Search

Your search keyword '"Lanke, K.H.W."' showing total 147 results
Start Over Author "Lanke, K.H.W."
147 results on '"Lanke, K.H.W."'

1. Naturally acquired antibodies to gametocyte antigens are associated with reduced transmission of Plasmodium vivax gametocytes to Anopheles arabiensis mosquitoes

Author

Tebeje, S.K., Chali, Wakweya, Hailemeskel, E., Ramjith, J., Gashaw, Abrham, Ashine, Temesgen, Teelen, K.A.E.M., Lanke, K.H.W., Jore, M.M., Hansen, I.S., Tadesse, F.G., Bousema, T., Tebeje, S.K., Chali, Wakweya, Hailemeskel, E., Ramjith, J., Gashaw, Abrham, Ashine, Temesgen, Teelen, K.A.E.M., Lanke, K.H.W., Jore, M.M., Hansen, I.S., Tadesse, F.G., and Bousema, T.

Abstract

Contains fulltext : 290145.pdf (Publisher’s version ) (Open Access)

Published
2023

2. Plasmodium falciparum gametocyte carriage in longitudinally monitored incident infections is associated with duration of infection and human host factors.

Author

Andolina, C., Ramjith, J., Rek, J., Lanke, K.H.W., Okoth, J., Grignard, L., Arinaitwe, E., Briggs, J., Bailey, J., Aydemir, O., Kamya, M.R., Greenhouse, B., Dorsey, G., Staedke, S.G., Drakeley, C., Jonker, M.A., Bousema, T., Andolina, C., Ramjith, J., Rek, J., Lanke, K.H.W., Okoth, J., Grignard, L., Arinaitwe, E., Briggs, J., Bailey, J., Aydemir, O., Kamya, M.R., Greenhouse, B., Dorsey, G., Staedke, S.G., Drakeley, C., Jonker, M.A., and Bousema, T.

Abstract

Item does not contain fulltext, Malaria transmission depends on the presence of Plasmodium gametocytes that are the only parasite life stage that can infect mosquitoes. Gametocyte production varies between infections and over the course of infections. Infection duration is highly important for gametocyte production but poorly quantified. Between 2017 and 2019 an all-age cohort of individuals from Tororo, eastern Uganda was followed by continuous passive and routine assessments. We longitudinally monitored 104 incident infections from 98 individuals who were sampled once every 28 days and on any day of symptoms. Among infections that lasted ≥ 3 months, gametocyte appearance was near-universal with 96% of infections having detectable gametocytes prior to clearance. However, most infections were of much shorter duration; 55.7% of asymptomatic infections were detected only once. When considering all asymptomatic infections, regardless of their duration, only 36.3% had detectable gametocytes on at least one time-point prior to parasite clearance. Infections in individuals with sickle-cell trait (HbAS) were more likely to have gametocytes detected (Hazard Rate (HR) = 2.68, 95% CI 1.12, 6.38; p = 0.0231) and had gametocytes detected at higher densities (Density Ratio (DR) = 9.19, 95% CI 2.79, 30.23; p = 0.0002) compared to infections in wildtype (HbAA) individuals. Our findings suggest that a large proportion of incident infections is too short in duration and of too low density to contribute to onward transmission.

Published
2023

3. A Cohort Study on the Duration of Plasmodium falciparum Infections During the Dry Season in The Gambia

Author

Collins, K.A., Ceesay, S., Drammeh, S., Jaiteh, F.K., Guery, M.A., Lanke, K.H.W., Grignard, L., Stone, W., Conway, D.J., D'Alessandro, U., Bousema, T., Claessens, A., Collins, K.A., Ceesay, S., Drammeh, S., Jaiteh, F.K., Guery, M.A., Lanke, K.H.W., Grignard, L., Stone, W., Conway, D.J., D'Alessandro, U., Bousema, T., and Claessens, A.

Abstract

Contains fulltext : 282500.pdf (Publisher’s version ) (Open Access), BACKGROUND: In areas where Plasmodium falciparum malaria is seasonal, a dry season reservoir of blood-stage infection is essential for initiating transmission during the following wet season. METHODS: In The Gambia, a cohort of 42 individuals with quantitative polymerase chain reaction-positive P falciparum infections at the end of the transmission season (December) were followed monthly until the end of the dry season (May) to evaluate infection persistence. The influence of human host and parasitological factors was investigated. RESULTS: A large proportion of individuals infected at the end of the wet season had detectable infections until the end of the dry season (40.0%; 16 of 40). At the start of the dry season, the majority of these persistent infections (82%) had parasite densities >10 p/µL compared to only 5.9% of short-lived infections. Persistent infections (59%) were also more likely to be multiclonal than short-lived infections (5.9%) and were associated with individuals having higher levels of P falciparum-specific antibodies (P = .02). CONCLUSIONS: Asymptomatic persistent infections were multiclonal with higher parasite densities at the beginning of the dry season. Screening and treating asymptomatic infections during the dry season may reduce the human reservoir of malaria responsible for initiating transmission in the wet season.

Published
2022

4. Single low-dose tafenoquine combined with dihydroartemisinin-piperaquine to reduce Plasmodium falciparum transmission in Ouelessebougou, Mali: a phase 2, single-blind, randomised clinical trial

Author

Stone, W., Mahamar, A., Smit, M.J., Sanogo, K., Sinaba, Y., Niambele, S.M., Sacko, A., Keita, S., Dicko, O.M., Diallo, M., Maguiraga, S.O., Samake, S., Attaher, O., Lanke, K.H.W., Heine, R. ter, Bradley, J., McCall, M.B.B., Issiaka, D., Traore, S.F., Bousema, T., Drakeley, C., Dicko, A., Stone, W., Mahamar, A., Smit, M.J., Sanogo, K., Sinaba, Y., Niambele, S.M., Sacko, A., Keita, S., Dicko, O.M., Diallo, M., Maguiraga, S.O., Samake, S., Attaher, O., Lanke, K.H.W., Heine, R. ter, Bradley, J., McCall, M.B.B., Issiaka, D., Traore, S.F., Bousema, T., Drakeley, C., and Dicko, A.

Abstract

Contains fulltext : 251206.pdf (Publisher’s version ) (Open Access), BACKGROUND: Tafenoquine was recently approved as a prophylaxis and radical cure for Plasmodium vivax infection, but its Plasmodium falciparum transmission-blocking efficacy is unclear. We aimed to establish the efficacy and safety of three single low doses of tafenoquine in combination with dihydroartemisinin-piperaquine for reducing gametocyte density and transmission to mosquitoes. METHODS: In this four-arm, single-blind, phase 2, randomised controlled trial, participants were recruited at the Clinical Research Unit of the Malaria Research and Training Centre of the University of Bamako in Mali. Eligible participants were aged 12-50 years, with asymptomatic P falciparum microscopy-detected gametocyte carriage, had a bodyweight of 80 kg or less, and had no clinical signs of malaria defined by fever. Participants were randomly assigned (1:1:1:1) to standard treatment with dihydroartemisinin-piperaquine, or dihydroartemisinin-piperaquine plus a single dose of tafenoquine (in solution) at a final dosage of 0·42 mg/kg, 0·83 mg/kg, or 1·66 mg/kg. Randomisation was done with a computer-generated randomisation list and concealed with sealed, opaque envelopes. Dihydroartemisinin-piperaquine was administered as oral tablets over 3 days (day 0, 1, and 2), as per manufacturer instructions. A single dose of tafenoquine was administered as oral solution on day 0 in parallel with the first dose of dihydroartemisinin-piperaquine. Tafenoquine dosing was based on bodyweight to standardise efficacy and risk variance. The primary endpoint, assessed in the per-protocol population, was median percentage change in mosquito infection rate 7 days after treatment compared with baseline. Safety endpoints included frequency and incidence of adverse events. The final follow-up visit was on Dec 23, 2021; the trial is registered with ClinicalTrials.gov, NCT04609098. FINDINGS: From Oct 29 to Nov 25, 2020, 1091 individuals were screened for eligibility, 80 of whom were enrolled and randomly assig

Published
2022

6. Sources of persistent malaria transmission in a setting with effective malaria control in eastern Uganda: a longitudinal, observational cohort study

Author

Andolina, C., Rek, John, Briggs, Jessica, Okoth, Joseph, Musiime, Alex K., Ramjith, J., Lanke, K.H.W., Meerstein-Kessel, L., Drakeley, C., Staedke, S.G., Bousema, T., Andolina, C., Rek, John, Briggs, Jessica, Okoth, Joseph, Musiime, Alex K., Ramjith, J., Lanke, K.H.W., Meerstein-Kessel, L., Drakeley, C., Staedke, S.G., and Bousema, T.

