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1. Viral Kinetics and Resistance Development in Children Treated with Neuraminidase Inhibitors: The Influenza Resistance Information Study (IRIS)

Author

Roosenhoff, R. (Rueshandra), Reed, V. (Vaughan), Kenwright, A. (Andy), Schutten, M. (Martin), Boucher, C.A.B. (Charles), Monto, A. (Arnold), Clinch, B. (Barry), Kumar, D. (Deepali), Whitley, R. (Richard), Nguyen-Van-Tam, J.S. (Jonathan), Osterhaus, A.D.M.E. (Albert), Fouchier, R.A.M. (Ron), Fraaij, P.L.A. (Pieter), Roosenhoff, R. (Rueshandra), Reed, V. (Vaughan), Kenwright, A. (Andy), Schutten, M. (Martin), Boucher, C.A.B. (Charles), Monto, A. (Arnold), Clinch, B. (Barry), Kumar, D. (Deepali), Whitley, R. (Richard), Nguyen-Van-Tam, J.S. (Jonathan), Osterhaus, A.D.M.E. (Albert), Fouchier, R.A.M. (Ron), and Fraaij, P.L.A. (Pieter)

Abstract

BACKGROUND: We studied the effect of age, baseline viral load, vaccination status, antiviral therapy, and emergence of drug resistance on viral shedding in children infected with influenza A or B virus. ME

Published
2020
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2. Influenza A/H3N2 virus infection in immunocompromised ferrets and emergence of antiviral resistance

Author

Roosenhoff, R. (Rueshandra), Vries, E. (Erhard) van der, Linden, A. van der, Amerongen, G. (Geert) van, Stittelaar, K.J. (Koert), Smits, S.L. (Saskia), Schutten, M. (Martin), Fouchier, R.A.M. (Ron), Roosenhoff, R. (Rueshandra), Vries, E. (Erhard) van der, Linden, A. van der, Amerongen, G. (Geert) van, Stittelaar, K.J. (Koert), Smits, S.L. (Saskia), Schutten, M. (Martin), and Fouchier, R.A.M. (Ron)

Abstract

Influenza viruses can cause severe life threatening infections in high-risk patients, including young children, the elderly and patients with compromised immunity due to underlying medical conditions or immunosuppressive treatment. The impaired immunity of these patients causes prolonged virus infection and combined with antiviral treatment facilitates the emergence of viruses with resistance mutations. The diverse nature of their immune status makes them a challenging group to study the impact of influenza virus infection and the efficacy of antiviral therapy. Immunocompromised ferrets may represent a suitable animal model to assess influenza virus infection and antiviral treatment strategies in immunocompromised hosts. Here, ferrets were given a daily oral solution of mycophenolate mofetil, tacrolimus and prednisolone sodium phosphate to suppress their immune system. Groups of immunocompromised and immunocompetent ferrets were inoculated with an A/H3N2 influenza virus and were subsequently treated with Oseltamivir or left untreated. Quantitative real-time reverse transcription polymerase chain reaction (qRT-PCR) was performed on the throat and nose specimens to study virus replication during the course of infection. All immunocompromised ferrets had prolonged presence of viral RNA and a higher total amount of virus shedding compared to the immunocompetent ferrets. Although Oseltamivir reduced the total amount of virus shedding from the nose and throat of treated ferrets, it also resulted in the emergence of the neuraminidase R292K resistance substitution in all these animals, as determined by mutation specific RT-PCR and next-generation sequencing. No additional mutations that could be associated with the emergence of the R292K resistance mutation were detected. The immunocompromised ferret model can be used to study A/ H3N2 virus shedding and is a promising model to study new antiviral strategies and the emergence of antiviral resistance in immunocompromised host

Published
2018
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3. Five years of monitoring for the emergence of oseltamivir resistance in patients with influenza A infections in the Influenza Resistance Information Study

Author

Lina, B. (Bruno), Boucher, C. (Charles), Osterhaus, A. (Albert), Monto, A. (Arnold), Schutten, M. (Martin), Whitley, R.J. (Richard J.), Nguyen-Van-Tam, J.S. (Jonathan), Lina, B. (Bruno), Boucher, C. (Charles), Osterhaus, A. (Albert), Monto, A. (Arnold), Schutten, M. (Martin), Whitley, R.J. (Richard J.), and Nguyen-Van-Tam, J.S. (Jonathan)

Abstract

Background and objectives: The Influenza Resistance Information Study (IRIS) was initiated in 2008 to study the emergence of neuraminidase inhibitor (NAI) resistance and the clinical course of influenza in immunocompetent treated and untreated patients. Methods: Patients had throat/nose swabs collected on days 1, 3, 6 and 10 for analyses of influenza type, subtype and virus susceptibility to NAIs. RT-PCR-positive samples were cultured and tested for NAI resistance by specific RT-PCR and phenotypic testing. Scores for influenza symptoms were recorded on diary cards (Days 1-10). This study focuses on influenza A-infected cases only. Results: Among 3230 RT-PCR-positive patients, 2316 had influenza A of whom 1216 received oseltamivir monotherapy within 2 days of symptom onset (9 seasonal H1N1; 662 H3N2; 545 H1N1pdm2009). Except for 9 patients with naturally resistant seasonal H1N1 (2008/9), no resistance was detected in Day 1 samples. Emergence of resistance (post-Day 1) was detected in 43/1207 (3.56%) oseltamivir-treated influenza A-infected patients, with a higher frequency in 1- to 5-year-olds (11.8%) vs >5-year-olds (1.4%). All N1- and N2-resistant viruses had H275Y (n = 27) or R292K (n = 16) substitutions, respectively. For 43 patients, virus clearance was significantly delayed vs treated patients with susceptible viruses (8.1 vs 10.9 days; P < .0001), and 11 (23.2%) remained RT-PCR positive for influenza at Day 10. However, their symptoms resolved by Day 6 or earlier. Conclusions: Oseltamivir resistance was only detected during antiviral treatment, with the highest incidence occurring among 1- to 5-year-olds. Resistance delayed viral clearance, but had no impact on symptom resolution.

Published
2018
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4. Bivalent Vaccine Effectiveness Against Type-Specific HPV Positivity: Evidence for Cross-Protection Against Oncogenic Types among Dutch STI Clinic Visitors

Author

Woestenberg, PJ, King, AJ, van Benthem, BH, Donken, R, Leussink, S, van der Klis, FRM, de Melker, HE, van der Sande, M A J, Hoebe, CJ, Bogaards, JA, Adema, D, Buist-Arkema, R, Beerens, A, Luijt, D, Meijer, S, Schirm, J, Peeters, M, Rossen, JWA (John), Verbakel, H, Esch, PV, Verweij, J, Baltissen - van der Eijk, Annemiek, Huisman, RC, Kerkhof, C, Korff, MH, Schutten, M (Martin), Velzing, J, Verduyn-Lunel, F, Lakbiach, S, Rosmalen, PV, Schuurman, R (Rob), Abma, D, Adams, K, Bruisten, S, Linde, I, Oostvogel, P, Touwen, C, Vermeulen, W, Brink, A, Nelissen, J, Wolffs, P, Duijvendijk, N, Schneeberger, P, Poppel, MDV, Melchers, W, Poort, Y, Hooghiemstra, M, Huisman, H, Weel, J, Bosma, F, Geeraedts, F, Polman, I, Van Goor, P, Wolfhagen, M, De Mooij, C, Koolwijk, EV, Peters, M, Swanink, C, Tiemessen, R, Zwet, TV, Janssen, J, Pelsers, M, Waal, W, Aalfs, G, Kiewiet, J, Sanders, P, Buel-Bruins, HV, Bokhoven-Rombouts, CV, Cornelissen, P, Kersten, M, Ruitenbeek, CV, Molenaar, I, van Doorn, E, Masthoff, L, Pannekoek, E, Sigurdsson, V, Bugter, M, Götz, H, Linden, M, Mattijssen, M, Stam, J, Swaders, E, Groot, FD, Postma, F, Brouwers, E, Niekamp, A, Smit, M, Botraby, A, Bukasa, D, Haan, CD, Vliet, P, Taconis, T, Graas, MD, Hondelink, I, Kampman, C, Gelissen-Hansen, A, Koning, ID, Kruchten, HV, Pas, MVD, Fennema, H, Heijman, T, Hogewoning, A, Leeuwen, AV, Rooijen, MV, Neienhuijsen, F, Pelgrim, M, Woestenberg, PJ, King, AJ, van Benthem, BH, Donken, R, Leussink, S, van der Klis, FRM, de Melker, HE, van der Sande, M A J, Hoebe, CJ, Bogaards, JA, Adema, D, Buist-Arkema, R, Beerens, A, Luijt, D, Meijer, S, Schirm, J, Peeters, M, Rossen, JWA (John), Verbakel, H, Esch, PV, Verweij, J, Baltissen - van der Eijk, Annemiek, Huisman, RC, Kerkhof, C, Korff, MH, Schutten, M (Martin), Velzing, J, Verduyn-Lunel, F, Lakbiach, S, Rosmalen, PV, Schuurman, R (Rob), Abma, D, Adams, K, Bruisten, S, Linde, I, Oostvogel, P, Touwen, C, Vermeulen, W, Brink, A, Nelissen, J, Wolffs, P, Duijvendijk, N, Schneeberger, P, Poppel, MDV, Melchers, W, Poort, Y, Hooghiemstra, M, Huisman, H, Weel, J, Bosma, F, Geeraedts, F, Polman, I, Van Goor, P, Wolfhagen, M, De Mooij, C, Koolwijk, EV, Peters, M, Swanink, C, Tiemessen, R, Zwet, TV, Janssen, J, Pelsers, M, Waal, W, Aalfs, G, Kiewiet, J, Sanders, P, Buel-Bruins, HV, Bokhoven-Rombouts, CV, Cornelissen, P, Kersten, M, Ruitenbeek, CV, Molenaar, I, van Doorn, E, Masthoff, L, Pannekoek, E, Sigurdsson, V, Bugter, M, Götz, H, Linden, M, Mattijssen, M, Stam, J, Swaders, E, Groot, FD, Postma, F, Brouwers, E, Niekamp, A, Smit, M, Botraby, A, Bukasa, D, Haan, CD, Vliet, P, Taconis, T, Graas, MD, Hondelink, I, Kampman, C, Gelissen-Hansen, A, Koning, ID, Kruchten, HV, Pas, MVD, Fennema, H, Heijman, T, Hogewoning, A, Leeuwen, AV, Rooijen, MV, Neienhuijsen, F, and Pelgrim, M

