond, Florence, and Descamps, Diane

Subjects

*DRUG resistance, *HIV, *DIAGNOSIS of HIV infections, *VIRAL load, *MIDDLE-income countries, *RALTEGRAVIR, *ANTIRETROVIRAL agents, *DRUG resistance in cancer cells

Abstract

Highly active antiretroviral (ARV) therapy has been used for many years, but the use in low- and middle-income countries of antiretroviral drugs with low genetic barrier to resistance, combined with limited availability of viral load testing, has led to higher rates of acquired drug resistance, sustaining the rate of transmitted drug resistance. Here, we describe the evolution of ARV drugs with the ongoing development of injectable long-acting forms and the requirements regarding all new ARV drugs (i.e., no transmitted drug resistance, no cross-resistance and high genetic barrier to resistance). Then, we report the evolution of both transmitted and acquired resistance regarding new ARV drugs. The WHO has set very ambitious but motivating goals for HIV testing, treatment and viral suppression, aiming to achieve rates of 95% for all three by 2025. Reaching these goals requires a wide implementation and use of close virological monitoring in LMICs. [ABSTRACT FROM AUTHOR]

Published

2023

170. Highly sensitive plasma RNA quantification by real-time PCR in HIV-2 group A and group B infection.

Author

Delarue, Séverine, Didier, Emmanuelle, Damond, Florence, Ponscarme, Diane, Brengle-Pesce, Karen, Resche-Rigon, Matthieu, Vray, Muriel, Gueudin, Marie, and Simon, François

Subjects

*RNA viruses, *POLYMERASE chain reaction, *HIV-positive persons, *BIOLOGICAL assay, *DIAGNOSIS of HIV infections, *VIRUS-induced enzymes

Abstract

Abstract: Plasma HIV-2 viral load has been reported as predictive of AIDS in HIV-2 infected patient but the lack of sensitivity of the current HIV2 viral load assay is a limitation for the monitoring of the HIV-2-infected patients. Objective: To validate a new quantification assay based on a synthetic HIV-2 RNA transcript and real-time PCR with primers and probes selected in the LTR region, together with high-performance reagents and a protective RNA carrier. Study design: We quantified 23 HIV-2 group A and B supernatants and 58 plasma samples with our TAQMAN-PCR assay and compared the results to those of our previously published in a real time reference PCR performed onto Light Cycler technology, the LC-PCR with a detection of 2.0log10 copies/ml. Results: The performance of TAQMAN-PCR was significantly improved, yielding a detection limit of 17 RNA copies/ml. There was a major difference (1–5log10 copies/ml) between LC-PCR and TAQMAN-PCR values for HIV-2 group B supernatants. Twenty-six of 27 plasma samples with levels higher than 2.0log10 copies/ml in LC-PCR were positive by TAQMAN-PCR. Ten of the 31 plasma samples below the LC-PCR detection limit were quantifiable with the TAQMAN-PCR. Conclusions: The new primers and probe in the LTR region can circumvent HIV-2 diversity, making our method suitable for use in HIV-2 group B-infected patients. Use of a high-performance RT enzyme and RNA carrier protection contributed to improving the detection limit. This study confirms that plasma viral load is lower than 17copies/ml in a large number of HIV-2-infected patients. [Copyright &y& Elsevier]

Published

2013

171. Association of Soluble CD14 and Inflammatory Biomarkers With HIV-2 Disease Progression.

Author

Thiébaut, Rodolphe, Charpentier, Charlotte, Damond, Florence, Taieb, Audrey, Antoine, Romain, Capeau, Jacqueline, Chêne, Geneviève, Collin, Gilles, Matheron, Sophie, Descamps, Diane, and Brun-Vézinet, Françoise

Subjects

*CD14 antigen, *INFLAMMATION, *BIOMARKERS, *HIV, *LONGITUDINAL method, *VIRUS diseases, *C-reactive protein

Abstract

In this longitudinal study including 384 plasma samples from 71 patients infected with human immunodeficiency virus type 2, higher levels of soluble CD14 were correlated with lower CD4 cell count and were independently associated with disease progression.Background. Human immunodeficiency virus type 2 (HIV-2) infection is characterized by a slower progression than HIV type 1. It is not known whether markers of inflammation such as high-sensitivity C-reactive protein (hsCRP), interleukin 6 (IL-6), and soluble CD14 (sCD14) may predict disease progression among HIV-2 patients.Methods. We performed longitudinal retrospective analysis using 384 samples from 71 patients included in the HIV-2 French cohort ANRS CO5 and followed for a median of 8 years. Baseline was the time of the first available measurement. Disease progression was defined by the occurrence of death, Centers for Disease Control and Prevention B/C stage HIV-related event, drop in CD4 <350 cells/µL, and HIV-2 RNA detection. Cox regression models and mixed models were used for statistical analyses.Results. At baseline, 75% of patients were asymptomatic, 34% were treated; 30% had detectable HIV-2 RNA load, and median CD4 cell count was 415/µL. The 3 biomarkers were positively related to each other. In adjusted analyses, sCD14 was the main factor explaining variation of hsCRP and IL-6 (P < .001). Lower CD4, older age, and advanced clinical stage were associated with higher sCD14. The biomarkers were correlated with HIV-2 RNA in unadjusted analyses only. Patients with baseline levels above either the median values (hsCRP = 1.38 mg/L; IL-6 = 1.97 pg/mL) or the highest quartile (sCD14 = 1.74 µg/mL) had a higher risk of disease progression (all P < .003). After adjustment for CD4 count, only sCD14 remained significantly associated with disease progression (hazard ratio, 3.59; P = .004).Conclusions. In this cohort of HIV-2–infected patients, sCD14 represents a better predictive biomarker of disease progression than hsCRP or IL-6, independent of CD4. [ABSTRACT FROM AUTHOR]

Published

2012

172. Plasma RNA Quantification and HIV-1 Divergent Strains.

Author

Plantier, Jean-Christophe, Gueudin, Marie, Damond, Florence, Braun, Joséphine, Mauclère, Philippe, and Simon, François

Subjects

*HIV, *RNA, *VIRUS-induced immunosuppression, *AIDS, *IMMUNOSUPPRESSION, *HIV infections

Abstract

Evaluates the new Light Cycler (LCx) HIV RNA Quantitative viral load assay kit developed for quantification of HIV-1 group M subtypes a to G and group O variants. Improvements in the quantification of non-B subtypes; Comparison of the LCx assay with the Cobas Amplicor HIV-1 monitor v1.5 assay with 133 plasma samples of the different subtypes; Nature of discordances between four HIV genotypic resistance interpretation algorithms according to drugs.

Published

2003

173. Nosocomial transmission clusters and lineage diversity characterized by SARS-CoV-2 genomes from two large hospitals in Paris, France, in 2020.