Abstract

Item does not contain fulltext

Published
2021

7. A Randomized Clinical Trial to Compare Plasmodium falciparum Gametocytemia and Infectivity After Blood- Stage or Mosquito Bite Induced Controlled Malaria Infection

Author

Alkema, M., Reuling, I.J., Jong, Gerdie M. de, Lanke, K.H.W., Coffeng, Luc E., Gemert, G.J.A. van, Vegte-Bolmer, M.G. van de, Mast, Q. de, Crevel, R. van, Sauerwein, R.W., Collins, K.A., Bousema, T., Alkema, M., Reuling, I.J., Jong, Gerdie M. de, Lanke, K.H.W., Coffeng, Luc E., Gemert, G.J.A. van, Vegte-Bolmer, M.G. van de, Mast, Q. de, Crevel, R. van, Sauerwein, R.W., Collins, K.A., and Bousema, T.

Abstract

Item does not contain fulltext

Published
2021

8. SARS-CoV-2 mucosal antibody development and persistence and their relation to viral load and COVID-19 symptoms

Author

Fröberg, J., Gillard, J.J., Philipsen, H.L.A., Lanke, K.H.W., Rust, Joyce, Tuijl, Diana van, Teelen, K.A., Bousema, T., Simonetti, E.R., Gaast-de Jongh, C.E. van der, Bos, Mariska, Kuppeveld, F.J.M. van, Nabuurs-Franssen, M.H., Daal, Charlotte van, Geest-Blankert, Nannet van der, Huynen, M.A., Jonge, M.I. de, Diavatopoulos, D.A., Fröberg, J., Gillard, J.J., Philipsen, H.L.A., Lanke, K.H.W., Rust, Joyce, Tuijl, Diana van, Teelen, K.A., Bousema, T., Simonetti, E.R., Gaast-de Jongh, C.E. van der, Bos, Mariska, Kuppeveld, F.J.M. van, Nabuurs-Franssen, M.H., Daal, Charlotte van, Geest-Blankert, Nannet van der, Huynen, M.A., Jonge, M.I. de, and Diavatopoulos, D.A.

Abstract

Contains fulltext : 238286.pdf (Publisher’s version ) (Open Access)

Published
2021

9. Plasmodium falciparum Gametocyte Density and Infectivity in Peripheral Blood and Skin Tissue of Naturally Infected Parasite Carriers in Burkina Faso

Author

Meibalan, E., Barry, A., Gibbins, M.P., Awandu, S.S., Meerstein-Kessel, L., Achcar, F., Bopp, S., Moxon, C., Diarra, A., Debe, S., Ouedraogo, N., Barry-Some, I., Badoum, E., Fagnima, T., Lanke, K.H.W., Goncalves, B.P., Bradley, J., Wirth, D., Drakeley, C., Guelbeogo, W.M., Tiono, A.B., Marti, M., Bousema, T., Meibalan, E., Barry, A., Gibbins, M.P., Awandu, S.S., Meerstein-Kessel, L., Achcar, F., Bopp, S., Moxon, C., Diarra, A., Debe, S., Ouedraogo, N., Barry-Some, I., Badoum, E., Fagnima, T., Lanke, K.H.W., Goncalves, B.P., Bradley, J., Wirth, D., Drakeley, C., Guelbeogo, W.M., Tiono, A.B., Marti, M., and Bousema, T.

Abstract

Contains fulltext : 227488.pdf (publisher's version ) (Open Access)

Published
2019

10. Safety of single low-dose primaquine in glucose-6-phosphate dehydrogenase deficient falciparum-infected African males: Two open-label, randomized, safety trials

Author

Bastiaens, G.J.H., Tiono, A.B., Okebe, J., Pett, H.E., Coulibaly, Sam A., Goncalves, B.P., Lanke, K.H.W., Bousema, T., and Drakeley, C.

Subjects
All institutes and research themes of the Radboud University Medical Center, lnfectious Diseases and Global Health Radboud Institute for Health Sciences [Radboudumc 4]
Abstract

Contains fulltext : 184044.pdf (Publisher’s version ) (Open Access)

Published
2018

11. Predicting the likelihood and intensity of mosquito infection from sex specific Plasmodium falciparum gametocyte density

Author

Bradly, John, Stone, W.J.R., Da, D.F., Morlais, I., Dicko, A., Cohuet, A., Lanke, K.H.W., Graumans, W., Siebelink-Stoter, R., Vegte-Bolmer, M.G. van de, Sauerwein, R.W., Churcher, T.S., Bousema, T., Bradly, John, Stone, W.J.R., Da, D.F., Morlais, I., Dicko, A., Cohuet, A., Lanke, K.H.W., Graumans, W., Siebelink-Stoter, R., Vegte-Bolmer, M.G. van de, Sauerwein, R.W., Churcher, T.S., and Bousema, T.

Abstract

Contains fulltext : 193046.pdf (publisher's version ) (Open Access)

Published
2018

12. A randomized feasibility trial comparing four antimalarial drug regimens to induce Plasmodium falciparum gametocytemia in the controlled human malaria infection model

Author

Reuling, I.J. (Isaie J.), Van De Schans, L.A. (Lisanne A.), Coffeng, L.E. (Luc), Lanke, K.H.W. (Kjerstin ), Meerstein-Kessel, L. (Lisette), Graumans, W. (Wouter), Gemert, G-J. (Geert-Jan) van, Teelen, K. (Karina), Siebelink-Stoter, R. (Rianne), Vegte-Bolmer, M. (Magda) van de, Mast, Q. (Quirijn) de, Ven, A.D. (Andre´) van, Ivinson, K. (Karen), Hermsen, C.C. (Cornelus), Vlas, S.J. (Sake) de, Bradley, J. (John), Collins, K.A. (Katharine A.), Ockenhouse, C.F. (Christian), McCarthy, J. (James), Sauerwein, R.W. (Robert), Bousema, T. (Teun), Reuling, I.J. (Isaie J.), Van De Schans, L.A. (Lisanne A.), Coffeng, L.E. (Luc), Lanke, K.H.W. (Kjerstin ), Meerstein-Kessel, L. (Lisette), Graumans, W. (Wouter), Gemert, G-J. (Geert-Jan) van, Teelen, K. (Karina), Siebelink-Stoter, R. (Rianne), Vegte-Bolmer, M. (Magda) van de, Mast, Q. (Quirijn) de, Ven, A.D. (Andre´) van, Ivinson, K. (Karen), Hermsen, C.C. (Cornelus), Vlas, S.J. (Sake) de, Bradley, J. (John), Collins, K.A. (Katharine A.), Ockenhouse, C.F. (Christian), McCarthy, J. (James), Sauerwein, R.W. (Robert), and Bousema, T. (Teun)

Abstract

Background: Malaria elimination strategies require a thorough understanding of parasite transmission from human to mosquito. A clinical model to induce gametocytes to understand their dynamics and evaluate transmission-blocking interventions (TBI) is currently unavailable. Here, we explore the use of the well-established Controlled

Published
2018
Full Text
View/download PDF

13. Examining the human infectious reservoir for Plasmodium falciparum malaria in areas of differing transmission intensity

Author

Goncalves, B.P., Kapulu, M.C., Sawa, P., Guelbeogo, W.M., Tiono, A.B., Grignard, L., Stone, W.J.R., Hellewell, J., Lanke, K.H.W., Bastiaens, G.J.H., Bradley, J., Nebie, I., Ngoi, J.M., Oriango, R., Mkabili, D., Nyaurah, M., Midega, J., Wirth, D.F., Marsh, K., Churcher, T.S., Bejon, P., Sirima, S.B., Drakeley, C., Bousema, J.T., Goncalves, B.P., Kapulu, M.C., Sawa, P., Guelbeogo, W.M., Tiono, A.B., Grignard, L., Stone, W.J.R., Hellewell, J., Lanke, K.H.W., Bastiaens, G.J.H., Bradley, J., Nebie, I., Ngoi, J.M., Oriango, R., Mkabili, D., Nyaurah, M., Midega, J., Wirth, D.F., Marsh, K., Churcher, T.S., Bejon, P., Sirima, S.B., Drakeley, C., and Bousema, J.T.