Published
2018

5. Virological failure and drug resistance during first line anti-retroviral treatment in Indonesia

Author

Fibriani, Azzania, Wisaksana, R, Indrati, A, Hartantri, Y, van de Vijver, David, Schutten, M (Martin), Alisjahbana, B, Sudjana, P, Boucher, Charles, van Crevel, R, van de Ven, A, and Virology

Subjects
SDG 3 - Good Health and Well-being, Poverty-related infectious diseases [N4i 3], Poverty-related infectious diseases Infectious diseases and international health [N4i 3]
Abstract

Item does not contain fulltext The virological response and development of drug resistance during first-line anti-retroviral treatment (ART) were studied in Indonesia where the majority of patients infected with HIV have a history of injecting drug use, which is often linked with lower treatment adherence and development of drug-resistance. As many as 575 patients starting ART between September 2007 and March 2010 in Hasan Sadikin Hospital Bandung were followed prospectively. Clinical and laboratory monitoring was performed every 6 months. Plasma samples with HIV-RNA >/=400 copies/ml were examined for drug resistance mutations. Most patients were male (72.3%), 59.7% had a history of injecting drug use, and the median CD4+ cells count before start of ART was 35 cells/mm(3) (IQR 10-104). From 438 HIV patients with HIV-RNA measurements, 40 (9.1%) subjects had HIV-RNA >/=400 copies/ml after 24 weeks (median follow-up 16 (IQR 8-25) months). Of these failing patients 16 (47%) subjects had drug resistance mutations, predominantly M184V (35.3%), Y181C (23.5%), K103N (11.7%), and TAMs (11.7%). A history of treatment discontinuation >/=1 month, reported by 5.3% (23) of patients, was strongly associated with virological failure (adjusted OR 12.64, 95% CI 4.51-35.41); and a history of injecting drug use was not (OR 0.75, 95% CI 0.38-1.46). This is the largest and most systematic evaluation of virological response to first line ART in Indonesia. Patients in this cohort responded well to first line ART, with low rates of virological failure and drug resistance. A history of injecting drug use should not be a reason to withhold ART in this setting. J. Med. Virol. 85:1394-1401, 2013. (c) 2013 Wiley Periodicals, Inc.

Published
2013

6. Discordant detection of avian influenza virus subtypes in time and space between poultry and wild birds; towards improvement of surveillance programs

Author

Verhagen, J.H. (Josanne), Lexmond, P. (Pascal), Vuong, O. (Oanh), Schutten, M. (Martin), Guldemeester, J., Osterhaus, A.D.M.E. (Albert), Elbers, A.R.W., Slaterus, R. (Roy), Hornman, M. (Menno), Koch, G. (Guus), Fouchier, R.A.M. (Ron), Verhagen, J.H. (Josanne), Lexmond, P. (Pascal), Vuong, O. (Oanh), Schutten, M. (Martin), Guldemeester, J., Osterhaus, A.D.M.E. (Albert), Elbers, A.R.W., Slaterus, R. (Roy), Hornman, M. (Menno), Koch, G. (Guus), and Fouchier, R.A.M. (Ron)

Abstract

Avian influenza viruses from wild birds can cause outbreaks in poultry, and occasionally infect humans upon exposure to infected poultry. Identification and characterization of viral reservoirs and transmission routes is important to develop strategies that prevent infection of poultry, and subsequently virus transmission between poultry holdings and to humans. Based on spatial, temporal and phylogenetic analyses of data generated as part of intense and large-scale influenza surveillance programs in wild birds and poultry in the Netherlands from 2006 to 2011, we demonstrate that LPAIV subtype distribution differed between wild birds and poultry, suggestive of host-range restrictions. LPAIV isolated from Dutch poultry were genetically most closely related to LPAIV isolated from wild birds in the Netherlands or occasionally elsewhere in Western Europe. However, a relatively long time interval was observed between the isolations of related viruses from wild birds and poultry. Spatial analyses provided evidence for mallards (Anas platyrhynchos) being more abundant near primary infected poultry farms. Detailed year-round investigation of virus prevalence and wild bird species distribution and behavior near poultry farms should be used to improve risk assessment in relation to avian influenza virus introduction and retarget avian influenza surveillance programs.

Published
2017
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7. Diagnostic performance of influenza viruses and RSV rapid antigen detection tests in children in tertiary care

Author

Moesker, F.M. (Fleur), Kampen, J.J.A. (Jeroen) van, Aron, G.I. (Georgina), Schutten, M. (Martin), Vijver, D.A.M.C. (David) van de, Koopmans D.V.M., M.P.G. (Marion), Osterhaus, A.D.M.E. (Albert), Fraaij, P.L.A. (Pieter), Moesker, F.M. (Fleur), Kampen, J.J.A. (Jeroen) van, Aron, G.I. (Georgina), Schutten, M. (Martin), Vijver, D.A.M.C. (David) van de, Koopmans D.V.M., M.P.G. (Marion), Osterhaus, A.D.M.E. (Albert), and Fraaij, P.L.A. (Pieter)

Abstract

__Background:__ Rapid antigen detection tests (RADTs) are increasingly used to detect influenza viruses and respiratory syncytial virus (RSV). However, their sensitivity and specificity are a matter of debate, challenging their clinical usefulness. __Objectives:__ Comparing diagnostic performances of BinaxNow Influenza AB® (BNI) and BinaxNow RSV® (BNR), to those of real-time reverse transcriptase PCR (RT-PCR), virus isolation and direct immunofluorescence (D-IF) in paediatric patients. __Study design:__ Between Novem

Published
2016
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9. Deep sequencing does not reveal additional transmitted mutations in patients diagnosed with HIV-1 variants with single nucleoside reverse transcriptase inhibitor resistance mutations

Author

Pingen, Marieke, Ende, Marchina, Wensing, AM, el Barzouhi, A, Simen, BB, Schutten, M (Martin), Boucher, Charles, Virology, and Internal Medicine

Subjects
SDG 3 - Good Health and Well-being
Abstract

Objectives The aim of the study was to gain more insight into the relationship between transmitted singletons found at HIV diagnosis by population sequencing and the possible presence of clinically relevant viral minorities containing additional resistance mutations. Methods We studied the viral quasispecies and therapy response in 10 individuals with transmitted single nucleoside reverse transcriptase inhibitor (NRTI)-related resistance mutations as detected by population sequencing. Results Ultra-deep pyrosequencing did not reveal additional drug-resistance mutations in nine of 10 patients. In these nine patients, no breakthrough with resistant viruses was observed despite the use of low genetic nonnucleoside reverse transcriptase inhibitor (NNRTI)-based regimens in the majority of patients. Conclusions These data suggest that viral minority variants containing additional resistance mutations may be rare in patients with transmitted NRTI singletons in the Netherlands. Larger studies are required to confirm these findings and to determine the therapeutic consequences.