Author

Leducq, Valentin, Jary, Aude, Bridier-Nahmias, Antoine, Daniel, Lena, Zafilaza, Karen, Damond, Florence, Goldstein, Valérie, Duval, Audrey, Blanquart, François, Calvez, Vincent, Descamps, Diane, Marcelin, Anne-Geneviève, and Visseaux, Benoit

Subjects

*COVID-19, *MEDICAL personnel, *SARS-CoV-2, *PUBLIC health, *HOSPITALS, *NUCLEOTIDE sequencing

Abstract

France went through three deadly epidemic waves due to the severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), causing major public health and socioeconomic issues. We proposed to study the course of the pandemic along 2020 from the outlook of two major Parisian hospitals earliest involved in the fight against COVID-19. Genome sequencing and phylogenetic analysis were performed on samples from patients and health care workers (HCWs) from Bichat (BCB) and Pitié-Salpêtrière (PSL) hospitals. A tree-based phylogenetic clustering method and epidemiological data were used to investigate suspected nosocomial transmission clusters. Clades 20A, 20B and 20C were prevalent during the spring wave and, following summer, clades 20A.EU2 and 20E.EU1 emerged and took over. Phylogenetic clustering identified 57 potential transmission clusters. Epidemiological connections between participants were found for 17 of these, with a higher proportion of HCWs. The joint presence of HCWs and patients suggest viral contaminations between these two groups. We provide an enhanced overview of SARS-CoV-2 phylogenetic changes over 2020 in the Paris area, one of the regions with highest incidence in France. Despite the low genetic diversity displayed by the SARS-CoV-2, we showed that phylogenetic analysis, along with comprehensive epidemiological data, helps to identify and investigate healthcare associated clusters. [ABSTRACT FROM AUTHOR]

Published

2022

174. Evaluation of SARS-CoV-2 in semen, seminal plasma, and spermatozoa pellet of COVID-19 patients in the acute stage of infection.

Author

Delaroche, Lucie, Bertine, Mélanie, Oger, Pierre, Descamps, Diane, Damond, Florence, Genauzeau, Emmanuel, Meicler, Philippe, Le Hingrat, Quentin, Lamazou, Frédéric, Gschwind, Rémi, Ruppé, Etienne, and Visseaux, Benoit

Subjects

*COVID-19, *SARS-CoV-2, *SPERMATOZOA, *BACTERIAL DNA, *SEMEN, *SEMEN analysis, *ACUTE diseases

Abstract

To date, there is limited information about the presence of SARS-CoV-2 in semen especially in the acute phase of the infection. While available data from cohort studies including a total of 342 patients in the acute or recovery phase of the infection are reassuring, one study mentioned detecting virus in the semen of 6/38 COVID-19 patients. Here we assessed SARS-CoV-2 presence in the semen of COVID-19 positive patients in the acute stage of infection, within 24 hours of the positive nasopharyngeal swabs. Semen, seminal plasma and spermatozoa pellet were screened for SARS-CoV-2 and manual or airborne contamination during semen sampling. Among the 32 COVID-19 volunteers, the median interval from the onset of symptoms to semen collection was 4 days [IQR: 0–8]. Only one presented positive SARS-CoV-2 PCR in semen and seminal plasma fractions, although the spermatozoa pellet was negative. Viral cultures were all negative. We observed slightly higher concentrations of bacterial DNA in the SARS-CoV-2 positive specimen than in all negative samples. The bacteria identified neither confirm nor rule out contamination by oropharyngeal secretions during collection. SARS-CoV-2 was rarely present in semen during the acute phase of the disease. This very rare situation could be connected to oral or manual contamination during semen collection. The possible presence of SARS-CoV-2 in semen calls for nasopharyngeal viral testing and strict hygiene protocols during semen collection before assisted reproductive attempts. [ABSTRACT FROM AUTHOR]

Published

2021

175. Performance of 30 commercial SARS-CoV-2 serology assays in testing symptomatic COVID-19 patients.

Author

Vauloup-Fellous, Christelle, Maylin, Sarah, Périllaud-Dubois, Claire, Brichler, Ségolène, Alloui, Chakib, Gordien, Emmanuel, Rameix-Welti, Marie-Anne, Gault, Elyanne, Moreau, Frédérique, Fourati, Slim, Challine, Dominique, Pawlotsky, Jean-Michel, Houhou-Fidouh, Nadhira, Damond, Florence, Mackiewicz, Vincent, Charpentier, Charlotte, Méritet, Jean-François, Rozenberg, Flore, Podglajen, Isabelle, and Marot, Stéphane

Subjects

*COVID-19, *SARS-CoV-2, *COVID-19 testing, *COVID-19 pandemic, *SEROLOGY

Abstract

We report evaluation of 30 assays' (17 rapid tests (RDTs) and 13 automated/manual ELISA/CLIA assay (IAs)) clinical performances with 2594 sera collected from symptomatic patients with positive SARS-CoV-2 rRT-PCR on a respiratory sample, and 1996 pre-epidemic serum samples expected to be negative. Only 4 RDT and 3 IAs fitted both specificity (> 98%) and sensitivity (> 90%) criteria according to French recommendations. Serology may offer valuable information during COVID-19 pandemic, but inconsistent performances observed among the 30 commercial assays evaluated, which underlines the importance of independent evaluation before clinical implementation. [ABSTRACT FROM AUTHOR]

Published

2021

176. Performance evaluation of two SARS-CoV-2 IgG/IgM rapid tests (Covid-Presto and NG-Test) and one IgG automated immunoassay (Abbott).

Author

Charpentier, Charlotte, Ichou, Houria, Damond, Florence, Bouvet, Elisabeth, Chaix, Marie-Laure, Ferré, Valentine, Delaugerre, Constance, Mahjoub, Nadia, Larrouy, Lucile, Le Hingrat, Quentin, Visseaux, Benoit, Mackiewicz, Vincent, Descamps, Diane, and Fidouh-Houhou, Nadhira

Subjects

*SARS-CoV-2, *IMMUNOASSAY, *IMMUNOGLOBULIN M, *COVID-19, *COVID-19 testing, *CROSS reactions (Immunology)

Abstract

The aim of this study was to assess the analytical performances, sensitivity and specificity, of two rapid tests (Covid- Presto® test rapid Covid-19 IgG/IgM and NG-Test® IgM-IgG COVID-19) and one automated immunoassay (Abbott SARS-CoV-2 IgG) for detecting anti- SARS-CoV-2 antibodies. This study was performed with: (i) a positive panel constituted of 88 SARS-CoV-2 specimens collected from patients with a positive SARS-CoV-2 RT-PCR, and (ii) a negative panel of 120 serum samples, all collected before November 2019, including 64 samples with a cross-reactivity panel. Sensitivity of Covid-Presto® test for IgM and IgG was 78.4% and 92.0%, respectively. Sensitivity of NG-Test® for IgM and IgG was 96.6% and 94.9%, respectively. Sensitivity of Abbott IgG assay was 96.5% showing an excellent agreement with the two rapid tests (κ = 0.947 and κ = 0.936 for NGTest ® and Covid-Presto® test, respectively). An excellent agreement was also observed between the two rapid tests (κ = 0.937). Specificity for IgM was 100% and 86.5% for Covid-Presto® test and NG-Test®, respectively. Specificity for IgG was 92.0%, 94.9% and 96.5% for Covid-Presto®, NGTest ®, and Abbott, respectively. Most of the false positive results observed with NG-Test® resulted from samples containing malarial antibodies. In conclusion, performances of these 2 rapid tests are very good and comparable to those obtained with automated immunoassay, except for IgM specificity with the NG-Test®. Thus, isolated IgM should be cautiously interpreted due to the possible false-positive reactions with this test. Finally, before their large use, the rapid tests must be reliably evaluated with adequate and large panel including early seroconversion and possible cross-reactive samples. [ABSTRACT FROM AUTHOR]