Abstract

Contains fulltext : 182487.pdf (publisher's version ) (Open Access), A detailed understanding of the human infectious reservoir is essential for improving malaria transmission-reducing interventions. Here we report a multi-regional assessment of population-wide malaria transmission potential based on 1209 mosquito feeding assays in endemic areas of Burkina Faso and Kenya. Across both sites, we identified 39 infectious individuals. In high endemicity settings, infectious individuals were identifiable by research-grade microscopy (92.6%; 25/27), whilst one of three infectious individuals in the lowest endemicity setting was detected by molecular techniques alone. The percentages of infected mosquitoes in the different surveys ranged from 0.05 (4/7716) to 1.6% (121/7749), and correlate positively with transmission intensity. We also estimated exposure to malaria vectors through genetic matching of blood from 1094 wild-caught bloodfed mosquitoes with that of humans resident in the same houses. Although adults transmitted fewer parasites to mosquitoes than children, they received more mosquito bites, thus balancing their contribution to the infectious reservoir.

Published
2017

14. The mengovirus leader protein blocks interferon-alpha/beta gene transcription and inhibits activation of interferon regulatory factor 3

Author

Hato, S.V., Ricour, C., Schulte, B.M., Lanke, K.H.W., Bruijni, M.A.M. de, Zoll, G.J., Melchers, W.J.G., Michiels, T., and Kuppeveld, F.J.M. van

Subjects
Pathogenesis and modulation of inflammation [N4i 1], Invasive mycoses and compromised host [N4i 2], Poverty-related infectious diseases [N4i 3], Microbial pathogenesis and host defense [UMCN 4.1], Infection and autoimmunity [NCMLS 1], Immunity, infection and tissue repair [NCMLS 1]
Abstract

Contains fulltext : 52463.pdf (Publisher’s version ) (Closed access) Viral infection of mammalian cells triggers the synthesis and secretion of type I interferons (i.e. IFN-alpha/beta), which induce the transcription of genes that cause cells to adopt an antiviral state. Many viruses have adapted mechanisms to evade IFN-alpha/beta-mediated responses. The leader protein of mengovirus, a picornavirus, has been implicated as an IFN-alpha/beta antagonist. Here, we show that the leader inhibits the transcription of IFN-alpha/beta and that both the presence of a zinc finger motif in its N-terminus and phosphorylation of threonine-47 are required for this function. Transcription of IFN-alpha/beta genes relies on the activity of a number of transcription factors, including interferon regulatory factor 3 (IRF-3). We show that the leader interferes with the transactivation activity of IRF-3 by interfering with its dimerization. Accordingly, mutant viruses with a disturbed leader function were impaired in their ability to suppress IFN-alpha/beta transcription in vivo. By consequence, the leader mutant viruses had an impaired ability to replicate and spread in normal mice but not in IFNAR-KO mice, which are incapable of mounting an IFN-alpha/beta-dependent antiviral response. These results suggest that the leader, by suppressing IRF3-mediated IFN-alpha/beta production, plays an important role in replication and dissemination of mengovirus in its host.

Published
2007

15. Quantification of female and male Plasmodium falciparum gametocytes by reverse transcriptase quantitative PCR

Author

Schneider, P., Reece, S.E., Schaijk, B.C.L. van, Bousema, T., Lanke, K.H.W., Meaden, C.S., Gadalla, A., Ranford-Cartwright, L.C., and Babiker, H.A.

Subjects
lnfectious Diseases and Global Health Radboud Institute for Health Sciences [Radboudumc 4], parasitic diseases
Abstract

Contains fulltext : 153785.pdf (Publisher’s version ) (Open Access) The transmission of malaria parasites depends on the presence of sexual stages (gametocytes) in the blood, making the ratio and densities of female and male gametocytes important determinants of parasite fitness. This manuscript describes the development of reverse transcriptase quantitative PCR (RT-qPCR) assays to separately quantify mature female and male gametocytes of the human malaria parasite Plasmodium falciparum, and reveals that Pfs25 mRNA is expressed only in female gametocytes. The female (Pfs25) and male (Pfs230p) gametocyte specific RT-qPCR assays have lower detection limits of 0.3 female and 1.8 male gametocytes per microlitre of blood, respectively, making them more sensitive than microscopy. Accurate quantification of the ratio and densities of female and male gametocytes will increase understanding of P. falciparum transmission and improve the evaluation of transmission blocking interventions.

Published
2015

16. Submicroscopic carriage of Plasmodium falciparum and Plasmodium vivax in a low endemic area in Ethiopia where no parasitaemia was detected by microscopy or rapid diagnostic test.

Author

Tadesse, F.G., Pett, H.E., Baidjoe, A., Lanke, K.H.W., Grignard, L., Sutherland, C., Hall, T., Drakeley, C.J., Bousema, T., Mamo, H., Tadesse, F.G., Pett, H.E., Baidjoe, A., Lanke, K.H.W., Grignard, L., Sutherland, C., Hall, T., Drakeley, C.J., Bousema, T., and Mamo, H.

Abstract

Contains fulltext : 154024.pdf (publisher's version ) (Open Access)

Published
2015

17. The RNA template channel of the RNA-dependent RNA polymerase as a target for development of antiviral therapy of multiple genera within a virus family.

Author

Linden, L. van der, Vives-Adrián, L., Selisko, B., Ferrer-Orta, C., Liu, X., Lanke, K.H.W., Ulferts, R., Palma, A.M. De, Tanchis, F., Goris, N., Lefebvre, D., Clercq, K. De, Leyssen, P., LaCroix, C., Pürstinger, G., Coutard, B., Canard, B., Boehr, D.D., Arnold, J.J., Cameron, C.E., Verdaguer, N., Neyts, J., Kuppeveld, F.J.M. van, Linden, L. van der, Vives-Adrián, L., Selisko, B., Ferrer-Orta, C., Liu, X., Lanke, K.H.W., Ulferts, R., Palma, A.M. De, Tanchis, F., Goris, N., Lefebvre, D., Clercq, K. De, Leyssen, P., LaCroix, C., Pürstinger, G., Coutard, B., Canard, B., Boehr, D.D., Arnold, J.J., Cameron, C.E., Verdaguer, N., Neyts, J., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 154135.PDF (publisher's version ) (Open Access)

Published
2015

18. Efficacy and safety of the mosquitocidal drug ivermectin to prevent malaria transmission after treatment: a double-blind, randomized, clinical trial

Author

Ouedraogo, A.L., Bastiaens, G.J.H., Tiono, A.B., Guelbeogo, W.M., Kobylinski, K.C., Barry, A., Bougouma, E.C., Nebie, I., Ouattara, M.S., Lanke, K.H.W., Fleckenstein, L., Sauerwein, R.W., Slater, H.C., Churcher, T.S., Sirima, S.B., Drakeley, C., Bousema, T., Ouedraogo, A.L., Bastiaens, G.J.H., Tiono, A.B., Guelbeogo, W.M., Kobylinski, K.C., Barry, A., Bougouma, E.C., Nebie, I., Ouattara, M.S., Lanke, K.H.W., Fleckenstein, L., Sauerwein, R.W., Slater, H.C., Churcher, T.S., Sirima, S.B., Drakeley, C., and Bousema, T.

Abstract

Item does not contain fulltext, BACKGROUND: Artemisinin combination therapy effectively clears asexual malaria parasites and immature gametocytes but does not prevent posttreatment malaria transmission. Ivermectin (IVM) may reduce malaria transmission by killing mosquitoes that take blood meals from IVM-treated humans. METHODS: In this double-blind, placebo-controlled trial, 120 asymptomatic Plasmodium falciparum parasite carriers were randomized to receive artemether-lumefantrine (AL) plus placebo or AL plus a single or repeated dose (200 microg/kg) of ivermectin (AL-IVM1 and AL-IVM2, respectively). Mosquito membrane feeding was performed 1, 3, and 7 days after initiation of treatment to determine Anopheles gambiae and Anopheles funestus survival and infection rates. RESULTS: The AL-IVM combination was well tolerated. IVM resulted in a 4- to 7-fold increased mortality in mosquitoes feeding 1 day after IVM (P < .001). Day 7 IVM plasma levels were positively associated with body mass index (r = 0.57, P < .001) and were higher in female participants (P = .003), for whom An. gambiae mosquito mortality was increased until 7 days after a single dose of IVM (hazard rate ratio, 1.34 [95% confidence interval, 1.07-1.69]; P = .012). Although we found no evidence that IVM reduced Plasmodium infection rates among surviving mosquitoes, the mosquitocidal effect of AL-IVM1 and AL-IVM2 resulted in 27% and 35% reductions, respectively, in estimated malaria transmission potential during the first week after initiation of treatment. CONCLUSIONS: We conclude that IVM can be safely given in combination with AL and can reduce the likelihood of malaria transmission by reducing the life span of feeding mosquitoes. CLINICAL TRIALS REGISTRATION: NCT0160325.