Published
2013

10. European survey on laboratory preparedness, response and diagnostic capacity for crimean-congo haemorrhagic fever, 2012

Author

Fernandez-Garcia, M.D. (Maria Dolores), Negredo, A., Papa, A. (Anna), Donoso-Mantke, O., Niedrig, M., Zeller, H. (Hervé), Tenorio, A., Franco, L. (Leticia), Aberle, S.W. (Stephan), Esbroeck, M. (M.) van, Christova, I., Markotic, A. (Alemka), Kurolt, I.-C. (Ivan-Christian), Zelena, H. (Hana), Golovljova, I., Pannetier, D. (Delphine), Charrel, R. (Remi), Schmidt-Chanasit, J. (Jonas), Wölfel, R. (Roman), Capobianchi, M.R. (Maria Rosaria), Jakupi, X. (Xhevat), Storozenko, J. (Jelena), Griskevicius, A. (Algirdas), Bosevska, G. (Golubinka), Muscat, C. (Clive), Schutten, M. (Martin), Dudman, S.G. (Susanne Gjeruldsen), Alves, M.J. (M. João), Ceianu, C.S., Platonov, A. (Alexander), Bozovic, B. (Bojana), Klempa, B., Avsic, T. (Tatjana), Lundkvist, Å. (Åke), Cherpillod, P. (Pascal), Korukluoglu, G., Brown, D.W.G. (D. W G), Brooks, T. (Tim), Fernandez-Garcia, M.D. (Maria Dolores), Negredo, A., Papa, A. (Anna), Donoso-Mantke, O., Niedrig, M., Zeller, H. (Hervé), Tenorio, A., Franco, L. (Leticia), Aberle, S.W. (Stephan), Esbroeck, M. (M.) van, Christova, I., Markotic, A. (Alemka), Kurolt, I.-C. (Ivan-Christian), Zelena, H. (Hana), Golovljova, I., Pannetier, D. (Delphine), Charrel, R. (Remi), Schmidt-Chanasit, J. (Jonas), Wölfel, R. (Roman), Capobianchi, M.R. (Maria Rosaria), Jakupi, X. (Xhevat), Storozenko, J. (Jelena), Griskevicius, A. (Algirdas), Bosevska, G. (Golubinka), Muscat, C. (Clive), Schutten, M. (Martin), Dudman, S.G. (Susanne Gjeruldsen), Alves, M.J. (M. João), Ceianu, C.S., Platonov, A. (Alexander), Bozovic, B. (Bojana), Klempa, B., Avsic, T. (Tatjana), Lundkvist, Å. (Åke), Cherpillod, P. (Pascal), Korukluoglu, G., Brown, D.W.G. (D. W G), and Brooks, T. (Tim)

Abstract

Crimean-Congo haemorrhagic fever (CCHF) is an infectious viral disease that has (re-)emerged in the last decade in south-eastern Europe, and there is a risk for further geographical expansion to western Europe. Here we report the results of a survey covering 28 countries, conducted in 2012 among the member laboratories of the European Network for Diagnostics of 'Imported' Viral Diseases (ENIVD) to assess laboratory preparedness and response capacities for CCHF. The answers of 31 laboratories of the European region regarding CCHF case definition, training necessity, biosafety, quality assurance and diagnostic tests are presented. In addition, we identifie

Published
2014

12. Performance evaluation of the new Roche cobas AmpliPrep/cobas TaqMan HCV test, version 2.0, for detection and quantification of hepatitis C virus RNA

Author

Pas, S.D. (Suzan), Molenkamp, R. (Richard), Schinkel, J. (Janke), Rebers, S., Copra, C. (Cederick), Seven-Deniz, S., Thamke, D. (Diana), Knegt, R.J. (Robert) de, Haagmans, B.L. (Bart), Schutten, M. (Martin), Pas, S.D. (Suzan), Molenkamp, R. (Richard), Schinkel, J. (Janke), Rebers, S., Copra, C. (Cederick), Seven-Deniz, S., Thamke, D. (Diana), Knegt, R.J. (Robert) de, Haagmans, B.L. (Bart), and Schutten, M. (Martin)

Abstract

To evaluate the analytical performance and explore the clinical applicability of the new Roche cobas AmpliPrep/cobas TaqMan HCV test, v2.0 (CAP/CTM v2.0), a platform comparison was performed on panels and diagnostic samples with the Roche cobas AmpliPrep/cobas TaqMan HCV test (CAP/CTM v1.0), the Siemens Versant HCV RNA 3.0 branched DNA (bDNA) test, the Abbottm2000 RealTime HCV assay (Realtime assay), and the Siemens Versant HCV transcription-mediated amplification (TMA) test (TMA assay). The analytical performance of the CAP/CTM v2.0 on WHO and Acrometrix panels and clinical specimens of patients infected with HCV genotype 1, 2, 3, 4, 5, or 6 relative to that of the CAP/CTM v1.0 was significantly improved. In a qualitative comparison of the CAP/CTM v2.0 relative to the TMA assay on genotype 1 to 4 samples, the two tests proved to be almost equally sensitive. Response-guided therapy in one of five HCV genotype 4-infected patients previously tested with the CAP/CTM v1.0 would have significantly changed if tested with the CAP/CTM v2.0. In conclusion, the Roche CAP/CTM v2.0 has significantly better performance characteristics than the former CAP/CTM HCV v1.0 and the bDNA assay and performance characteristics comparable to those of the Realtime assay. Copyright

Published
2013
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13. Prolonged Influenza Virus Shedding and Emergence of Antiviral Resistance in Immunocompromised Patients and Ferrets

Author

Vries, E. (Erhard) van der, Stittelaar, K.J. (Koert), Amerongen, G. (Geert) van, Veldhuis Kroeze, E.J.B. (Edwin), Waal, L. (Leon) de, Fraaij, P.L.A. (Pieter), Schneider, P. (Petra), Luider, T.M. (Theo), Nagel, B.C. (Bart) van der, Koch, B.C.P. (Birgit), Vulto, A.G. (Arnold), Schutten, M. (Martin), Osterhaus, A.D.M.E. (Albert), Vries, E. (Erhard) van der, Stittelaar, K.J. (Koert), Amerongen, G. (Geert) van, Veldhuis Kroeze, E.J.B. (Edwin), Waal, L. (Leon) de, Fraaij, P.L.A. (Pieter), Schneider, P. (Petra), Luider, T.M. (Theo), Nagel, B.C. (Bart) van der, Koch, B.C.P. (Birgit), Vulto, A.G. (Arnold), Schutten, M. (Martin), and Osterhaus, A.D.M.E. (Albert)

Abstract

Immunocompromised individuals tend to suffer from influenza longer with more serious complications than otherwise healthy patients. Little is known about the impact of prolonged infection and the efficacy of antiviral therapy in these patients. Among all 189 influenza A virus infected immunocompromised patients admitted to ErasmusMC, 71 were hospitalized, since the start of the 2009 H1N1 pandemic. We identified 11 (15%) cases with prolonged 2009 pandemic virus replication (longer than 14 days), despite antiviral therapy. In 5 out of these 11 (45%) cases oseltamivir resistant H275Y viruses emerged. Given the inherent difficulties in studying antiviral efficacy in immunocompromised patients, we have infected immunocompromised ferrets with either wild-type, or oseltamivir-resistant (H275Y) 2009 pandemic virus. All ferrets showed prolonged virus shedding. In wild-type virus infected animals treated with oseltamivir, H275Y resistant variants emerged within a week after infection. Unexpectedly, oseltamivir therapy still proved to be partially protective in animals infected with resistant virus. Immunocompromised ferrets offer an attractive alternative to study efficacy of novel antiviral therapies.