Published

2020

177. Genetic variability of Long Terminal Repeat region between HIV-2 groups impacts transcriptional activity.

Author

Le Hingrat, Quentin, Visseaux, Benoit, Bertine, Mélanie, Chauveau, Lise, Schwartz, Olivier, Collin, Fidéline, Damond, Florence, Matheron, Sophie, Descamps, Diane, and Charpentier, Charlotte

Subjects

*BINDING sites, *VIRAL proteins, *VIRUS reactivation, *T cells, *TRANSCRIPTION factors

Abstract

HIV-2 Long Terminal Repeat (LTR) region contains several transcription factors (TF) binding sites. Efficient LTR transactivation by cellular TF and viral proteins is crucial for HIV-2 reactivation and viral production. Proviral LTR sequences of 66 antiretroviral-naïve HIV-2-infected patients included in the French ANRS HIV-2 CO5 cohort were sequenced. A high genetic variability within HIV-2 LTR was observed, notably in the U3 sub-region, the sub-region encompassing most known TF binding sites. Genetic variability was significantly higher in HIV-2 group B than in group A viruses. Notably, all group B viruses lacked the peri-ETS binding site and 4 group B sequences (11 %) also presented a complete deletion of the first Sp1 binding site. The lack of a peri-ETS binding site was responsible for a lowered transcriptional activity in activated T lymphocytes, while deletion of the first Sp1 binding site lowered basal or Tat-mediated transcriptional activities, depending on the cell line. Interestingly, HIV-2 cellular reservoir was less frequently quantifiable in patients infected by group B viruses and, when quantifiable, reservoirs were significantly smaller than in patients infected by group A viruses. Our findings suggest that mutations observed in vivo in HIV-2 LTR sequences are associated with differences in transcriptional activity and may explain the low cellular reservoir in patients infected by HIV-2 group B viruses, providing a new insight into the reduced pathogenicity of HIV-2 infection. [ABSTRACT FROM AUTHOR]

Published

2020

178. Multicenter comparison of the new Cobas 6800 system with Cobas Ampliprep/Cobas TaqMan and Abbott RealTime for the quantification of HIV, HBV and HCV viral load.

Author

Wirden, Marc, Larrouy, Lucile, Mahjoub, Nadia, Todesco, Eve, Damond, Florence, Delagreverie, Heloise, Akhavan, Sepideh, Charpentier, Charlotte, Chaix, Marie-Laure, Descamps, Diane, Calvez, Vincent, and Marcelin, Anne-Genevieve

Subjects

*VIRAL load, *VIREMIA, *RNA, *HIV, *HEPATITIS B virus, *HEPATITIS C virus

Abstract

Background The new Roche Cobas 6800 platform (C6800) has been recently introduced for viral load (VL) measurement. Objectives Comparing C6800 to Cobas Ampliprep/Cobas TaqMan v2.0 (CAP/CTM) for the quantification of HIV, HBV and HCV viremia, and to the Abbott RealTime assay (ABB) for HCV quantification. Study design We analysed 121 samples for HBV, and 139 for HIV-1 including 2 groupO and 137 group M viruses (36.5% subtype B, 27.0% CRF02_AG, 22.6% from other clades, and 14% subtype not available). For the 100 HCV samples compared with CAP/CTM, 42% were genotype 1 and 17% were genotype 4. For the 68 HCV samples compared with ABB, 52.9% were genotype 1 and 22.1% were genotype 4. Results C6800 results correlated well with those of CAP/CTM for all three viruses (R 2 : 0.97–0.99). However, C6800 can yield different viraemia results: higher for HIV (mean difference: +0.11 log 10 copies/mL, p < 0.0001), and lower for HBV (mean difference:-0.11 log 10 IU/mL, p < 0.0001). Differences exceeded 0.5 log 10 for 6.5% of HIV-1 samples and 7.4% of HBV samples. For HCV quantification, C6800 gave mostly lower values than the other assays towards the bottom of the range, and higher values in the upper part of the range, especially in comparisons with ABB, for which 28% of differences exceeded 0.5 log 10 IU/mL. No particular HCV genotype was identified as responsible for these differences. Conclusion Overall, the comparison tests between C6800 and CAP/CTM systems are satisfactory for the three viruses. Frequent discrepancies were observed between C6800 and ABB for HCV. [ABSTRACT FROM AUTHOR]

Published

2017

179. Women infected with human immunodeficiency virus type 1 have poorer assisted reproduction outcomes: a case-control study.

Author

Stora, Camille, Epelboin, Sylvie, Devouche, Emmanuel, Matheron, Sophie, Epelboin, Loïc, Yazbeck, Chadi, Damond, Florence, Longuet, Pascale, Dzineku, Frederick, Rajguru, Mandovi, Delaroche, Lucie, Mandelbrot, Laurent, Luton, Dominique, and Patrat, Catherine

Subjects

*HIV-positive women, *REPRODUCTIVE technology, *HEALTH outcome assessment, *HIGHLY active antiretroviral therapy, *INTRACYTOPLASMIC sperm injection

Abstract

Objective: To compare the efficacy of assisted reproductive technology (ART) in women infected with human immunodeficiency virus type 1 (HIV-1) versus HIV-negative controls.Design: Retrospective case-control study.Setting: University hospital ART unit.Patient(s): Eighty-two women infected with HIV-1 and 82 women as seronegative controls.Intervention(s): Ovarian stimulation, oocytes retrieval, standard in vitro fertilization (IVF) or intracytoplasmic sperm injection, embryo transfer.Main Outcome Measure(s): Clinical pregnancies and live-birth rates.Result(s): After oocyte retrieval, all women infected with HIV-1 infected were matched 1:1 to HIV-negative controls according to the following criteria: date of ART attempt, age, parity, main cause of infertility, ART technique, and rank of attempt. Only the first IVF cycle during the study period was considered for each couple. We found no statistically significant differences between the two groups for ovarian stimulation data, fertilization rate, or average number of embryos transferred. The clinical pregnancy rate per transfer was statistically significantly lower for the cases compared with the controls (12% vs. 32%), as were the implantation rate (10% vs. 21%) and the live-birth rate (7% vs. 19%).Conclusion(s): In one of the largest studies to pair six factors that influence the results of ART, HIV infection in women was associated with poorer outcomes after ART. These results suggest that women with controlled HIV-1-infection should be counseled not to delay ART in cases of self-insemination failure or other causes of infertility. Fertility preservation by vitrification of oocytes in women whose pregnancy should be delayed may be an important future consideration. [ABSTRACT FROM AUTHOR]

Published

2016

180. Dolutegravir in HIV-2-Infected Patients With Resistant Virus to First-line Integrase Inhibitors From the French Named Patient Program.