Published
2015

19. Itraconazole inhibits enterovirus replication by targeting the oxysterol-binding protein.

Author

Strating, J.R.P.M., Linden, L. van der, Albulescu, L., Bigay, J., Arita, M., Delang, L., Leyssen, P., Schaar, H.M. van der, Lanke, K.H.W., Thibaut, H.J., Ulferts, R., Drin, G., Schlinck, N., Wubbolts, R.W., Sever, N., Head, S.A., Liu, J.O., Beachy, P.A., Matteis, M.A. De, Shair, M.D., Olkkonen, V.M., Neyts, J., Kuppeveld, F.J.M. van, Strating, J.R.P.M., Linden, L. van der, Albulescu, L., Bigay, J., Arita, M., Delang, L., Leyssen, P., Schaar, H.M. van der, Lanke, K.H.W., Thibaut, H.J., Ulferts, R., Drin, G., Schlinck, N., Wubbolts, R.W., Sever, N., Head, S.A., Liu, J.O., Beachy, P.A., Matteis, M.A. De, Shair, M.D., Olkkonen, V.M., Neyts, J., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 153240.pdf (publisher's version ) (Open Access)

Published
2015

20. A comparison of Plasmodium falciparum circumsporozoite protein-based slot blot and ELISA immuno-assays for oocyst detection in mosquito homogenates.

Author

Stone, W.J.R., Grabias, B., Lanke, K.H.W., Zheng, H., Locke, E., Diallo, D., Birkett, A., Morin, M., Bousema, T., Kumar, S., Stone, W.J.R., Grabias, B., Lanke, K.H.W., Zheng, H., Locke, E., Diallo, D., Birkett, A., Morin, M., Bousema, T., and Kumar, S.

Abstract

Contains fulltext : 152039.pdf (publisher's version ) (Open Access)

Published
2015

21. Selective serotonin reuptake inhibitor fluoxetine inhibits replication of human enteroviruses B and D by targeting viral protein 2C

Author

Ulferts, R., Thibaut, H.J., Lanke, K.H.W., Leyssen, P., Coutard, B., De Palma, A.M., Canard, B., Neyts, J., van Kuppeveld, F.J.M., Strategic Infection Biology, Dep Infectieziekten Immunologie, and I&I SIB1

Subjects
Viral protein, Serotonin reuptake inhibitor, viruses, Coronacrisis-Taverne, Enterovirus D, Pharmacology, Biology, Viral Nonstructural Proteins, medicine.disease_cause, Antiviral Agents, Virus, 03 medical and health sciences, Poverty-related infectious diseases Infection and autoimmunity [N4i 3], Fluoxetine, medicine, Pharmacology (medical), Serotonin Uptake Inhibitors, 030304 developmental biology, Enterovirus D, Human, 0303 health sciences, 030306 microbiology, virus diseases, Pathogenesis and modulation of inflammation Infection and autoimmunity [N4i 1], Virology, digestive system diseases, 3. Good health, Enterovirus B, Human, Infectious Diseases, Enterovirus, Reuptake inhibitor, Carrier Proteins, Selective Serotonin Reuptake Inhibitors, medicine.drug
Abstract

Although the genus Enterovirus contains many important human pathogens, there is no licensed drug for either the treatment or the prophylaxis of enterovirus infections. We report that fluoxetine (Prozac)—a selective serotonin reuptake inhibitor—inhibits the replication of human enterovirus B (HEV-B) and HEV-D but does not affect the replication of HEV-A and HEV-C or human rhinovirus A or B. We show that fluoxetine interferes with viral RNA replication, and we identified viral protein 2C as the target of this compound.

Published
2013

22. The relevance and applicability of oocyst prevalence as a read-out for mosquito feeding assays

Author

Stone, W.J.R., Eldering, M., Gemert, G.J.A. van, Lanke, K.H.W., Grignard, L., Vegte-Bolmer, M.G. van de, Siebelink-Stoter, R., Graumans, W., Roeffen, W.F.G., Drakeley, C.J., Sauerwein, R.W., and Bousema, T.

Subjects
Poverty-related infectious diseases Infection and autoimmunity [N4i 3], GeneralLiterature_REFERENCE(e.g.,dictionaries,encyclopedias,glossaries)
Abstract

Contains fulltext : 126147.pdf (Publisher’s version ) (Open Access)

Published
2013

23. Prevalence of xenotropic murine leukaemia virus-related virus in patients with chronic fatigue syndrome in the Netherlands: retrospective analysis of samples from an established cohort

Author

Kuppeveld, F.J.M. van, Jong, A.S. de, Lanke, K.H.W., Verhaegh, G.W.C.T., Melchers, W.J.G., Swanink, C.M.A., Bleijenberg, G., Netea, M.G., Galama, J.M.D., and Meer, J.W.M. van der

Subjects
Pathogenesis and modulation of inflammation [N4i 1], Psychological determinants of chronic illness [NCEBP 8], Infection and autoimmunity [NCMLS 1]
Abstract

Contains fulltext : 89642.pdf (Publisher’s version ) (Open Access) OBJECTIVE: The presence of the retrovirus xenotropic murine leukaemia virus-related virus (XMRV) has been reported in peripheral blood mononuclear cells of patients with chronic fatigue syndrome. Considering the potentially great medical and social relevance of such a discovery, we investigated whether this finding could be confirmed in an independent European cohort of patients with chronic fatigue syndrome. DESIGN: Analysis of a well defined cohort of patients and matched neighbourhood controls by polymerase chain reaction. SETTING: Certified (ISO 15189) laboratory of clinical virology in a university hospital in the Netherlands. Population Between December 1991 and April 1992, peripheral blood mononuclear cells were isolated from 76 patients and 69 matched neighbourhood controls. In this study we tested cells from 32 patients and 43 controls from whom original cryopreserved phials were still available. MAIN OUTCOME MEASURES: Detection of XMRV in peripheral blood mononuclear cells by real time polymerase chain reaction assay targeting the XMRV integrase gene and/or a nested polymerase chain reaction assay targeting the XMRV gag gene. RESULTS: We detected no XMRV sequences in any of the patients or controls in either of the assays, in which relevant positive and negative isolation controls and polymerase chain reaction controls were included. Spiking experiments showed that we were able to detect at least 10 copies of XMRV sequences per 10(5) peripheral blood mononuclear cells by real time as well as by nested polymerase chain reaction, demonstrating high sensitivity of both assays. CONCLUSIONS: This study failed to show the presence of XMRV in peripheral blood mononuclear cells of patients with chronic fatigue syndrome from a Dutch cohort. These data cast doubt on the claim that XMRV is associated with chronic fatigue syndrome in the majority of patients.

Published
2010

24. A scalable assessment of Plasmodium falciparum transmission in the standard membrane-feeding assay, using transgenic parasites expressing green fluorescent protein-luciferase

Author

Stone, W.J.R., Churcher, T.S., Graumans, W., Gemert, G.J.A. van, Vos, M.W., Lanke, K.H.W., Vegte-Bolmer, M.G. van de, Siebelink-Stoter, R., Dechering, K.J., Vaughan, A.M., Camargo, N., Kappe, S.H., Sauerwein, R.W., Bousema, T., Stone, W.J.R., Churcher, T.S., Graumans, W., Gemert, G.J.A. van, Vos, M.W., Lanke, K.H.W., Vegte-Bolmer, M.G. van de, Siebelink-Stoter, R., Dechering, K.J., Vaughan, A.M., Camargo, N., Kappe, S.H., Sauerwein, R.W., and Bousema, T.

Abstract

Item does not contain fulltext, BACKGROUND: The development of drugs and vaccines to reduce malaria transmission is an important part of eradication plans. The transmission-reducing activity (TRA) of these agents is currently determined in the standard membrane-feeding assay (SMFA), based on subjective microscopy-based readouts and with limitations in upscaling and throughput. METHODS: Using a Plasmodium falciparum strain expressing the firefly luciferase protein, we present a luminescence-based approach to SMFA evaluation that eliminates the requirement for mosquito dissections in favor of a simple approach in which whole mosquitoes are homogenized and examined directly for luciferase activity. RESULTS: Analysis of 6860 Anopheles stephensi mosquitoes across 68 experimental feeds shows that the luminescence assay was as sensitive as microscopy for infection detection. The mean luminescence intensity of individual and pooled mosquitoes accurately quantifies mean oocyst intensity and generates comparable TRA estimates. The luminescence assay presented here could increase SMFA throughput so that 10-30 experimental feeds could be evaluated in a single 96-well plate. CONCLUSIONS: This new method of assessing Plasmodium infection and transmission intensity could expedite the screening of novel drug compounds, vaccine candidates, and sera from malaria-exposed individuals for TRA. Luminescence-based estimates of oocyst intensity in individual mosquitoes should be interpreted with caution.