Published
2013
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14. Carriage of Mycoplasma pneumoniae in the Upper Respiratory Tract of Symptomatic and Asymptomatic Children: An Observational Study

Author

Spuesens, E.B.M. (Emiel), Fraaij, P.L.A. (Pieter), Visser, E. (Eline), Hoogenboezem, T. (Theo), Hop, W.C.J. (Wim), Adrichem, L.N.A. (Léon) van, Weber, F. (Frank), Moll, H.A. (Henriëtte), Broekman, B. (Berth), Berger, M.Y. (Marjolein), Rijsoort-Vos, T. (Tineke) van, Belkum, A.F. (Alex) van, Schutten, M. (Martin), Pas, S.D. (Suzan), Osterhaus, A.D.M.E. (Albert), Hartwig, N.G. (Nico), Vink, C. (Cornelis), Rossum, A.M.C. (Annemarie) van, Spuesens, E.B.M. (Emiel), Fraaij, P.L.A. (Pieter), Visser, E. (Eline), Hoogenboezem, T. (Theo), Hop, W.C.J. (Wim), Adrichem, L.N.A. (Léon) van, Weber, F. (Frank), Moll, H.A. (Henriëtte), Broekman, B. (Berth), Berger, M.Y. (Marjolein), Rijsoort-Vos, T. (Tineke) van, Belkum, A.F. (Alex) van, Schutten, M. (Martin), Pas, S.D. (Suzan), Osterhaus, A.D.M.E. (Albert), Hartwig, N.G. (Nico), Vink, C. (Cornelis), and Rossum, A.M.C. (Annemarie) van

Abstract

Background:Mycoplasma pneumoniae is thought to be a common cause of respiratory tract infections (RTIs) in children. The diagnosis of M. pneumoniae RTIs currently relies on serological methods and/or the detection of bacterial DNA in the upper respiratory tract (URT). It is conceivable, however, that these diagnostic methods also yield positive results if M. pneumoniae is carried asymptomatically in the URT. Positive results from these tests may therefore not always be indicative of a symptomatic infection. The existence of asymptomatic carriage of M. pneumoniae has not been established. We hypothesized that asymptomatic carriage in children exists and investigated whether colonization and symptomatic infection could be differentiated by current diagnostic methods.Methods and Findings:This study was conducted at the Erasmus MC-Sophia Children's Hospital and the after-hours General Practitioners Cooperative in Rotterdam, The Netherlands. Asymptomatic children (n = 405) and children with RTI symptoms (n = 321) aged 3 mo to 16 y were enrolled in a cross-sectional study from July 1, 2008, to November 30, 2011. Clinical data, pharyngeal and nasopharyngeal specimens, and serum samples were collected. The primary objective was to differentiate between colonization and symptomatic infection with M. pneumoniae by current diagnostic methods, especially real-time PCR. M. pneumoniae DNA was detected in 21.2% (95% CI 17.2%-25.2%) of the asymptomatic children and in 16.2% (95% CI 12.2%-20.2%) of the symptomatic children (p = 0.11). Neither serology nor quantitative PCR nor culture differentiated asymptomatic carriage from infection. A total of 202 children were tested for the presence of other bacterial and viral pathogens. Two or more pathogens were found in 56% (63/112) of the asymptomatic children and in 55.5% (50/90) of the symptomatic children. Finally, longitudinal sampling showed persistence of M. pneumoniae in the URT for up to 4 mo. Fifteen of the 21 asymptomatic childre

Published
2013
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16. Avian influenza a virus in wild birds in highly urbanized areas

Author

Verhagen-Oldenampsen, J.H.E. (Judith), Munster, V.J. (Vincent), Majoor-Krakauer, D.F. (Danielle), Lexmond, P. (Pascal), Vuong, O. (Oanh), Stumpel, J.B.G. (Job ), Rimmelzwaan, G.F. (Guus), Osterhaus, A.D.M.E. (Albert), Schutten, M. (Martin), Slaterus, R. (Roy), Fouchier, R.A.M. (Ron), Verhagen-Oldenampsen, J.H.E. (Judith), Munster, V.J. (Vincent), Majoor-Krakauer, D.F. (Danielle), Lexmond, P. (Pascal), Vuong, O. (Oanh), Stumpel, J.B.G. (Job ), Rimmelzwaan, G.F. (Guus), Osterhaus, A.D.M.E. (Albert), Schutten, M. (Martin), Slaterus, R. (Roy), and Fouchier, R.A.M. (Ron)

Abstract

Avian influenza virus (AIV) surveillance studies in wild birds are usually conducted in rural areas and nature reserves. Less is known of avian influenza virus prevalence in wild birds located in densely populated urban areas, while these birds are more likely to be in close contact with humans. Influenza virus prevalence was investigated in 6059 wild birds sampled in cities in the Netherlands between 2006 and 2009, and compared with parallel AIV surveillance data from low urbanized areas in the Netherlands. Viral prevalence varied with the level of urbanization, with highest prevalence in low urbanized areas. Within cities virus was detected in 0.5% of birds, while seroprevalence exceeded 50%. Ring recoveries of urban wild birds sampled for virus detection demonstrated that most birds were sighted within the same city, while few were sighted in other cities or migrated up to 2659 km away from the sample location in the Netherlands. Here we show that urban birds were infected with AIVs and that urban birds were not separated completely from populations of long-distance migrants. The latter suggests that wild birds in cities may play a role in the introduction of AIVs into cities. Thus, urban bird populations should not be excluded as a human-animal interface for influenza viruses.

Published
2012
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17. H1N1 2009 Pandemic Influenza Virus: Resistance of the I223R Neuraminidase Mutant Explained by Kinetic and Structural Analysis

Author

Vries, E. (Erhard) van der, Collins, P.J. (Patrick ), Vachieri, S.G. (Sebastien), Xiong, X. (Xiaoli), Liu, J. (Jinhua), Walker, P.A. (Philip), Haire, L.F. (Lesley ), Hay, A.J. (Alan), Schutten, M. (Martin), Osterhaus, A.D.M.E. (Albert), Martin, S.R. (Steve ), Boucher, C.A.B. (Charles), Skehel, J.J. (John ), Gamblin, S.J. (Steve ), Vries, E. (Erhard) van der, Collins, P.J. (Patrick ), Vachieri, S.G. (Sebastien), Xiong, X. (Xiaoli), Liu, J. (Jinhua), Walker, P.A. (Philip), Haire, L.F. (Lesley ), Hay, A.J. (Alan), Schutten, M. (Martin), Osterhaus, A.D.M.E. (Albert), Martin, S.R. (Steve ), Boucher, C.A.B. (Charles), Skehel, J.J. (John ), and Gamblin, S.J. (Steve )

Abstract

Two classes of antiviral drugs, neuraminidase inhibitors and adamantanes, are approved for prophylaxis and therapy against influenza virus infections. A major concern is that antiviral resistant viruses emerge and spread in the human population. The 2009 pandemic H1N1 virus is already resistant to adamantanes. Recently, a novel neuraminidase inhibitor resistance mutation I223R was identified in the neuraminidase of this subtype. To understand the resistance mechanism of this mutation, the enzymatic properties of the I223R mutant, together with the most frequently observed resistance mutation, H275Y, and the double mutant I223R/H275Y were compared. Relative to wild type, KMvalues for MUNANA increased only 2-fold for the single I223R mutant and up to 8-fold for the double mutant. Oseltamivir inhibition constants (KI) increased 48-fold in the single I223R mutant and 7500-fold in the double mutant. In both cases the change was largely accounted for by an increased dissociation rate constant for oseltamivir, but the inhibition constants for zanamivir were less increased. We have used X-ray crystallography to better understand the effect of mutation I223R on drug binding. We find that there is shrinkage of a hydrophobic pocket in the active site as a result of the I223R change. Furthermore, R223 interacts with S247 which changes the rotamer it adopts and, consequently, binding of the pentoxyl substituent of oseltamivir is not as favorable as in the wild type. However, the polar glycerol substituent present in zanamivir, which mimics the natural substrate, is accommodated

Published
2012
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18. H1N1 2009 Pandemic Influenza Virus: Resistance of the I223R Neuraminidase Mutant Explained by Kinetic and Structural Analysis

Author

Vries, Erhard, Collins, PJ, Vachieri, SG, Xiong, XL, Liu, JF, Walker, PA, Haire, LF, Hay, AJ, Schutten, M (Martin), Osterhaus, Ab, Martin, SR, Boucher, Charles, Skehel, JJ, Gamblin, SJ, Vries, Erhard, Collins, PJ, Vachieri, SG, Xiong, XL, Liu, JF, Walker, PA, Haire, LF, Hay, AJ, Schutten, M (Martin), Osterhaus, Ab, Martin, SR, Boucher, Charles, Skehel, JJ, and Gamblin, SJ

Abstract

Two classes of antiviral drugs, neuraminidase inhibitors and adamantanes, are approved for prophylaxis and therapy against influenza virus infections. A major concern is that antiviral resistant viruses emerge and spread in the human population. The 2009 pandemic H1N1 virus is already resistant to adamantanes. Recently, a novel neuraminidase inhibitor resistance mutation I223R was identified in the neuraminidase of this subtype. To understand the resistance mechanism of this mutation, the enzymatic properties of the I223R mutant, together with the most frequently observed resistance mutation, H275Y, and the double mutant I223R/H275Y were compared. Relative to wild type, KM values for MUNANA increased only 2-fold for the single I223R mutant and up to 8-fold for the double mutant. Oseltamivir inhibition constants (K-I) increased 48-fold in the single I223R mutant and 7500-fold in the double mutant. In both cases the change was largely accounted for by an increased dissociation rate constant for oseltamivir, but the inhibition constants for zanamivir were less increased. We have used X-ray crystallography to better understand the effect of mutation I223R on drug binding. We find that there is shrinkage of a hydrophobic pocket in the active site as a result of the I223R change. Furthermore, R223 interacts with S247 which changes the rotamer it adopts and, consequently, binding of the pentoxyl substituent of oseltamivir is not as favorable as in the wild type. However, the polar glycerol substituent present in zanamivir, which mimics the natural substrate, is accommodated in the I223R mutant structure in a similar way to wild type, thus explaining the kinetic data. Our structural data also show that, in contrast to a recently reported structure, the active site of 2009 pandemic neuraminidase can adopt an open conformation.