Author

Descamps, Diane, Peytavin, Gilles, Visseaux, Benoit, Tubiana, Roland, Damond, Florence, Campa, Pauline, Charpentier, Charlotte, Khuong-Josses, Marie-Aude, Duvivier, Claudine, Karmochkine, Marina, Lukiana, Tuna, and Matheron, Sophie

Subjects

*HIV infections, *THERAPEUTICS, *INTEGRASE inhibitors, *ANTIVIRAL agents, *DRUG resistance in microorganisms, *PUBLIC health, *REVERSE transcriptase inhibitors

Abstract

Background. Dolutegravir has shown in vitro activity against human immunodeficiency virus type 2 (HIV-2). We report safety and efficacy data of regimens containing dolutegravir (50 mg twice daily) in antiretroviral-experienced, HIV-2-infected patients. Methods. HIV-2-infected patients experiencing virological failure to raltegravir received dolutegravir with optimized background antiretroviral combinations within the French Named Patient Program (NPP). Plasma HIV-2 RNA (pVL) was assessed at time of dolutegravir initiation (baseline), month 3, and month 6. Antiretroviral trough plasma concentrations (C12h) were determined using liquid chromatography coupled with tandem mass spectrometry. Results. Thirteen HIV-2-infected-patients, with a median duration of 15 years' infection and given 16 previous antiretroviral regimens, were included in NPP. Median follow-up was 9 months (min-max, 3-15 months). Median baseline pVL and CD4 cell count were 9544 copies/mL (inter quartile range [IQR], 3096-23 120 copies/mL) and 100 cells/μL (IQR, 77-171 cells/μL), respectively. Available integrase genotypic resistance patterns were Y143C/G/H/ R (n = 5), Q148R/K (n = 2), and N155H (n = 4). Optimized background antiretroviral regimens conferring a genotypic sensitivity score ⩽2 in 10 patients included nucleoside reverse transcriptase inhibitors associated with darunavir/ritonavir (n = 12), saquinavir/ritonavir (n = 2), and maraviroc (n = 3). At months 3 and 6, pVL was undetectable in 6 of 13 and 4 of 12 patients, respectively, and median CD4 count was 161 (101-188) cells/μL and 167 (135-1353) cells/μL, respectively. Median dolutegravir C12h was 4086 (1756-5717 ng/mL) ng/mL in 9 patients. No serious events were notified except 1 death from progressive multifocal leukoencephalopathy at month 4. Conclusions. Optimized dolutegravir-containing antiretroviral regimens supported by good plasma exposure provide a substantial initial efficacy rate for salvage therapy in heavily antiretroviral-experienced HIV-2-infected patients with virus harboring resistance to first-generation integrase inhibitors. Larger numbers of patients and longer follow-up are needed to confirm these findings. [ABSTRACT FROM AUTHOR]

Published

2015

181. Persistent low-level HIV-1 RNA between 20 and 50 copies/mL in antiretroviral-treated patients: associated factors and virological outcome.

Author

Charpentier, Charlotte, Landman, Roland, Laouénan, Cédric, Joly, Véronique, Hamet, Gwenn, Damond, Florence, Brun-Vézinet, Françoise, Mentré, France, Descamps, Diane, and Yeni, Patrick

Subjects

*HIV infections, *THERAPEUTICS, *VIREMIA, *ANTIRETROVIRAL agents, *VIRUS research, *VIRAL load

Abstract

Objectives The aim of our study was to identify factors associated with persistent low-level viraemia (LLV) in HIV-infected patients under suppressive antiretroviral therapy and to assess the virological outcome of these patients. Methods LLV was defined as at least two HIV-1 RNA values between 20 and 50 copies/mL during 1 year of follow-up. We compared patients with all values <20 copies/mL (LLV−) and patients with LLV (LLV+). The ‘blip ratio’ was defined as (number of HIV-1 RNA values >50 copies/mL)/(number of HIV-1 RNA determinations) before study inclusion. Results Among the 656 patients included, 5.8% were in group LLV+. CDC stage B/C at study inclusion and a higher blip ratio before the study period were the only factors independently associated with LLV. During the 1 year follow-up, the proportion of patients experiencing virological failure was not different between the LLV− and LLV+ groups, and 40% of patients shifted from LLV+ to LLV− status. Conclusions LLV was infrequent in our series and the follow-up did not evidence a higher rate of virological failure than in fully suppressed patients. LLV seems to be a transient phenomenon that might be driven by residual ongoing viral replication and/or viral release and/or accuracy of viral load assay at lower values. [ABSTRACT FROM PUBLISHER]

Published

2012

182. Impact of freezing/thawing technique on sperm DNA integrity in HIV-1 patients.

Author

Frainais, Christophe, Vialard, François, Rougier, Nathalie, Aegerther, Philippe, Damond, Florence, Ayel, Jean-Philippe, Yazbeck, Chadi, Hazout, André, and Selva, Jacqueline

Subjects

*HIV-positive persons, *SPERMATOZOA, *AIDS prevention, *THAWING, *SEMEN

Abstract

According french legislation, sperm freezing/thawing procedures are used to prevent ART contaminations in couple with HIV-1 infected men. We determined sperm nuclear fragmentation rate before and after selection and freezing/thawing in HIV-1 14 patients. Two groups of patients were studied: 20 control patients with normal sperm (group 1) and without viral infection and 20 fertile treated HIV-1 patients (group 2). DNA fragmentation was evaluated using terminal uridine nick end labeling, before and after gradient selection, and after cryopreservation and thawing procedures. DNA fragmentation rates in fresh semen were increased in HIV patients (6.38% vs 3.39%) ( p < 0.05) compared with control patients. After sperm migration, fragmentation rates were significantly lower ( p < 0.0001) in the two groups compared with fresh sperm rates. After freezing/thawing, values were similar to those of fresh semen with an increased rate ( p < 0.01) for HIV-1 patients, with respectively 3.40% and 5.18% rates in control and infected patients. HIV-1-infected patients treated by antiretroviral therapy showed a significant increase in sperm DNA fragmentation in fresh sperm and also after freezing/thawing procedures, but these two fragmentation rates were not significantly different. So, freezing/thawing procedures do not seem to impair sperm DNA and preserve probability of conception for couples with HIV-1 infected men. [ABSTRACT FROM AUTHOR]

Published

2010

183. Evaluation of the Roche Cobas TaqMan and Abbott RealTime Extraction-Quantification Systems for HIV-1 Subtypes.

Author

Gueudin, Marie, Plantier, Jean Christophe, Lemée, Véronique, Schmitt, Marie Paule, Chartier, Loic, Bourlet, Thomas, Ruffault, Annick, Damond, Florence, Vray, Muriel, and Simon, Francois

Subjects

*EXTRACTION apparatus, *POLYMERASE chain reaction, *RNA, *CLINICAL trials, *NUCLEIC acids

Abstract

The article compares the Abbott Molecular RealTime to the Roche Diagnostics Cobas Taqman automated nucleic acid extraction and real-time polymerase chain reaction (PCR) amplification systems for their capacity to quantify HIV RNA of various subtypes. The Abbott RealTime system quantified all 29 HIV-1 group M supernatants. The limitation of the real-time PCR to span the entire diversity of HIV must be taken into account during treatment monitoring, resistance studies and clinical trials.