Published
2014

26. Application of a cell-based protease assay for testing inhibitors of picornavirus 3C proteases

Author

Linden, L. van der, Ulferts, R., Nabuurs, S.B., Kusov, Y., Liu, H., George, S., LaCroix, C., Goris, N., Lefebvre, D., Lanke, K.H.W., Clercq, K. De, Hilgenfeld, R., Neyts, J., Kuppeveld, F.J.M. van, Linden, L. van der, Ulferts, R., Nabuurs, S.B., Kusov, Y., Liu, H., George, S., LaCroix, C., Goris, N., Lefebvre, D., Lanke, K.H.W., Clercq, K. De, Hilgenfeld, R., Neyts, J., and Kuppeveld, F.J.M. van

Abstract

Item does not contain fulltext, Proteolytical cleavage of the picornaviral polyprotein is essential for viral replication. Therefore, viral proteases are attractive targets for anti-viral therapy. Most assays available for testing proteolytical activity of proteases are performed in vitro, using heterologously expressed proteases and peptide substrates. To deal with the disadvantages associated with in vitro assays, we modified a cell-based protease assay for picornavirus proteases. The assay is based on the induction of expression of a firefly luciferase reporter by a chimeric transcription factor in which the viral protease and cleavage sites are inserted between the GAL4 binding domain and the VP16 activation domain. Firefly luciferase expression is dependent on cleavage of the transcription factor by the viral protease. This biosafe assay enables testing the effect of compounds on protease activity in cells while circumventing the need for infection. We designed the assay for 3C proteases (3C(pro)) of various enteroviruses as well as of viruses of several other picornavirus genera, and show that the assay is amenable for use in a high-throughput setting. Furthermore, we show that the spectrum of activity of 3C(pro) inhibitor AG7088 (rupintrivir) not only encompasses enterovirus 3C(pro) but also 3C(pro) of foot-and-mouth disease virus (FMDV), an aphthovirus. In contrary, AG7404 (compound 1), an analogue of AG7088, had no effect on FMDV 3C(pro) activity, for which we provide a structural explanation.

Published
2014

27. Single dose primaquine for clearance of Plasmodium falciparum gametocytes in children with uncomplicated malaria in Uganda: a randomised, controlled, double-blind, dose-ranging trial.

Author

Eziefula, A.C., Bousema, T., Yeung, S., Kamya, M., Owaraganise, A., Gabagaya, G., Bradley, J., Grignard, L., Lanke, K.H.W., Wanzira, H., Mpimbaza, A., Nsobya, S., White, N.J., Webb, E.L., Staedke, S.G., Drakeley, C., Eziefula, A.C., Bousema, T., Yeung, S., Kamya, M., Owaraganise, A., Gabagaya, G., Bradley, J., Grignard, L., Lanke, K.H.W., Wanzira, H., Mpimbaza, A., Nsobya, S., White, N.J., Webb, E.L., Staedke, S.G., and Drakeley, C.

Abstract

Contains fulltext : 136831.pdf (publisher's version ) (Open Access)

Published
2014

28. Saffold cardiovirus and multiple sclerosis: no evidence for an association

Author

Galama, J.M.D., Zoll, J.G., Lanke, K.H.W., Jong, A.S. de, Melief, J., Huitinga, I., Verbeek, M.M., Kuppeveld, F.J.M. van, Galama, J.M.D., Zoll, J.G., Lanke, K.H.W., Jong, A.S. de, Melief, J., Huitinga, I., Verbeek, M.M., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 138713.pdf (publisher's version ) (Open Access), Saffold cardiovirus, a newly discovered human cardiovirus, has close similarity with Theiler's murine encephalomyelitis virus (TMEV) which can cause a chronic demyelinating encephalomyelitis in mice. In this study, we tested whether Saffold cardiovirus infection of the brain is associated with multiple sclerosis (MS). Autopsy white matter samples from 19 MS and 9 normal brain donors were tested by polymerase chain reaction. All were negative. Paired cerebrospinal fluid and serum samples from 24 MS patients and 27 controls were tested for Saffold cardiovirus-specific oligoclonal bands, two patients and two controls reacted positive. We conclude that an association between Saffold cardiovirus and MS is highly improbable.

Published
2014

29. Enterovirus 2Apro targets MDA5 and MAVS in infected cells

Author

Feng, Q., Langereis, M.A., Lork, M., Nguyen, M.H., Hato, S.V., Lanke, K.H.W., Emdad, L., Bhoopathi, P., Fisher, P.B., Lloyd, R.E., Kuppeveld, F.J.M. van, Feng, Q., Langereis, M.A., Lork, M., Nguyen, M.H., Hato, S.V., Lanke, K.H.W., Emdad, L., Bhoopathi, P., Fisher, P.B., Lloyd, R.E., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 137931.pdf (publisher's version ) (Open Access), RIG-I-like receptors (RLRs) MDA5 and RIG-I are key players in the innate antiviral response. Upon recognition of viral RNA, they interact with MAVS, eventually inducing type I interferon production. The interferon induction pathway is commonly targeted by viruses. How enteroviruses suppress interferon production is incompletely understood. MDA5 has been suggested to undergo caspase- and proteasome-mediated degradation during poliovirus infection. Additionally, MAVS is reported to be cleaved during infection with coxsackievirus B3 (CVB3) by the CVB3 proteinase 3C(pro), whereas MAVS cleavage by enterovirus 71 has been attributed to 2A(pro). As yet, a detailed examination of the RLR pathway as a whole during any enterovirus infection is lacking. We performed a comprehensive analysis of crucial factors of the RLR pathway, including MDA5, RIG-I, LGP2, MAVS, TBK1, and IRF3, during infection of CVB3, a human enterovirus B (HEV-B) species member. We show that CVB3 inhibits the RLR pathway upstream of TBK1 activation, as demonstrated by limited phosphorylation of TBK1 and a lack of IRF3 phosphorylation. Furthermore, we show that MDA5, MAVS, and RIG-I all undergo proteolytic degradation in CVB3-infected cells through a caspase- and proteasome-independent manner. We convincingly show that MDA5 and MAVS cleavages are both mediated by CVB3 2A(pro), while RIG-I is cleaved by 3C(pro). Moreover, we show that proteinases 2A(pro) and 3C(pro) of poliovirus (HEV-C) and enterovirus 71 (HEV-A) exert the same functions. This study identifies a critical role of 2A(pro) by cleaving MDA5 and MAVS and shows that enteroviruses use a common strategy to counteract the interferon response in infected cells. IMPORTANCE: Human enteroviruses (HEVs) are important pathogens that cause a variety of diseases in humans, including poliomyelitis, hand, foot, and mouth disease, viral meningitis, cardiomyopathy, and more. Like many other viruses, enteroviruses target the host immune pathways to gain replicat

Published
2014

30. Structure-function analysis of the coxsackievirus protein 3A: identification of residues important for dimerization, viral rna replication, and transport inhibition

Author

Wessels, E., Notebaart, R.A., Duijsings, D.M., Lanke, K.H.W., Vergeer, B., Melchers, W.J.G., and Kuppeveld, F.J.M. van

Subjects
Pathogenesis and modulation of inflammation [N4i 1], Invasive mycoses and compromised host [N4i 2], Bioinformatics, viruses, Poverty-related infectious diseases [N4i 3], Microbial pathogenesis and host defense [UMCN 4.1], Cellular energy metabolism [UMCN 5.3], Infection and autoimmunity [NCMLS 1], Immunity, infection and tissue repair [NCMLS 1]
Abstract

Contains fulltext : 35369.pdf (Publisher’s version ) (Open Access) The coxsackievirus B3 3A protein forms homodimers and plays important roles in both viral RNA (vRNA) replication and the viral inhibition of intracellular protein transport. The molecular determinants that are required for each of these functions are yet poorly understood. Based on the NMR structure of the closely related poliovirus 3A protein, a molecular model of the coxsackievirus B3 3A protein was constructed. Using this structural model, specific mutants were designed to study the structure-function relationship of 3A. The mutants were tested for their capacity to dimerize, support vRNA replication, and block protein transport. A hydrophobic interaction between the monomers and an intermolecular salt bridge were identified as major determinants required for dimerization. We show that dimerization is important for both efficient vRNA replication and inhibition of protein transport. In addition, determinants were identified that were not required for dimerization but that were essential for either one of the biological functions of 3A. The combination of the in silico and in vivo results obtained in this study provides important insights in both the structural and functional aspects of 3A.