Published
2012

19. Avian Influenza A Virus in Wild Birds in Highly Urbanized Areas

Author

Verhagen, Josanne, Munster, VJ (Vincent), Majoor, F, Lexmond, Pascal, Vuong, Oanh, Stumpel, JBG, Rimmelzwaan, Guus, Osterhaus, Ab, Schutten, M (Martin), Slaterus, R, Fouchier, Ron, Verhagen, Josanne, Munster, VJ (Vincent), Majoor, F, Lexmond, Pascal, Vuong, Oanh, Stumpel, JBG, Rimmelzwaan, Guus, Osterhaus, Ab, Schutten, M (Martin), Slaterus, R, and Fouchier, Ron

Abstract

Avian influenza virus (AIV) surveillance studies in wild birds are usually conducted in rural areas and nature reserves. Less is known of avian influenza virus prevalence in wild birds located in densely populated urban areas, while these birds are more likely to be in close contact with humans. Influenza virus prevalence was investigated in 6059 wild birds sampled in cities in the Netherlands between 2006 and 2009, and compared with parallel AIV surveillance data from low urbanized areas in the Netherlands. Viral prevalence varied with the level of urbanization, with highest prevalence in low urbanized areas. Within cities virus was detected in 0.5% of birds, while seroprevalence exceeded 50%. Ring recoveries of urban wild birds sampled for virus detection demonstrated that most birds were sighted within the same city, while few were sighted in other cities or migrated up to 2659 km away from the sample location in the Netherlands. Here we show that urban birds were infected with AIVs and that urban birds were not separated completely from populations of long-distance migrants. The latter suggests that wild birds in cities may play a role in the introduction of AIVs into cities. Thus, urban bird populations should not be excluded as a human-animal interface for influenza viruses.

Published
2012

20. Vaccination with Rev and Tat against AIDS?

Author

Osterhaus, Ab, Baalen, Carel, van Baalen, M, Schutten, M (Martin), Gruters, Rob, Girard, M., Dodet, B., and Virology

Subjects
SDG 3 - Good Health and Well-being
Published
2000

21. Multidrug resistant 2009 a/h1n1 influenza clinical isolate with a neuraminidase i223r mutation retains its virulence and transmissibility in ferrets

Author

Vries, E. (Erhard) van der, Veldhuis Kroeze, E.J.B. (Edwin), Stittelaar, K.J. (Koert), Linster, M. (Martin), Linden, A. van der, Schrauwen, E.J.A. (Eefje), Leijten, L.M.E. (Lonneke), Amerongen, G. (Geert) van, Schutten, M. (Martin), Kuiken, T. (Thijs), Osterhaus, A.D.M.E. (Albert), Fouchier, R.A.M. (Ron), Boucher, C.A.B. (Charles), Herfst, S. (Sander), Vries, E. (Erhard) van der, Veldhuis Kroeze, E.J.B. (Edwin), Stittelaar, K.J. (Koert), Linster, M. (Martin), Linden, A. van der, Schrauwen, E.J.A. (Eefje), Leijten, L.M.E. (Lonneke), Amerongen, G. (Geert) van, Schutten, M. (Martin), Kuiken, T. (Thijs), Osterhaus, A.D.M.E. (Albert), Fouchier, R.A.M. (Ron), Boucher, C.A.B. (Charles), and Herfst, S. (Sander)

Abstract

Only two classes of antiviral drugs, neuraminidase inhibitors and adamantanes, are approved for prophylaxis and therapy against influenza virus infections. A major concern is that influenza virus becomes resistant to these antiviral drugs and spreads in the human population. The 2009 pandemic A/H1N1 influenza virus is naturally resistant to adamantanes. Recently a novel neuraminidase I223R mutation was identified in an A/H1N1 virus showing cross-resistance to the neuraminidase inhibitors oseltamivir, zanamivir and peramivir. However, the ability of this virus to cause disease and spread in the human population is unknown. Therefore, this clinical isolate (NL/2631-R223) was compared with a well-characterized reference virus (NL/602). In vitro experiments showed that NL/2631-I223R replicated as well as NL/602 in MDCK cells. In a ferret pathogenesis model, body weight loss was similar in animals inoculated with NL/2631-R223 or NL/602. In addition, pulmonary lesions were similar at day 4 post inoculation. However, at day 7 post inoculation, NL/2631-R223 caused milder pulmonary lesions and degree of alveolitis than NL/602. This indicated that the mutant virus was less pathogenic. Both NL/2631-R223 and a recombinant virus with a single I223R change (recNL/602-I223R), transmitted among ferrets by aerosols, despite observed attenuation of recNL/602-I223R in vitro. In conclusion, the I223R mutated virus isolate has comparable replicative ability and transmissibility, but lower pathogenicity than the reference virus based on these in vivo studies. This implies that the 2009 pandemic influenza A/H1N1 virus subtype with an isoleucine to arginine change at position 223 in the neuraminidase has the potential to spread in the human population. It is important to be vigilant for this mutation in influenza surveillance and to continue efforts to increase the arsenal of antiviral drugs to combat influenza.

Published
2011
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22. Multidrug Resistant 2009 A/H1N1 Influenza Clinical Isolate with a Neuraminidase I223R Mutation Retains Its Virulence and Transmissibility in Ferrets

Author

Vries, Erhard, Veldhuis Kroeze, Edwin, Stittelaar, Koert, Linster, Martin, van der Linden, Anne, Schrauwen, Eefje, Leijten, Lonneke, Amerongen, Geert, Schutten, M (Martin), Kuiken, Thijs, Osterhaus, Ab, Fouchier, Ron, Boucher, Charles, Herfst, Sander, Vries, Erhard, Veldhuis Kroeze, Edwin, Stittelaar, Koert, Linster, Martin, van der Linden, Anne, Schrauwen, Eefje, Leijten, Lonneke, Amerongen, Geert, Schutten, M (Martin), Kuiken, Thijs, Osterhaus, Ab, Fouchier, Ron, Boucher, Charles, and Herfst, Sander

Abstract

Only two classes of antiviral drugs, neuraminidase inhibitors and adamantanes, are approved for prophylaxis and therapy against influenza virus infections. A major concern is that influenza virus becomes resistant to these antiviral drugs and spreads in the human population. The 2009 pandemic A/H1N1 influenza virus is naturally resistant to adamantanes. Recently a novel neuraminidase I223R mutation was identified in an A/H1N1 virus showing cross-resistance to the neuraminidase inhibitors oseltamivir, zanamivir and peramivir. However, the ability of this virus to cause disease and spread in the human population is unknown. Therefore, this clinical isolate (NL/2631-R223) was compared with a well-characterized reference virus (NL/602). In vitro experiments showed that NL/2631-I223R replicated as well as NL/602 in MDCK cells. In a ferret pathogenesis model, body weight loss was similar in animals inoculated with NL/2631-R223 or NL/602. In addition, pulmonary lesions were similar at day 4 post inoculation. However, at day 7 post inoculation, NL/2631-R223 caused milder pulmonary lesions and degree of alveolitis than NL/602. This indicated that the mutant virus was less pathogenic. Both NL/2631-R223 and a recombinant virus with a single I223R change (recNL/602-I223R), transmitted among ferrets by aerosols, despite observed attenuation of recNL/602-I223R in vitro. In conclusion, the I223R mutated virus isolate has comparable replicative ability and transmissibility, but lower pathogenicity than the reference virus based on these in vivo studies. This implies that the 2009 pandemic influenza A/H1N1 virus subtype with an isoleucine to arginine change at position 223 in the neuraminidase has the potential to spread in the human population. It is important to be vigilant for this mutation in influenza surveillance and to continue efforts to increase the arsenal of antiviral drugs to combat influenza.