Published

2007

184. Interclade Neutralization and Enhancement of Human Immunodeficiency Virus Type 1 Identified by an Assay Using HeLa Cells Expressing Both CD4 Receptor and CXCR4/CCR5 Coreceptors.

Author

Barin, Francis, Brunet, Sylvie, Brand, Denys, Moog, Christiane, Peyre, Robert, Damond, Florence, Charneau, Pierre, and Barre-Sinoussi, Françoise

Subjects

*HIV, *HELA cells, *CD4 antigen, *SERUM, *CLONE cells, *GENES

Abstract

We report on the development and evaluation of a human immunodeficiency virus (HIV) neutralization assay that uses P4P cells, which are CD4[sup+]CXCR4[sup+]CCR5[sup+] HeLa cells that carry the lacZ gene under the control of the HIV-1 long terminal repeat. The results of the present study suggest that the P4P assay can be used for the extensive study of both neutralizing and enhancing activity in serum samples from HIV-1-infected patients and from vaccinated individuals. [ABSTRACT FROM AUTHOR]

Published

2004

185. Corrigendum to 'detection of SARS-CoV-2 N-antigen in blood during acute COVID-19 provides a sensitive new marker and new testing alternatives'.

Author

Le Hingrat, Quentin, Visseaux, Benoit, Laouenan, Cédric, Tubiana, Sarah, Bouadma, Lila, Yazdanpanah, Yazdan, Duval, Xavier, Burdet, Charles, Ichou, Houria, Damond, Florence, Bertine, Mélanie, Benmalek, Nabil, Choquet, Christophe, Timsit, Jean-François, Ghosn, Jade, Charpentier, Charlotte, Descamps, Diane, and Houhou-Fidouh, Nadhira

Subjects

*COVID-19, *SARS-CoV-2

Published

2021

186. Evaluation of three extraction-free SARS-CoV-2 RT-PCR assays: A feasible alternative approach with low technical requirements.

Author

Visseaux, Benoit, Collin, Gilles, Houhou-Fidouh, Nadhira, Le Hingrat, Quentin, Ferré, Valentine Marie, Damond, Florence, Ichou, Houria, Descamps, Diane, and Charpentier, Charlotte

Subjects

*SARS-CoV-2, *DIAGNOSTIC reagents & test kits, *VIRAL load, *EXTRACTION (Chemistry), *BOTTLENECKS (Manufacturing)

Abstract

• Assessment of performances of 3 extraction-free SARS-CoV-2 RT-PCR assays. • Good sensitivity of assays for samples with RT-PCR Ct< 30. • Good specificity for 2 of the 3 assays. • Extraction-free PCR: alternative valuable option, easier and less-reagent consuming. The worldwide demand for SARS-CoV-2 RT-PCR testing resulted in a shortage of diagnostic kits. RNA extraction step constitutes a major bottleneck to perform diagnostic. The aim of this study was to assess performances of different extraction-free SARS-CoV-2 RT-PCR assays compared to a reference RT-PCR assay. The panel of evaluation consisted of 94 samples: 69 positive and 25 negative for SARS-CoV-2 by reference RT-PCR. Three extraction-free RT-PCR assays were assessed: (i) PrimeDirect® Probe RT-qPCR Mix (Takara), (ii) PrimeScript®RT-PCR (Takara), and (iii) SARS-CoV-2 SANSURE®BIOTECH Novel Coronavirus (Sansure). The overall sensitivity of PrimeDirect, PrimeScript and Sansure assays was 55.1 %, 69.6 % and 69.6 %, respectively. The sensitivity increased among samples with Ct < 30: 91.9 % (n = 34/37), 89.2 % (n = 33/37) and 94.6 % (n = 35/37) for PrimeDirect, PrimeScript and Sansure assays, respectively. The specificity was 88 %, 100 % and 100 % for PrimeDirect, PrimeScript and Sansure assays, respectively. In the present study, we showed a good sensitivity of extraction-free PCR assays, especially for high viral loads (Ct < 30), except PrimeDirect that displayed imperfect sensitivity and specificity. Despite a lower sensitivity for low viral loads, extraction-free reagents can provide a valuable option, cheaper, easier and less reagent consuming for SARS-CoV-2 diagnostic, especially in laboratory with lower experience and equipment for molecular assays. [ABSTRACT FROM AUTHOR]

Published

2021

187. The Human Immunodeficiency Virus Type 2 Vpx Protein Usurps the CUL4A-DDB1DCAF1 Ubiquitin Ligase To Overcome a Postentry Block in Macrophage Infection.

Author

Bergamaschi, Anna, Ayinde, Diana, David, Annie, Le Rouzic, Erwann, Morel, Marina, Collin, Gilles, Descamps, Diane, Damond, Florence, Brun-Vezinet, Françoise, Nisole, Sebastien, Margottin-Goguet, Florence, Pancino, Gianfranco, and Transy, Catherine

Subjects

*HIV, *UBIQUITIN, *LIGASES, *MACROPHAGES, *IMMUNOSUPPRESSION, *VIRAL replication

Abstract

The human immunodeficiency virus (HIV) and simian immunodeficiency virus (SIV) genomes encode several auxiliary proteins that have increasingly shown their importance in the virus-host relationship. One of these proteins, Vpx, is unique to the HIV-2/SIVsm lineage and is critical for viral replication in macrophages. The functional basis for this requirement, as well as the Vpx mode of action, has remained unexplained, and it is all the more enigmatic that HIV type 1 (HIV-1), which has no Vpx counterpart, can infect macrophages. Here, we underscore DCAF1 as a critical host effector of Vpx in its ability to mediate infection and long-term replication of HIV-2 in human macrophages. Vpx assembles with the CUL4A-DDB1 ubiquitin ligase through DCAF1 recruitment. Precluding Vpx present in the incoming virions from recruiting DCAF1 in target macrophages leads to a postentry block characterized by defective accumulation of HIV-2 reverse transcripts. In addition, Vpx from SIVsm functionally complements Vpx-defective HIV-2 in a DCAF1-binding-dependent manner. Altogether, our data point to a mechanism in which Vpx diverts the Cul4A-DDB1DCAF1 ligase to inactivate an evolutionarily conserved factor, which restricts macrophage infection by HIV-2 and closely related simian viruses. [ABSTRACT FROM AUTHOR]