Published
2006

31. A novel, broad-spectrum inhibitor of enterovirus replication that targets host cell factor phosphatidylinositol 4-kinase IIIβ.

Author

Schaar, H.M. van der, Leyssen, P., Thibaut, H.J., Palma, A., Linden, L. van der, Lanke, K.H.W., LaCroix, C., Verbeken, E., Conrath, K., MacLeod, A.M., Mitchell, D.R., Palmer, N.J., Poël, H. van de, Andrews, M., Neyts, J., Kuppeveld, F.J.M. van, Schaar, H.M. van der, Leyssen, P., Thibaut, H.J., Palma, A., Linden, L. van der, Lanke, K.H.W., LaCroix, C., Verbeken, E., Conrath, K., MacLeod, A.M., Mitchell, D.R., Palmer, N.J., Poël, H. van de, Andrews, M., Neyts, J., and Kuppeveld, F.J.M. van

Abstract

Item does not contain fulltext

Published
2013

32. Selective serotonin reuptake inhibitor fluoxetine inhibits replication of human enterovirus B and D by targeting viral protein 2C

Author

Strategic Infection Biology, Dep Infectieziekten Immunologie, I&I SIB1, Ulferts, R., Thibaut, H.J., Lanke, K.H.W., Leyssen, P., Coutard, B., De Palma, A.M., Canard, B., Neyts, J., van Kuppeveld, F.J.M., Strategic Infection Biology, Dep Infectieziekten Immunologie, I&I SIB1, Ulferts, R., Thibaut, H.J., Lanke, K.H.W., Leyssen, P., Coutard, B., De Palma, A.M., Canard, B., Neyts, J., and van Kuppeveld, F.J.M.

Published
2013

33. Coxsackievirus mutants that can bypass host factor PI4KIIIbeta and the need for high levels of PI4P lipids for replication

Author

van der Schaar, H.M., van der Linden, L., Lanke, K.H.W., Strating, J.R.P.M., Purstinger, G., Vries, E. De, de Haan, C.A., Neyts, J., Kuppeveld, F.J.M. van, van der Schaar, H.M., van der Linden, L., Lanke, K.H.W., Strating, J.R.P.M., Purstinger, G., Vries, E. De, de Haan, C.A., Neyts, J., and Kuppeveld, F.J.M. van

Abstract

Item does not contain fulltext, RNA viruses can rapidly mutate and acquire resistance to drugs that directly target viral enzymes, which poses serious problems in a clinical context. Therefore, there is a growing interest in the development of antiviral drugs that target host factors critical for viral replication, since they are unlikely to mutate in response to therapy. We recently demonstrated that phosphatidylinositol-4-kinase IIIbeta (PI4KIIIbeta) and its product phosphatidylinositol-4-phosphate (PI4P) are essential for replication of enteroviruses, a group of medically important RNA viruses including poliovirus (PV), coxsackievirus, rhinovirus, and enterovirus 71. Here, we show that enviroxime and GW5074 decreased PI4P levels at the Golgi complex by directly inhibiting PI4KIIIbeta. Coxsackievirus mutants resistant to these inhibitors harbor single point mutations in the non-structural protein 3A. These 3A mutations did not confer compound-resistance by restoring the activity of PI4KIIIbeta in the presence of the compounds. Instead, replication of the mutant viruses no longer depended on PI4KIIIbeta, since their replication was insensitive to siRNA-mediated depletion of PI4KIIIbeta. The mutant viruses also did not rely on other isoforms of PI4K. Consistently, no high level of PI4P could be detected at the replication sites induced by the mutant viruses in the presence of the compounds. Collectively, these findings indicate that through specific single point mutations in 3A, CVB3 can bypass an essential host factor and lipid for its propagation, which is a new example of RNA viruses acquiring resistance against antiviral compounds, even when they directly target host factors.

Published
2012

34. Cytokine and chemokine production by human pancreatic islets upon enterovirus infection.

Author

Schulte, B.M., Lanke, K.H.W., Piganelli, J.D., Kers-Rebel, E.D., Bottino, R., Trucco, M., Huijbens, R.J.F., Radstake, T.R.D.J., Engelse, M.A., Koning, E.J. de, Galama, J.M.D., Adema, G.J., Kuppeveld, F.J.M. van, Schulte, B.M., Lanke, K.H.W., Piganelli, J.D., Kers-Rebel, E.D., Bottino, R., Trucco, M., Huijbens, R.J.F., Radstake, T.R.D.J., Engelse, M.A., Koning, E.J. de, Galama, J.M.D., Adema, G.J., and Kuppeveld, F.J.M. van

Abstract

1 augustus 2012, Item does not contain fulltext, Enteroviruses of the human enterovirus B species (HEV-Bs) (e.g., coxsackie B viruses [CVBs] and echoviruses) have been implicated as environmental factors that trigger/accelerate type 1 diabetes, but the underlying mechanism remains elusive. The aim of this study was to gain insight into the cytokines and chemokines that are produced by human pancreatic islets upon infection with CVBs. To this end, we studied the response of human islets of Langerhans upon mock or CVB3 infection. Using quantitative PCR, we showed that upon CVB3 infection, transcription of interferon (IFN), IFN-stimulated genes, and inflammatory genes was induced. Analysis of secreted cytokines and chemokines by Luminex technology confirmed production and secretion of proinflammatory cytokines (e.g., interleukin [IL]-6 and tumor necrosis factor-alpha) as well as various chemotactic proteins, such as IFN-gamma-induced protein 10, macrophage inflammatory protein (MIP)-1alpha, MIP-1beta, and IL-8. Infection with other HEV-Bs induced similar responses, yet their extent depended on replication efficiency. Ultra violet-inactivated CVB3 did not induce any response, suggesting that virus replication is a prerequisite for antiviral responses. Our data represent the first comprehensive overview of inflammatory mediators that are secreted by human islets of Langerhans upon CVB infection and may shed light on the role of enteroviruses in type 1 diabetes pathogenesis.

Published
2012

35. Seroepidemiology of Saffold cardiovirus type 2

Author

Galama, J.M.D., Lanke, K.H.W., Zoll, J., Roivainen, M., Kuppeveld, F.J.M. van, Galama, J.M.D., Lanke, K.H.W., Zoll, J., Roivainen, M., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 93841.pdf (publisher's version ) (Open Access)

Published
2011

36. Differential effects of the putative GBF1 inhibitors Golgicide A and AG1478 on enterovirus replication.

Author

Linden, L. van der, Schaar, H.M. van der, Lanke, K.H.W., Neyts, J., Kuppeveld, F.J.M. van, Linden, L. van der, Schaar, H.M. van der, Lanke, K.H.W., Neyts, J., and Kuppeveld, F.J.M. van

Abstract

01 augustus 2010, Contains fulltext : 88880.pdf (publisher's version ) (Open Access), The genus Enterovirus, belonging to the family Picornaviridae, includes well-known pathogens, such as poliovirus, coxsackievirus, and rhinovirus. Brefeldin A (BFA) impedes replication of several enteroviruses through inhibition of Golgi-specific BFA resistance factor 1 (GBF1), a regulator of secretory pathway integrity and transport. GBF1 mediates the GTP exchange of Arf1, which in activated form recruits coatomer protein complex I (COP-I) to Golgi vesicles, a process important in transport between the endoplasmic reticulum and Golgi vesicles. Recently, the drugs AG1478 and Golgicide A (GCA) were put forward as new inhibitors of GBF1. In this study, we investigated the effects of these putative GBF1 inhibitors on secretory pathway function and enterovirus replication. We show that both drugs induced fragmentation of the Golgi vesicles and caused dissociation of Arf1 and COP-I from Golgi membranes, yet they differed in their effect on GBF1 localization. The effects of AG1478, but not those of GCA, could be countered by overexpression of Arf1, indicating a difference in their molecular mechanism of action. Consistent with this idea, we observed that GCA drastically reduced replication of coxsackievirus B3 (CVB3) and other human enterovirus species, whereas AG1478 had no effect at all on enterovirus replication. Time-of-addition studies and analysis of RNA replication using a subgenomic replicon both showed that GCA suppresses RNA replication of CVB3, which could be countered by overexpression of GBF1. These results indicate that, in contrast to AG1478, GCA inhibits CVB3 RNA replication by targeting GBF1. AG1478 and GCA may be valuable tools to further dissect enterovirus replication.