Published
2011

23. Performance evaluation of the new roche cobas ampliprep/cobas taqman HIV-1 test version 2.0 for quantification of human immunodeficiency virus type 1 RNA

Author

Pas, S.D. (Suzan), Rossen, J.W. (John), Schoener, D. (Daniel), Thamke, D. (Diana), Pettersson, A. (Annika), Babiel, R. (Reiner), Schutten, M. (Martin), Pas, S.D. (Suzan), Rossen, J.W. (John), Schoener, D. (Daniel), Thamke, D. (Diana), Pettersson, A. (Annika), Babiel, R. (Reiner), and Schutten, M. (Martin)

Abstract

Despite FDA approval and CE marking of commercial tests, manufacturer-independent testing of the technical aspects of newly developed tests is important. To evaluate the analytical performance and explore the clinical applicability of the new Roche COBAS AmpliPrep COBAS TaqMan HIV-1 test, version 2.0 (CAP/CTM v2.0), platform comparison was performed with the Roche CAP/CTM test, version 2.0, the COBAS Amplicor HIV-1 Monitor Test, version 1.5 (CAP/CA v1.5), the COBAS AmpliPrep COBAS TaqMan HIV-1 Test (CAP/ CTM v1.0), and the Abbott m2000 RealTime HIV-1 assay on panels and diagnostic samples. Specificity was tested for HIV-2 samples. Furthermore, samples from HIV-1-seropositive individuals with CAP/CA v1.5-measured viral loads below 50 HIV-1 RNA copies per ml (cp/ml) and replicates of HIV-1-seronegative plasma were tested in a checkerboard analysis. CAP/CTM v2.0 is HIV-1 specific, with broad genotype inclusivity and no serious underquantification of viral load relative to the other assays used. Low viral loads below the threshold of quantification for CAP/CA v1.5 are observed with CAP/CTM v2.0. A CAP/CTM v2.0-measured viral load of >50 copies/ml in these samples correlated with therapy failure. In conclusion, CAP/CTM v2.0 is an accurate and reliable test for HIV-1 viral load measurement relative to the other assays used with respect to specificity, sensitivity, and genotype inclusivity. Copyright

Published
2010
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24. The effect of primer-template mismatches on the detection and quantification of nucleic acids using the 5′ nuclease assay

Author

Stadhouders, R. (Ralph), Pas, S.D. (Suzan), Anber, J. (Jeer), Voermans, J. (Jolanda), Mes, T.H.M., Schutten, M. (Martin), Stadhouders, R. (Ralph), Pas, S.D. (Suzan), Anber, J. (Jeer), Voermans, J. (Jolanda), Mes, T.H.M., and Schutten, M. (Martin)

Abstract

Real-time polymerase chain reaction (PCR) is the current method of choice for detection and quantification of nucleic acids, especially for molecular diagnostics. Complementarity between primers and template is often crucial for PCR applications, as mismatches can severely reduce priming efficiency. However, little quantitative data on the effect of these mismatches is available. We quantitatively investigated the effects of primer-template mismatches within the 3′-end primer region on real-time PCR using the 5′-nuclease assay. Our results show that single mismatches i

Published
2010
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25. Practical considerations for high-throughput influenza A virus surveillance studies of wild birds by use of molecular diagnostic tests

Author

Munster, V.J. (Vincent), Baas, C. (Chantal), Lexmond, P. (Pascal), Bestebroer, T.M. (Theo), Guldemeester, J., Beyer, W.E.Ph. (Walter), Wit, E. (Emmie) de, Schutten, M. (Martin), Rimmelzwaan, G.F. (Guus), Osterhaus, A.D.M.E. (Albert), Fouchier, R.A.M. (Ron), Munster, V.J. (Vincent), Baas, C. (Chantal), Lexmond, P. (Pascal), Bestebroer, T.M. (Theo), Guldemeester, J., Beyer, W.E.Ph. (Walter), Wit, E. (Emmie) de, Schutten, M. (Martin), Rimmelzwaan, G.F. (Guus), Osterhaus, A.D.M.E. (Albert), and Fouchier, R.A.M. (Ron)

Abstract

Influenza A virus surveillance studies of wild bird populations are essential to improving our understanding of the role of wild birds in the ecology of low-pathogenic avian influenza viruses and their potential contribution to the spread of H5N1 highly pathogenic avian influenza viruses. Whereas the primary results of such surveillance programs have been communicated extensively, p

Published
2009
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26. P18-03. Dendritic cell-based immune therapy against HIV-1

Author

Gruters, R.A. (Rob), Keersmaecker, B. (Brenda) de, Goede, A.L. (Anna) de, Allard, S.D., Koetsveld, J. (Jeanette), Corthals, J. (Jurgen), Schutten, M. (Martin), Heirman, C. (Carlo), Ende, M.E. (Marchina) van der, Lacor, P. (Patrick), Osterhaus, A.D.M.E. (Albert), Thielemans, K. (Kris), Baalen, C.A. (Carel) van, Aerts, J.L. (Joeri), Gruters, R.A. (Rob), Keersmaecker, B. (Brenda) de, Goede, A.L. (Anna) de, Allard, S.D., Koetsveld, J. (Jeanette), Corthals, J. (Jurgen), Schutten, M. (Martin), Heirman, C. (Carlo), Ende, M.E. (Marchina) van der, Lacor, P. (Patrick), Osterhaus, A.D.M.E. (Albert), Thielemans, K. (Kris), Baalen, C.A. (Carel) van, and Aerts, J.L. (Joeri)

Published
2009
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28. Spatial, temporal, and species variation in prevalence of influenza A viruses in wild migratory birds

Author

Munster, V.J. (Vincent), Baas, C. (Chantal), Lexmond, P. (Pascal), Waldenström, J. (Jonas), Wallensten, A. (Anders), Fransson, T. (Thord), Rimmelzwaan, G.F. (Guus), Beyer, W.E.Ph. (Walter), Schutten, M. (Martin), Olsen, B. (Björn), Osterhaus, A.D.M.E. (Albert), Fouchier, R.A.M. (Ron), Munster, V.J. (Vincent), Baas, C. (Chantal), Lexmond, P. (Pascal), Waldenström, J. (Jonas), Wallensten, A. (Anders), Fransson, T. (Thord), Rimmelzwaan, G.F. (Guus), Beyer, W.E.Ph. (Walter), Schutten, M. (Martin), Olsen, B. (Björn), Osterhaus, A.D.M.E. (Albert), and Fouchier, R.A.M. (Ron)

Abstract

Although extensive data exist on avian influenza in wild birds in North America, limited information is available from elsewhere, including Europe. Here, molecular diagnostic tools were employed for high-throughput surveillance of migratory birds, as an alternative to classical labor-intensive methods of virus isolation in eggs. This study included 36,809 samples from 323 bird species belonging to 18 orders, of which only 25 species of three orders were positive for influenza A virus. Information on species, locations, and timing is provided for all samples tested. Seven previously unknown host species for avian influenza virus were identified: barnacle goose, bean goose, brent goose, pink-footed goose, bewick's swan, common gull, and guillemot. Dabbling ducks were more frequently infected than other ducks and Anseriformes; this distinction was probably related to bird behavior rather than population sizes. Waders did not appear to play a role in the epidemiology of avian influenza in Europe, in contrast to the Americas. The high virus prevalence in ducks in Europe in spring as compared with North America could explain the differences in virus-host ecology between these continents. Most influenza A virus subtypes were detected in ducks, but H13 and H16 subtypes were detected primarily in gulls. Viruses of subtype H6 were more promiscuous in host range than other subtypes. Temporal and spatial variation in influenza virus prevalence in wild birds was observed, with influenza A virus prevalence varying by sampling location; this is probably related to migration patterns from northeast to southwest and a higher prevalence farther north along the flyways. We discuss the ecology and epidemiology of avian influenza A virus in wild birds in relation to host ecology and compare our results with published studies. These data are useful for designing new surveillance programs and are particularly relevant due to increased interest in avian influenza in wild birds.

Published
2007
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29. Multicenter evaluation of the new Abbott Realtime assays for quantitative detection of human immunodeficiency virus type 1 and hepatitis C virus RNA

Author

Schutten, M. (Martin), Peters, D. (D.), Back, N. (Nicole), Beld, A.W. (Annewieke) van den, Beuselinck, B. (B.), Foulongne, V. (V.), Geretti, A.M. (Anna Maria), Pandiani, L. (L.), Tiemann, M., Niesters, H.G.M. (Bert), Schutten, M. (Martin), Peters, D. (D.), Back, N. (Nicole), Beld, A.W. (Annewieke) van den, Beuselinck, B. (B.), Foulongne, V. (V.), Geretti, A.M. (Anna Maria), Pandiani, L. (L.), Tiemann, M., and Niesters, H.G.M. (Bert)

Abstract

The analytical performances of the new Abbott RealTime hepatitis C virus (HCV) and human immunodeficiency virus type 1 viral load assays were compared at nine laboratories with different competitor assays. These included the Abbott LcX, Bayer Versant bDNA, Roche COBAS Amplicor, and Roche COBAS TaqMan assays. Two different protocols used during the testing period with and without a pre-m1000 RNA isolation spin were compared. The difference proved to be nonsignificant. A uracil-N-glycosylase (UNG) contamination control option in the HCV test for previous Roche COBAS Amplicor users was evaluated. It proved to decrease amplicon carryover by 100-fold independent of the amplicon input concentration. The protocol including UNG proved to overcome problems with false-positive negative controls. Comparison with other assays revealed only minor differences. The largest difference was observed between the Abbott HCV RealTime assay and the Roche COBAS Amplicor HCV Monitor version 2.0 assay. Copyright

Published
2007
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32. Avian influenza A virus (H7N7) associated with human conjunctivitis and a fatal case of acute respiratory distress syndrome.