Published

2009

188. Rapid Selection of HIV-2 Capsid Mutations in Salvage Therapy with Lenacapavir-Containing Regimen.

Author

Montrouge T, Bertine M, Peytavin G, Saint Joannis T, Bachelard A, De Truchis P, Lariven S, Morlat P, Pouderoux C, Damond F, Sayre N, Tubiana R, Valin N, Charpentier C, Descamps D, Ghosn J, and Le Hingrat Q

Abstract

Lenacapavir is the first capsid inhibitor, its use is currently approved for multidrug resistant HIV-1 infection. We report that, despite an initial efficacy of a LEN-containing regimen in patients with multi-drug resistant HIV-2 viruses, virological suppression was not achieved after a year and most patients selected capsid drug-resistance associated mutations., (© The Author(s) 2024. Published by Oxford University Press on behalf of Infectious Diseases Society of America. All rights reserved. For commercial re-use, please contact reprints@oup.com for reprints and translation rights for reprints. All other permissions can be obtained through our RightsLink service via the Permissions link on the article page on our site—for further information please contact journals.permissions@oup.com.)

Published

2024

189. Immuno-virological and Clinical Follow-up of Persons Living With HIV-2 (PWHIV-2) Receiving Bictegravir/Emtricitabine/Tenofovir Alafenamide Fumarate (BIC/FTC/TAF): A Retrospective Study.

Author

Joly V, Ferre VM, Le Hingrat Q, Peytavin G, Cresta M, Charpentier C, Digumber M, Damond F, Yazdanpanah Y, Matheron S, Descamps D, and Ghosn J

Abstract

This retrospective study evaluated Bictegravir/FTC/TAF in 24 PWHIV, 5 naive and 19 pretreated. After a median follow-up of 37.5 months, all PWHIV-2 had a plasma viral load < 40 copies/mL. Median CD4 count increased significantly from 580 to 625 cells/mm3, suggesting the effectiveness of Bictegravir/FTC/TAF to treat HIV-2 infection., (© The Author(s) 2024. Published by Oxford University Press on behalf of Infectious Diseases Society of America. All rights reserved. For commercial re-use, please contact reprints@oup.com for reprints and translation rights for reprints. All other permissions can be obtained through our RightsLink service via the Permissions link on the article page on our site—for further information please contact journals.permissions@oup.com.)

Published

2024

190. Pharmaco-virological outcomes and genotypic resistance profiles among children and adolescents receiving a DTG-based regimen in Togo.

Author

Konu YR, Takassi E, Peytavin G, Dapam N, Damond F, Oumarou WA, Zaidi M, Franco-Yusti AM, Dagnra CA, Le Hingrat Q, Coppée R, Descamps D, Diallo FBT, Ekouevi DK, and Charpentier C

Abstract

Background: Few data are available on the real-world efficacy of receiving tenofovir-lamivudine-dolutegravir (DTG) as HIV treatment, particularly among young people in West Africa. Here, we evaluated pharmaco-virological outcomes and resistance profiles among Togolese children and adolescents., Methods: A cross-sectional study was conducted in Lomé, Togo, enrolling antiretroviral-treated people with HIV aged from 18 months to 24 years. Plasma HIV-1 viral load and antiretroviral concentrations were measured. Next-Generation Sequencing (NGS) of protease, Reverse Transcriptase (RT) and integrase was performed on all samples with viral load >200 c/mL. Drug resistance mutations (DRMs) were identified and interpreted using the ANRS-MIE algorithm., Results: 264 participants were enrolled (median age=17 years), 226 received a DTG-based regimen for a median of 20.5 months. Among them, virological suppression at the 200 c/mL threshold in 80.0% of the participants. Plasma DTG concentrations were adequate (i.e., >640 ng/mL), suboptimal and below the limit of quantification in 74.1%, 6.7% and 19.2% of participants receiving DTG, respectively. Overall, viruses resistant to any of Nucleoside RT Inhibitors, Non-NRTIs, and protease inhibitors were found in 52%, 66% and 1.6% of participants, respectively. A major integrase inhibitor DRM was observed in 9.4% (n=3/32, R263K, E138A-G140A-Q148R, and N155H) of participants with a viral load >200 c/mL., Conclusions: These first findings in such a large series of adolescents in a low-income country, showed a good virological response of 80% and the presence of an integrase DRM in 9.4% of the virological failures, supporting the need to monitor DTG drug resistance to reduce the risk of resistance acquisition., (© The Author(s) 2024. Published by Oxford University Press on behalf of Infectious Diseases Society of America. All rights reserved. For commercial re-use, please contact reprints@oup.com for reprints and translation rights for reprints. All other permissions can be obtained through our RightsLink service via the Permissions link on the article page on our site—for further information please contact journals.permissions@oup.com.)

Published

2024

191. Are Confirmatory Assays Reliable for HIV-1/HIV-2 Infection Differentiation? A Multicenter Study.

Author

Guiraud V, Bocobza J, Desmonet M, Damond F, Plantier JC, Moreau G, Wirden M, Stefic K, Barin F, and Gautheret-Dejean A

Subjects

Humans, HIV-2 genetics, Sensitivity and Specificity, HIV Antibodies, HIV-1, HIV Infections diagnosis, HIV Seropositivity

Abstract

Immunoblots remain the gold standard for HIV-1/HIV-2 infection confirmation. However, their ability to differentiate HIV-1 from HIV-2 infection on an antigenically diversified HIV-1 and HIV-2 panel remain uncommon. We performed a multicenter study on 116 serum samples accounting for most of the diversity of HIV-1 (9 different subtypes in group M, 17 circulating recombinant forms (CRFs), and 3 group O) and HIV-2 (groups A and B), evaluating seven confirmatory assays (six commercially available assays and one in-house assay) with genotyping as the reference. The assays were INNO-LIA HIV I/II score, HIV-2 blot 1.2, HIV blot 2.2, New Lav blot I and II, Geenius, and an in-house serotyping enzyme-linked immunosorbent assay (ELISA). Among the HIV-1 samples, INNO-LIA, HIV blot 2.2, New Lav blot I, Geenius, and serotyping had comparable high sensitivities, from 98% to 100%, whereas HIV-2 blot 1.2 and New Lav blot II had high rates of "undetermined" results (85% and 95%, respectively). HIV-2 blot 1.2 and New Lav blot II misclassified 7% and 5% of HIV-1 samples as HIV-2, respectively, and HIV-2 blot 1.2 had an 8% false-negative rate. Among the HIV-2 samples, INNO-LIA, New Lav blot II, HIV-2 blot 1.2, and serotyping had high sensitivities, from 96% to 100%. HIV blot 2.2 misclassified 17% of HIV-2 samples as HIV-1/HIV-2 dual infections. New Lav blot I misclassified 19% of HIV-2 samples as HIV-1 with a high (81%) undetermined rate, and Geenius misclassified 2% as HIV-1 and 7% as untypeable HIV positive. For HIV-1/HIV-2 dual infection, the results were less sensitive, with at most 87.5% for INNO-LIA and Geenius and 75% for HIV blot 2.2 and serotyping. Overall, confirmatory assays remain useful for most cases, with the exception of HIV-1/HIV-2 dual-infection suspicion., Competing Interests: The authors declare no conflict of interest.