Published
2010

37. Detection of enterovirus RNA in peripheral blood mononuclear cells of type 1 diabetic patients beyond the stage of acute infection.

Author

Schulte, B.M., Bakkers, J.M.J.E., Lanke, K.H.W., Melchers, W.J.G., Westerlaken, C., Allebes, W.A., Aanstoot, H.J., Bruining, G.J., Adema, G.J., Kuppeveld, F.J.M. van, Galama, J.M.D., Schulte, B.M., Bakkers, J.M.J.E., Lanke, K.H.W., Melchers, W.J.G., Westerlaken, C., Allebes, W.A., Aanstoot, H.J., Bruining, G.J., Adema, G.J., Kuppeveld, F.J.M. van, and Galama, J.M.D.

Abstract

1 februari 2010, Contains fulltext : 88377.pdf (publisher's version ) (Open Access), Previous studies have shown that enteroviral RNA can be detected in blood at the onset of type 1 diabetes (T1D). The infection may play a role in triggering T1D and genetic host factors may contribute to this process. We investigated (1) whether enterovirus is present at the onset of T1D in peripheral blood mononuclear cells (PBMC), plasma, throat, or stool, and (2) whether enteroviral presence is linked with HLA-DR type and/or polymorphisms in melanoma differentiation-associated gene 5 (MDA5) and 2'-5' oligoadenylate synthetase 1 (OAS1), factors of antiviral immunity. To this end, PBMC, plasma, throat, and stool samples from 10 T1D patients and 20 unrelated controls were tested for the presence of enteroviruses (RT-PCR), for HLA-DR type, and polymorphisms in MDA5 and OAS1. Enterovirus RNA was detected in PBMC of 4/10 T1D patients, but none of 20 controls. Plasma was positive in 2/10 T1D patients and none of 20 controls, suggesting that enteroviruses found at the onset of T1D are mainly present in PBMC. All throat samples from positive T1D patients were virus-negative and only 1 fecal sample was positive. The negative results for all throat and most stool samples argues against acute infection. Enterovirus presence was linked with HLA-DR4, but not with polymorphisms in MDA5 or OAS1.

Published
2010

38. Phagocytosis of enterovirus-infected pancreatic beta-cells triggers innate immune responses in human dendritic cells.

Author

Schulte, B.M., Kramer, M., Ansems, M., Lanke, K.H.W., Doremalen, N. van, Piganelli, J.D., Bottino, R., Trucco, M., Galama, J.M.D., Adema, G.J., Kuppeveld, F.J.M. van, Schulte, B.M., Kramer, M., Ansems, M., Lanke, K.H.W., Doremalen, N. van, Piganelli, J.D., Bottino, R., Trucco, M., Galama, J.M.D., Adema, G.J., and Kuppeveld, F.J.M. van

Abstract

1 mei 2010, Contains fulltext : 89763.pdf (publisher's version ) (Closed access), OBJECTIVE: Type 1 diabetes is a chronic endocrine disorder in which enteroviruses, such as coxsackie B viruses and echoviruses, are possible environmental factors that can trigger or accelerate disease. The development or acceleration of type 1 diabetes depends on the balance between autoreactive effector T-cells and regulatory T-cells. This balance is particularly influenced by dendritic cells (DCs). The goal of this study was to investigate the interaction between enterovirus-infected human pancreatic islets and human DCs. RESEARCH DESIGN AND METHODS: In vitro phagocytosis of human or porcine primary islets or Min6 mouse insuloma cells by DCs was investigated by flow cytometry and confocal analysis. Subsequent innate DC responses were monitored by quantitative PCR and Western blotting of interferon-stimulated genes (ISGs). RESULTS: In this study, we show that both mock- and coxsackievirus B3 (CVB3)-infected human and porcine pancreatic islets were efficiently phagocytosed by human monocyte-derived DCs. Phagocytosis of CVB3-infected, but not mock-infected, human and porcine islets resulted in induction of ISGs in DCs, including the retinoic acid-inducible gene (RIG)-I-like helicases (RLHs), RIG-I, and melanoma differentiation-associated gene 5 (Mda5). Studies with murine Min6 insuloma cells, which were also efficiently phagocytosed, revealed that increased ISG expression in DCs upon encountering CVB-infected cells resulted in an antiviral state that protected DCs from subsequent enterovirus infection. The observed innate antiviral responses depended on RNA within the phagocytosed cells, required endosomal acidification, and were type I interferon dependent. CONCLUSIONS: Human DCs can phagocytose enterovirus-infected pancreatic cells and subsequently induce innate antiviral responses, such as induction of RLHs. These responses may have important consequences for immune homeostasis in vivo and may play a role in the etiology of type 1 diabetes.

Published
2010

39. GBF1, a guanine nucleotide exchange factor for Arf, is crucial for coxsackievirus B3 RNA replication.

Author

Lanke, K.H.W., Schaar, H.M. van der, Belov, G.A., Feng, Q., Duijsings, D., Jackson, C.L., Ehrenfeld, E., Kuppeveld, F.J.M. van, Lanke, K.H.W., Schaar, H.M. van der, Belov, G.A., Feng, Q., Duijsings, D., Jackson, C.L., Ehrenfeld, E., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 80659.pdf (publisher's version ) (Open Access), The replication of enteroviruses is sensitive to brefeldin A (BFA), an inhibitor of endoplasmic reticulum-to-Golgi network transport that blocks activation of guanine exchange factors (GEFs) of the Arf GTPases. Mammalian cells contain three BFA-sensitive Arf GEFs: GBF1, BIG1, and BIG2. Here, we show that coxsackievirus B3 (CVB3) RNA replication is insensitive to BFA in MDCK cells, which contain a BFA-resistant GBF1 due to mutation M832L. Further evidence for a critical role of GBF1 stems from the observations that viral RNA replication is inhibited upon knockdown of GBF1 by RNA interference and that replication in the presence of BFA is rescued upon overexpression of active, but not inactive, GBF1. Overexpression of Arf proteins or Rab1B, a GTPase that induces GBF1 recruitment to membranes, failed to rescue RNA replication in the presence of BFA. Additionally, the importance of the interaction between enterovirus protein 3A and GBF1 for viral RNA replication was investigated. For this, the rescue from BFA inhibition of wild-type (wt) replicons and that of mutant replicons of both CVB3 and poliovirus (PV) carrying a 3A protein that is impaired in binding GBF1 were compared. The BFA-resistant GBF1-M832L protein efficiently rescued RNA replication of both wt and mutant CVB3 and PV replicons in the presence of BFA. However, another BFA-resistant GBF1 protein, GBF1-A795E, also efficiently rescued RNA replication of the wt replicons, but not that of mutant replicons, in the presence of BFA. In conclusion, this study identifies a critical role for GBF1 in CVB3 RNA replication, but the importance of the 3A-GBF1 interaction requires further study.

Published
2009

40. Mutations in the nonstructural protein 3A confer resistance to the novel enterovirus replication inhibitor TTP-8307.

Author

Palma, A.M. De, Thibaut, H.J., Linden, L. van der, Lanke, K.H.W., Heggermont, W., Ireland, S., Andrews, R., Arimilli, M., Al-Tel, T.H., Clercq, E. De, Kuppeveld, F.J.M. van, Neyts, J., Palma, A.M. De, Thibaut, H.J., Linden, L. van der, Lanke, K.H.W., Heggermont, W., Ireland, S., Andrews, R., Arimilli, M., Al-Tel, T.H., Clercq, E. De, Kuppeveld, F.J.M. van, and Neyts, J.

Abstract

Contains fulltext : 79778.pdf (publisher's version ) (Open Access), A novel compound, TTP-8307, was identified as a potent inhibitor of the replication of several rhino- and enteroviruses. TTP-8307 inhibits viral RNA synthesis in a dose-dependent manner, without affecting polyprotein synthesis and/or processing. Drug-resistant variants of coxsackievirus B3 were all shown to carry at least one amino acid mutation in the nonstructural protein 3A. In particular, three mutations located in a nonstructured region preceding the hydrophobic domain (V45A, I54F, and H57Y) appeared to contribute to the drug-resistant phenotype. This region has previously been identified as a hot sport for mutations that resulted in resistance to enviroxime, the sole 3A-targeting enterovirus inhibitor reported thus far. This was corroborated by the fact that TTP-8307 and enviroxime proved cross-resistant. It is hypothesized that TTP-8307 and enviroxime disrupt proper interactions of 3A(B) with other viral or cellular proteins that are required for efficient replication.