Author

Fouchier, R.A.M. (Ron), Schneeberger, P.M. (Peter), Rozendaal, F.W. (Frans), Broekman, J.M. (Jan), Kemink, S.A. (Stiena), Munster, V.J. (Vincent), Rimmelzwaan, G.F. (Guus), Schutten, M. (Martin), Doornum, G.J.J. (Gerard) van, Koch, G. (Guus), Bosman, A. (Arnold), Koopmans D.V.M., M.P.G. (Marion), Osterhaus, A.D.M.E. (Albert), Kuiken, T. (Thijs), Fouchier, R.A.M. (Ron), Schneeberger, P.M. (Peter), Rozendaal, F.W. (Frans), Broekman, J.M. (Jan), Kemink, S.A. (Stiena), Munster, V.J. (Vincent), Rimmelzwaan, G.F. (Guus), Schutten, M. (Martin), Doornum, G.J.J. (Gerard) van, Koch, G. (Guus), Bosman, A. (Arnold), Koopmans D.V.M., M.P.G. (Marion), Osterhaus, A.D.M.E. (Albert), and Kuiken, T. (Thijs)

Abstract

Highly pathogenic avian influenza A viruses of subtypes H5 and H7 are the causative agents of fowl plague in poultry. Influenza A viruses of subtype H

Published
2004
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33. Comparison of the efficacy of early versus late viral proteins in vaccination against SIV.

Author

Stittelaar, K.J. (Koert), Gruters, R.A. (Rob), Schutten, M. (Martin), Baalen, C.A. (Carel) van, Amerongen, G. (Geert) van, Cranage, M.P. (Martin), Liljeström, P. (Peter), Sutter, G. (Gerd), Osterhaus, A.D.M.E. (Albert), Stittelaar, K.J. (Koert), Gruters, R.A. (Rob), Schutten, M. (Martin), Baalen, C.A. (Carel) van, Amerongen, G. (Geert) van, Cranage, M.P. (Martin), Liljeström, P. (Peter), Sutter, G. (Gerd), and Osterhaus, A.D.M.E. (Albert)

Abstract

The immune response against early regulatory proteins of simian- and human immunodeficiency virus (SIV, HIV) has been associated with a milder course of infection. Here, we directly compared vaccination with Tat/Rev versus Pol/Gag. Challenge infection with SIVmac32H (pJ5) suggested that vaccination with Tat/Rev induced cellular immune responses that enabled cynomolgus macaques to more efficiently control SIV replication than the vaccine-induced immune responses against Pol/Gag. Vaccination with Tat/Rev resulted in reduced plasma SIV loads compared with control (P=0.058) or Pol/Gag-vaccinated (P=

Published
2002
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34. Antibody-mediated enhancement of human immunodeficiency virus type 1 infectivity is determined by the structure of gp120 and depends on modulation of the gp120-CCR5 interaction

Author

Guillon, C. (Christophe), Schutten, M. (Martin), Boers, P.H.M. (Patrick), Gruters, R.A. (Rob), Osterhaus, A.D.M.E. (Albert), Guillon, C. (Christophe), Schutten, M. (Martin), Boers, P.H.M. (Patrick), Gruters, R.A. (Rob), and Osterhaus, A.D.M.E. (Albert)

Abstract

In this study, we characterized the viral determinants of coreceptor usage in relation to susceptibility to antibody-mediated neutralization or enhancement of infectivity by using chimeras of three highly related human immunodeficiency virus type 1 (HIV-1) isolates of different phenotypes. We found that the V3 region was the main determinant of antibody-mediated enhancement and coreceptor specificity but that the overall structure of gp120 was also important for these properties. Constructs susceptible to antibody-mediated enhancement preferentially use CCR5 as a coreceptor, in contrast to constructs that were neutralized or not affected. Using monoclonal antibodies directed against CD4 or CCR5, we were able to show that antibody-mediated enhancement was CD4 dependent. Altogether, our results suggest that the modulation of the interaction of gp120 with CCR5 is the mechanism underlying antibody-mediated enhancement of HIV-1 infectivity.

Published
2002

37. Macrophage tropism of human immunodeficiency virus type 1 facilitates in vivo escape from cytotoxic T-lymphocyte pressure.

Author

Schutten, M. (Martin), Baalen, C.A. (Carel) van, Guillon, C. (Christophe), Huisman, R.C. (Robin), Boers, P.H.M. (Patrick), Sintnicolaas, K. (Krijn), Gruters, R.A. (Rob), Osterhaus, A.D.M.E. (Albert), Schutten, M. (Martin), Baalen, C.A. (Carel) van, Guillon, C. (Christophe), Huisman, R.C. (Robin), Boers, P.H.M. (Patrick), Sintnicolaas, K. (Krijn), Gruters, R.A. (Rob), and Osterhaus, A.D.M.E. (Albert)

Abstract

Early after seroconversion, macrophage-tropic human immunodeficiency virus type 1 (HIV-1) variants are predominantly found, even when a mixture of macrophage-tropic and non-macrophage-tropic variants was transmitted. For virus contracted by sexual transmission, this is presently explained by selection at the port of entry, where macrophages are infected and T cells are relatively rare. Here we explore an additional mechanism to explain the selection of macrophage-tropic variants in cases where the mucosa is bypassed during transmission, such as blood transfusion, needle-stick accidents, or intravenous drug abuse. With molecularly cloned primary isolates of HIV-1 in irradiated mice that had been reconstituted with a high dose of human peripheral blood mononuclear cells, we found that a macrophage-tropic HIV-1 clone escaped more efficiently from specific cytotoxic T-lymphocyte (CTL) pressure than its non-macrophage-tropic counterpart. We propose that CTLs favor the selective outgrowth of macrophage-tropic HIV-1 variants because infected macrophages are less susceptible to CTL activity than infected T cells.

Published
2001
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38. Antiviral resistance of biologic HIV-2 clones obtained from individuals on nucleoside reverse transcriptase inhibitor therapy

Author

Ende, M.E. (Marchina) van der, Guillon, C. (Christophe), Boers, P.H.M. (Patrick), Ly, T.D. (Thoai Duong), Gruters, R.A. (Rob), Osterhaus, A.D.M.E. (Albert), Schutten, M. (Martin), Ende, M.E. (Marchina) van der, Guillon, C. (Christophe), Boers, P.H.M. (Patrick), Ly, T.D. (Thoai Duong), Gruters, R.A. (Rob), Osterhaus, A.D.M.E. (Albert), and Schutten, M. (Martin)

Abstract

Objective: To study phenotypic and genotypic resistance of HIV-2 against nucleoside reverse transcriptase inhibitors (NRTI). Methods: Biologic HIV-2 clones were generated from 3 patients before and after initiation of antiretroviral therapy with zidovudine (AZT) in patient RH2-7, AZT and didanosine (ddI) in patient PH2-1, and after addition of lamivudine (3TC) to AZT monotherapy in patient RH2-5. The sensitivity to NRTI of the virus clones, as defined by the 50% inhibitory concentration (IC50), was determined in vitro. The predicted amino acid sequences of the reverse transcriptase proteins from these clones were determined. Results: Comparing the sensitivity of the biologic HIV-2 clones obtained after start of therapy with those from antiviral naive patients, resistance had developed to AZT (patients RH2-7 and RH2-5) and 3TC (patient PH2-1 and RH2-5). No resistance to AZT was observed in the biologic clone from PH2-1 obtained after start of therapy. The resistant clones from RH2-5 and PH2-1, but not RH2-7, contained amino acid mutations at positions where HIV-1 has been shown to mutate after AZT and 3TC treatment. Conclusions: Phenotypic resistance of HIV-2 to nucleoside analogues, which developed in HIV-2-infected patients treated with NRTIs, was associated with genotypic changes. Some of the mutations at amino acid positions in the HIV-2 reverse transcriptase gene corresponded with those involved in HIV-1 resistance, although no conventional mutations associated with resistance to AZT were observed.

Published
2000
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39. Broadening of coreceptor usage by human immunodeficiency virus type 2 does not correlate with increased pathogenicity in an in vivo model.