Published

2023

192. Molecular confirmation of HIV-1 and HIV-2 coinfections among initially serologically dually-reactive samples from patients living in West Africa.

Author

Tchounga BK, Bertine M, Damond F, Ferré VM, Inwoley A, Boni SP, Moisan A, Plantier JC, Descamps D, Ekouevi DK, and Charpentier C

Subjects

Humans, Cross-Sectional Studies, HIV Antibodies, Cote d'Ivoire epidemiology, HIV-2 genetics, Coinfection diagnosis, HIV Infections complications, HIV Infections diagnosis, HIV Seropositivity, HIV-1 genetics

Abstract

Objectives: This study aimed to confirm the co-infection with HIV-1 and HIV-2, among West African patients using in-house HIV type/group enzyme-immuno assays and molecular diagnosis., Design: A cross-sectional survey was conducted from April 2016 to October 2017 in the biggest HIV clinics of Côte d'Ivoire and Burkina Faso., Method: A first serological confirmation was done in the referral laboratory using an in-house, indirect immuno-enzymatic essay allowing the qualitative detection of both HIV-1 and HIV-2 antibodies. In order to separately detect anti-HIV-1 and anti-HIV-2 antibodies, a type/group specific enzyme-immuno assay (HIV-GSEIA) was used. To confirm the co-infections, HIV-1 and HIV-2 DNA-qualitative PCR assays were performed., Results: A total of 91 patients were enrolled in the study and provided blood sample for HIV type confirmatory testing including 13 (14.3%) HIV-2 mono-reactive and 78 (85.7%) HIV-1/HIV-2 dually-reactive based on the HIV testing National Algorithms. The first serological ELISA confirmatory test performed showed that 80 (78.9%) of the 91 participants were dually-reactive. The HIV-GSEIA performed on these 80 serum samples retrieve one 61 HIV-1/HIV-2 dually-reactive samples. HIV-1 and HIV-2 DNA PCR were performed on 54 of the 61 HIV-1/HIV-2 dually-reactive samples and 46 out of 61 (75.4%) samples were found HIV-1/HIV-2 coinfected., Conclusion: The contribution of type/group specific enzyme-immuno assay to accurately identify HIV-1/HIV-2 coinfections remain suboptimal, emphasizing the need for molecular diagnosis platforms in West Africa, to avail HIV DNA PCR test for the confirmation of HIV-1/HIV-2 co-infections., Competing Interests: The authors have declared that no competing interests exist., (Copyright: © 2023 Tchounga et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.)

Published

2023

193. Ibalizumab shows in-vitro activity against group A and group B HIV-2 clinical isolates.

Author

Le Hingrat Q, Collin G, Bachelard A, Ghosn J, Chalal S, Pacanowski J, Peytavin G, Weinheimer S, Marsolais C, Damond F, Matheron S, Charpentier C, and Descamps D

Subjects

Antibodies, Monoclonal adverse effects, HIV-2, Humans, Leukocytes, Mononuclear, Anti-HIV Agents therapeutic use, HIV Infections drug therapy, HIV-1

Abstract

Objective: Treatment of multidrug-resistant HIV-2 is an emerging issue, because of the rapid selection of mutations at time of virological failure and the low number of antiretrovirals active on HIV-2. The aim of this study was to determine the susceptibility of HIV-2 primary isolates to ibalizumab, a long-acting monoclonal antibody that binds to CD4 that is approved for the treatment of MDR HIV-1., Methods: In-vitro phenotypic susceptibility of 16 HIV-2 primary isolates was measured using a modified version of the ANRS peripheral blood mononuclear cells (PBMC) assay. Susceptibility to ibalizumab was assessed through 50% inhibitory concentrations and maximum percentage inhibitions (MPI), and gp105 was sequenced to look for determinants of reduced susceptibility., Results: Ibalizumab inhibited viral replication of all 16 isolates, with a median IC 50 value of 0.027 μg/ml (range = 0.001-0.506 μg/ml), and a median MPI of 93%. Although two isolates presented higher IC 50 (above 0.1 μg/ml), they did not exhibit a loss of potential N-linked glycosylation sites in V5 loop, as reported in HIV-1 strains with reduced susceptibility. However, both presented shorter V1 and V2 loops than the HIV-2 reference strain., Conclusion: Ibalizumab inhibits HIV-2 replication, with IC 50 and MPI in the range of those reported for HIV-1. These in vitro data support the use of ibalizumab in patients with MDR HIV-2, in combination with an optimized background regimen., (Copyright © 2022 Wolters Kluwer Health, Inc. All rights reserved.)

Published

2022

194. Alpha (B.1.1.7) and Delta (B.1.617.2 - AY.40) SARS-CoV-2 variants present strong neutralization decay at M4 post-vaccination and a faster replication rates than D614G (B.1) lineage.

Author

Lebourgeois S, Menidjel R, Chenane HR, Ferré VM, Collin G, Damond F, Coppée R, Yazdanpanah Y, Timsit JF, Houhou-Fidouh N, Descamps D, Charpentier C, and Visseaux B

Subjects

Antibodies, Neutralizing, Humans, Neutralization Tests, Vaccination, COVID-19 prevention & control, SARS-CoV-2 genetics

Abstract

Competing Interests: Declaration of Competing Interest The authors have no relevant competing interest to disclose in relation to this work.

Published

2022

195. Lymphoma in HIV-2-infected patients in combination antiretroviral therapy era.

Author

Ronchetti AM, Matheron S, Galicier L, Damond F, Mahjoub N, Chaghil N, Meignin V, Mechaï F, Simon F, Oksenhendler E, and Gérard L

Subjects

Antineoplastic Combined Chemotherapy Protocols, HIV-2, Humans, Prospective Studies, HIV Infections complications, HIV Infections drug therapy, Lymphoma, AIDS-Related drug therapy, Lymphoma, AIDS-Related epidemiology