Author

Ende, M.E. (Marchina) van der, Guillon, C. (Christophe), Boers, P.H.M. (Patrick), Gruters, R.A. (Rob), Racz, P., Tenner-Racz, K., Osterhaus, A.D.M.E. (Albert), Schutten, M. (Martin), Ende, M.E. (Marchina) van der, Guillon, C. (Christophe), Boers, P.H.M. (Patrick), Gruters, R.A. (Rob), Racz, P., Tenner-Racz, K., Osterhaus, A.D.M.E. (Albert), and Schutten, M. (Martin)

Abstract

The pathogenic properties of four primary human immunodeficiency virus type 2 (HIV-2) isolates and two primary HIV-2 biological clones were studied in an in vivo human-to-mouse chimeric model. The cell-associated viral load and the ability to reduce the severity of the induced graft-versus-host disease symptoms, the CD4/CD8 ratio and the level of repopulation of the mouse tissues by the graft, were determined. All HIV-2 strains, irrespective of their in vitro biological phenotype, replicated to high titres and significantly reduced graft-versus-host disease symptoms as well as the CD4/CD8 ratios. Reduction of graft repopulation caused by infection with the respective HIV-2 strains showed that the in vitro replication rate, syncytium-inducing capacity and ability to infect human macrophages did influence the in vivo pathogenic potential whereas broadening of coreceptor usage did not.

Published
2000

42. CD4 T cells remain the major source of HIV-1 during end stage disease.

Author

Ende, M.E. (Marchina) van der, Schutten, M. (Martin), Raschdorff, B., Grosschupff, G., Racz, P., Osterhaus, A.D.M.E. (Albert), Tenner-Racz, K., Ende, M.E. (Marchina) van der, Schutten, M. (Martin), Raschdorff, B., Grosschupff, G., Racz, P., Osterhaus, A.D.M.E. (Albert), and Tenner-Racz, K.

Abstract

OBJECTIVE: To assess the source of HIV-1 production in lymphoid tissue biopsies from HIV-infected patients, with no prior anti-retroviral protease inhibitor treatment, with a CD4 cell count > 150 x 10(6)/l (group I) or < 50 x 10(6)/l (group II), co-infected with Mycobacterium tuberculosis or Mycobacterium avium complex. DESIGN AND METHODS: Lymphoid tissue biopsies from 11 HIV-1-infected patients, taken for diagnostic purposes, were studied by HIV-1 RNA in situ hybridization and immunohistochemistry. RESULTS: Patients of group I showed well organized granulomas, in contrast with patients of group II, in which granuloma formation was absent. HIV-1 RNA-positive cells in group I patients were found mainly around the granulomas, whereas in group II HIV-1-producing cells were confined to areas with remaining intact lymphoid tissue. Despite the abundant presence of macrophages, the productively infected HIV-1-positive cells in both groups were almost exclusively CD4 T cells. CONCLUSION: In contrast with previously published data, CD4 T cells appear to remain the major source of HIV-1 production in end-stage disease.

Published
1999

44. Coreceptor usage of human immunodeficiency virus type 2 primary isolates and biological clones is broad and does not correlate with their syncytium-inducing capacities

Author

Guillon, C. (Christophe), Boers, P.H.M. (Patrick), Gruters, R.A. (Rob), Schutten, M. (Martin), Ende, M.E. (Marchina) van der, Osterhaus, A.D.M.E. (Albert), Guillon, C. (Christophe), Boers, P.H.M. (Patrick), Gruters, R.A. (Rob), Schutten, M. (Martin), Ende, M.E. (Marchina) van der, and Osterhaus, A.D.M.E. (Albert)

Abstract

Entry of human immunodeficiency virus type 1 (HIV-1) into target cells is mediated by binding of the surface envelope glycoprotein to the CD4 molecule. Interaction of the resulting CD4-glycoprotein complex with alpha- or beta-chemokine receptors, depending on the biological phenotype of the virus, then initiates the fusion process. Here, we show that primary HIV-2 isolates and biological clones, in contrast to those of HIV-1, may use a broad range of coreceptors, including CCR-1, CCR-3, CCR-5, and CXCR-4. The syncytium-inducing capacity of these viruses did not correlate with the ability to infect via CXCR-4 or any other coreceptor. One cell-free passage of the intermediate isolates in mitogen-stimulated, CD8+ cell-depleted peripheral blood mononuclear cells resulted in the outgrowth of variants with CCR-5 only, whereas the coreceptor usage of late and early isolates did not change. Since HIV-2 is less pathogenic in vivo than HIV-1, these data suggest that HIV pathogenicity in vivo is not directly related to the spectrum of coreceptors used in in vitro systems.

Published
1998

45. Kinetics of antiviral activity by human immunodeficiency virus type 1-specific cytotoxic T lymphocytes (CTL) and rapid selection of CTL escape virus in vitro

Author

Schutten, M. (Martin), Huisman, R.C. (Robin), Boers, P.H.M. (Patrick), Gruters, R.A. (Rob), Baalen, C.A. (Carel) van, Osterhaus, A.D.M.E. (Albert), Schutten, M. (Martin), Huisman, R.C. (Robin), Boers, P.H.M. (Patrick), Gruters, R.A. (Rob), Baalen, C.A. (Carel) van, and Osterhaus, A.D.M.E. (Albert)

Abstract

The antiviral activity of a CD8(+) cytotoxic T-lymphocyte (CTL) clone (TCC108) directed against a newly identified HLA-B14-restricted epitope, human immunodeficiency virus type 1 (HIV-1) Rev(67-75) SAEPVPLQL, was analyzed with respect to its kinetics of target cell

Published
1998

48. HIV-2 infection in 12 European residents: virus characteristics and disease progression.

Author

Ende, M.E. (Marchina) van der, Schutten, M. (Martin), Ly, T.D., Gruters, R.A. (Rob), Osterhaus, A.D.M.E. (Albert), Ende, M.E. (Marchina) van der, Schutten, M. (Martin), Ly, T.D., Gruters, R.A. (Rob), and Osterhaus, A.D.M.E. (Albert)

Abstract

OBJECTIVE: To assess the disease progression rate among 12 HIV-2-infected West European residents (nine of West African descent), compared with the disease progression rate among HIV-1-infected individuals of the same population, and the characteristics of the HIV-2 strains involved. METHODS: HIV-2-infected individuals were identified by commercially available serological assays, their clinical status and CD4+ cell counts were monitored, and HIV-2 was isolated from their peripheral blood mononuclear cells. T-cell-line tropism and syncytium-inducing capacities of the isolated viruses were determined and their phylogenetic relationships were analysed by comparing polymerase chain reaction-amplified nucleotide sequences of reverse transcriptase (RT) gene segments. RESULTS: Eight of the 12 HIV-2-infected individuals presented with progressive disease and one of them progressed from Centers for Disease Control and Prevent

Published
1996

49. Human antibodies that neutralize primary human immunodeficiency virus type 1 in vitro do not provide protection in an in vivo model.

Author

Schutten, M. (Martin), Tenner-Racz, K., Racz, P., Bekkum, D.W. (Dirk) van, Osterhaus, A.D.M.E. (Albert), Schutten, M. (Martin), Tenner-Racz, K., Racz, P., Bekkum, D.W. (Dirk) van, and Osterhaus, A.D.M.E. (Albert)

Abstract

Recently, conflicting data have been published about the ability of antibodies which efficiently neutralize T cell-adapted human immunodeficiency virus type 1 (HIV-1) strains to neutralize primary HIV-1 strains in vitro and in vivo. Here we present data indicating that such antibodies fail to neutralize primary HIV-1 strains in vivo. To this end, a newly developed chimeric human-to-mouse model was used, in which several aspects of primary HIV-1 infection are mimicked. Poly- and monoclonal antibodies protected the grafted human cells, in a dose-dependent way, from infection with T cell-adapted HIV-1 in this system. A human monoclonal antibody specific for the CD4 binding domain that efficiently neutralizes HIV-1 IIIB in vitro did not protect the human graft from HIV-1 IIIB infection. None of the antibodies provided protection in the in vivo model against infection with primary HIV-1 strains, although they were able to neutralize these same strains in vitro.

Published
1996

50. Characterization of a V3 domain-specific neutralizing human monoclonal antibody that preferentially recognizes non-syncytium-inducing human immunodeficiency virus type 1 strains.

Author

Schutten, M. (Martin), Langedijk, J.P.M., Andeweg, A.C. (Arno), Huisman, R.C. (Robin), Meloen, R.H., Osterhaus, A.D.M.E. (Albert), Schutten, M. (Martin), Langedijk, J.P.M., Andeweg, A.C. (Arno), Huisman, R.C. (Robin), Meloen, R.H., and Osterhaus, A.D.M.E. (Albert)

Abstract

A type-specific human immunodeficiency virus type 1 (HIV-1)-neutralizing human monoclonal antibody (HuMAb MN215) is described that reacts with the V3 domain of a number of subtype B virus strains. Pepscan analysis indicated that amino acids at both sides of the tip of the V3 loop were involved in the binding of HuMAb MN215. The minimum epitope in a V3 sequence, obtained from the donor from whom the cell line originated, was 9 amino acids long and proved to be located at the C-terminal side of the tip of the loop. In a replacement Pepscan analysi

Published
1995

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