Abstract

Objective: To describe lymphoma in HIV-2-infected patients and compare their characteristics with lymphoma in HIV-1-infected patients., Design: Ancillary analysis from a single center prospective cohort of HIV-lymphoma., Methods: We report on 16 patients with HIV-2-lymphoma diagnosed after 1996 and included in a prospective cohort of HIV lymphoma. Five additional HIV-2-infected patients coinfected with HIV-1 or/and HTLV-I (6 lymphomas) are separately reported. The incidence of lymphoma in HIV-2-infected patients was evaluated in the French multicentric HIV-2 cohort., Results: Incidence of lymphoma in the French HIV-2 cohort was estimated as 0.6/1000 patient-years. In our series, the median CD4+ cell count was 166 × 106/l at the time of lymphoma diagnosis and 50% of patients had undetectable plasma HIV-2-RNA. Lymphomas were non-Hodgkin lymphoma (n = 12) and classical Hodgkin lymphoma (n = 4). Similarly to HIV-1-lymphoma, clinical presentation was aggressive in most cases. All but one patient received intensive chemotherapy. Complete remission was achieved in 13 cases and 1 patient relapsed. The overall survival was not statistically different from that observed in patients with HIV-1 lymphoma. The six additional lymphomas observed in five HIV-2-infected patients coinfected with HIV-1 or/and HTLV-I presented with similar clinical presentation but worse prognosis., Conclusion: Despite the lower pathogenicity of HIV-2, the risk of developing lymphoma seems to be close to that observed in HIV-1 population with similar lymphoma characteristics. Compared with HIV-1, HIV-2-infected patients developed lymphoma later in their life but at a similar CD4+ cell count level., (Copyright © 2021 Wolters Kluwer Health, Inc. All rights reserved.)

Published

2021

196. HIV-2 diversity displays two clades within group A with distinct geographical distribution and evolution.

Author

Visseaux B, Bertine M, Le Hingrat Q, Ferré V, Charpentier C, Collin F, Damond F, Matheron S, Hué S, and Descamps D

Abstract

Genetic diversity of HIV-2 groups A and B has not yet been fully described, especially in a few Western Africa countries such as Ivory-Coast or Mali. We collected 444 pol , 152 vif , 129 env , and 74 LTR sequences from patients of the French ANRS CO5 HIV-2 cohort completed by 221 pol , 18 vif , 377 env , and 63 LTR unique sequences from public databases. We performed phylogenetic reconstructions and revealed two distinct lineages within HIV-2 group A, herein called A1 and A2, presenting non-negligible genetic distances and distinct geographic distributions as A1 is related to coastal Western African countries and A2 to inland Western countries. Estimated early diversification times for groups A and B in human populations were 1940 [95% higher probability densitiy: 1935-53] and 1961 [1952-70]. A1 experienced an early diversification in 1942 [1937-58] with two distinct early epidemics in Guinea-Bissau or Senegal, raising the possibility of group A emergence in those countries from an initial introduction from Ivory-Coast to Senegal, two former French colonies. Changes in effective population sizes over time revealed that A1 exponentially grew concomitantly to Guinea-Bissau independence war, but both A2 and B lineages experienced a latter growth, starting during the 80s economic crisis. This large HIV-2 genetic analysis provides the existence of two distinct subtypes within group A and new data about HIV-2 early spreading patterns and recent epidemiologic evolution for which data are scarce outside Guinea-Bissau., (© The Author(s) 2021. Published by Oxford University Press.)

Published

2021

197. SARS-CoV-2 IGM and IGG rapid serologic test for the diagnosis of COVID-19 in the emergency department.

Author

Cancella de Abreu M, Choquet C, Petit H, Bouzid D, Damond F, Marot S, Ferre VM, Burrel S, Boutolleau D, Houdou-Fidouh N, Marcelin AG, Descamps D, and Hausfater P

Subjects

Betacoronavirus, COVID-19, COVID-19 Testing, Clinical Laboratory Techniques, Emergency Service, Hospital, Humans, Immunoglobulin G, Immunoglobulin M, SARS-CoV-2, Serologic Tests, Coronavirus Infections diagnosis, Coronavirus Infections epidemiology, Pandemics, Pneumonia, Viral epidemiology

Published

2020

198. Interlaboratory quality control of total HIV-1 DNA load measurement for multicenter reservoir studies.

Author

Gantner P, Mélard A, Damond F, Delaugerre C, Dina J, Gueudin M, Maillard A, Sauné K, Rodallec A, Tuaillon E, Plantier JC, Rouzioux C, and Avettand-Fenoel V

Subjects

Clinical Laboratory Techniques methods, Disease Reservoirs virology, HIV-1 genetics, Humans, Intersectoral Collaboration, RNA, Viral blood, Real-Time Polymerase Chain Reaction methods, Reproducibility of Results, Clinical Laboratory Techniques standards, DNA, Viral analysis, HIV-1 isolation & purification, HIV-1 physiology, Quality Control, Real-Time Polymerase Chain Reaction standards, Viral Load standards

Abstract

Background: Viral reservoirs represent an important barrier to HIV cure. Accurate markers of HIV reservoirs are needed to develop multicenter studies. The aim of this multicenter quality control (QC) was to evaluate the inter-laboratory reproducibility of total HIV-1-DNA quantification., Methods: Ten laboratories of the ANRS-AC11 working group participated by quantifying HIV-DNA with a real-time qPCR assay (Biocentric) in four samples (QCMD)., Results: Good reproducibility was found between laboratories (standard deviation ≤ 0.2 log 10 copies/10 6 PBMC) for the three positive QC that were correctly classified by each laboratory (QC1

Published

2017

199. Hiv-2 molecular epidemiology.

Author

Visseaux B, Damond F, Matheron S, Descamps D, and Charpentier C

Subjects

Africa, Western epidemiology, Genetic Variation, Humans, Molecular Epidemiology, HIV Infections epidemiology, HIV Infections virology, HIV-2 classification, HIV-2 genetics

Abstract

The Simian Immunodeficiency Virus of sooty mangabeys (SIVsmm) has been revealed to be at the origin of Human Immunodeficiency Virus type 2 (HIV-2) in humans, firstly detected from two Portuguese patients in 1986. HIV-2 is mainly restricted to West Africa where it infects up to 1 to 2 million people. HIV-2 is also present in Europe, mainly Portugal and France, India and United States of America. Two major HIV-2 groups, groups A and B, were generated by two independent transmission events involving infected sooty mangabeys from the Taï forest in Ivory Coast. Seven other HIV-2 groups have been described, but each has only been identified in one patient. To date, no subtypes have been formally described but some preliminary data suggest that HIV-2 group A may be divided in two distinct subtypes with distinct geographical origins. To date only two recombinant forms have been described: one circulating recombinant form (CRF01&#95;AB) and one unique recombinant form. In this review, we focused mainly on molecular data available and their insights about HIV-2 origins, diversity, drug resistance and global epidemiology., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

200. Evidence of Sexual Transmission of Zika Virus.

Author

D'Ortenzio E, Matheron S, Yazdanpanah Y, de Lamballerie X, Hubert B, Piorkowski G, Maquart M, Descamps D, Damond F, and Leparc-Goffart I

Subjects

Disease Transmission, Infectious, Humans, Middle Aged, Phylogeny, RNA, Viral analysis, RNA, Viral urine, Saliva virology, Semen virology, Urine virology, Young Adult, Zika Virus isolation & purification, Sexually Transmitted Diseases, Viral, Zika Virus genetics, Zika Virus Infection transmission

Published

2016