Published
2009

41. Saffold virus, a human Theiler's-like cardiovirus, is ubiquitous and causes infection early in life.

Author

Zoll, J., Erkens Hulshof, S., Lanke, K.H.W., Verduyn Lunel, F.M., Melchers, W.J.G., Schoondermark-van de Ven, E.M.E., Roivainen, M., Galama, J.M.D., Kuppeveld, F.J.M. van, Zoll, J., Erkens Hulshof, S., Lanke, K.H.W., Verduyn Lunel, F.M., Melchers, W.J.G., Schoondermark-van de Ven, E.M.E., Roivainen, M., Galama, J.M.D., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 81623.pdf (publisher's version ) (Open Access), The family Picornaviridae contains well-known human pathogens (e.g., poliovirus, coxsackievirus, rhinovirus, and parechovirus). In addition, this family contains a number of viruses that infect animals, including members of the genus Cardiovirus such as Encephalomyocarditis virus (EMCV) and Theiler's murine encephalomyelits virus (TMEV). The latter are important murine pathogens that cause myocarditis, type 1 diabetes and chronic inflammation in the brains, mimicking multiple sclerosis. Recently, a new picornavirus was isolated from humans, named Saffold virus (SAFV). The virus is genetically related to Theiler's virus and classified as a new species in the genus Cardiovirus, which until the discovery of SAFV did not contain human viruses. By analogy with the rodent cardioviruses, SAFV may be a relevant new human pathogen. Thus far, SAFVs have sporadically been detected by molecular techniques in respiratory and fecal specimens, but the epidemiology and clinical significance remained unclear. Here we describe the first cultivated SAFV type 3 (SAFV-3) isolate, its growth characteristics, full-length sequence, and epidemiology. Unlike the previously isolated SAFV-1 and -2 viruses, SAFV-3 showed efficient growth in several cell lines with a clear cytopathic effect. The latter allowed us to conduct a large-scale serological survey by a virus-neutralization assay. This survey showed that infection by SAFV-3 occurs early in life (>75% positive at 24 months) and that the seroprevalence reaches >90% in older children and adults. Neutralizing antibodies were found in serum samples collected in several countries in Europe, Africa, and Asia. In conclusion, this study describes the first cultivated SAFV-3 isolate, its full-length sequence, and epidemiology. SAFV-3 is a highly common and widespread human virus causing infection in early childhood. This finding has important implications for understanding the impact of these ubiquitous viruses and their possible role in acute and

Published
2009

42. Antiviral activity of the zinc ionophores pyrithione and hinokitiol against picornavirus infections.

Author

Krenn, B.M., Gaudernak, E., Holzer, B., Lanke, K.H.W., Kuppeveld, F.J.M. van, Seipelt, J., Krenn, B.M., Gaudernak, E., Holzer, B., Lanke, K.H.W., Kuppeveld, F.J.M. van, and Seipelt, J.

Abstract

Contains fulltext : 80130.pdf (publisher's version ) (Closed access), We have discovered two metal ion binding compounds, pyrithione (PT) and hinokitiol (HK), that efficiently inhibit human rhinovirus, coxsackievirus, and mengovirus multiplication. Early stages of virus infection are unaffected by these compounds. However, the cleavage of the cellular eukaryotic translation initiation factor eIF4GI by the rhinoviral 2A protease was abolished in the presence of PT and HK. We further show that these compounds inhibit picornavirus replication by interfering with proper processing of the viral polyprotein. In addition, we provide evidence that these structurally unrelated compounds lead to a rapid import of extracellular zinc ions into cells. Imported Zn(2+) was found to be localized in punctate structures, as well as in mitochondria. The observed elevated level of zinc ions was reversible when the compounds were removed. As the antiviral activity of these compounds requires the continuous presence of the zinc ionophore PT, HK, or pyrrolidine-dithiocarbamate, the requirement for zinc ions for the antiviral activity is further substantiated. Therefore, an increase in intracellular zinc levels provides the basis for a new antipicornavirus mechanism.

Published
2009

43. Differential membrane association properties and regulation of class I and class II Arfs.

Author

Duijsings, D., Lanke, K.H.W., Dooren, S.H. van, Dommelen, M.M. van, Wetzels, R., Mattia, F.P. de, Wessels, E., Kuppeveld, F.J.M. van, Duijsings, D., Lanke, K.H.W., Dooren, S.H. van, Dommelen, M.M. van, Wetzels, R., Mattia, F.P. de, Wessels, E., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 80476.pdf (publisher's version ) (Closed access), ADP-ribosylation factor (Arf) proteins are small guanosine triphosphatases (GTPases) that act as major regulators of intracellular vesicular trafficking and secretory organelle pathway integrity. Like all small monomeric GTPases, Arf proteins cycle between a GDP-bound and a GTP-bound state, and this cycling is catalysed by guanine nucleotide exchange factors (GEFs) and GTPase-activating proteins. While the class I Arfs, especially Arf1, have been studied extensively, little is known as yet about the function and regulation of class II Arfs, Arf4 and Arf5. In this study, we show that Arf proteins show class-specific dynamic behaviour. Moreover, unlike class I Arfs, membrane association of class II Arfs is resistant to inhibition of large Arf GEFs by Brefeldin A. Through the construction of Arf chimeric proteins, evidence is provided that the N-terminal amphipathic helix and a class-specific residue in the conserved interswitch domain determine the membrane-binding properties of class I and class II Arf proteins. Our results show that fundamental differences exist in behaviour and regulation of these small GTPases.

Published
2009

44. Phagocytosis of picornavirus-infected cells induces an RNA-dependent antiviral state in human dendritic cells.

Author

Kramer, M., Schulte, B.M., Toonen, L.W.J., Barral, P.M., Fisher, P.B., Lanke, K.H.W., Galama, J.M.D., Kuppeveld, F.J.M. van, Adema, G.J., Kramer, M., Schulte, B.M., Toonen, L.W.J., Barral, P.M., Fisher, P.B., Lanke, K.H.W., Galama, J.M.D., Kuppeveld, F.J.M. van, and Adema, G.J.

Abstract

Contains fulltext : 71489.pdf (publisher's version ) (Closed access), Dendritic cells (DCs) play a central role in instructing antiviral immune responses. DCs, however, can become targeted by different viruses themselves. We recently demonstrated that human DCs can be productively infected with echoviruses (EVs), but not coxsackie B viruses (CVBs), both of which are RNA viruses belonging to the Enterovirus genus of the Picornaviridae family. We now show that phagocytosis of CVB-infected, type I interferon-deficient cells induces an antiviral state in human DCs. Uptake of infected cells increased the expression of the cytoplasmic RNA helicases retinoic acid-inducible gene I and melanoma differentiation-associated gene 5 as well as other interferon-stimulated genes and protected DCs against subsequent infection with EV9. These effects depended on recognition of viral RNA and could be mimicked by exposure to the synthetic double-stranded RNA analogue poly(I:C) but not other Toll-like receptor (TLR) ligands. Blocking endosomal acidification abrogated protection, suggesting a role for TLRs in the acquisition of an antiviral state in DCs. In conclusion, recognition of viral RNA rapidly induces an antiviral state in human DCs. This might provide a mechanism by which DCs protect themselves against viruses when attracted to an environment with ongoing infection.

Published
2008

45. Functional analysis of picornavirus 2B proteins: effects on calcium homeostasis and intracellular protein trafficking.

Author

Jong, A.S. de, Mattia, F.P. de, Dommelen, M.M.T. van, Lanke, K.H.W., Melchers, W.J.G., Willems, P.H.G.M., Kuppeveld, F.J.M. van, Jong, A.S. de, Mattia, F.P. de, Dommelen, M.M.T. van, Lanke, K.H.W., Melchers, W.J.G., Willems, P.H.G.M., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 70251.pdf (publisher's version ) (Open Access), The family Picornaviridae consists of a large group of plus-strand RNA viruses that share a similar genome organization. The nomenclature of the picornavirus proteins is based on their position in the viral RNA genome but does not necessarily imply a conserved function of proteins of different genera. The enterovirus 2B protein is a small hydrophobic protein that, upon individual expression, is localized to the endoplasmic reticulum (ER) and the Golgi complex, reduces ER and Golgi complex Ca(2+) levels, most likely by forming transmembrane pores, and inhibits protein trafficking through the Golgi complex. At present, little is known about the function of the other picornavirus 2B proteins. Here we show that rhinovirus 2B, which is phylogenetically closely related to enterovirus 2B, shows a similar subcellular localization and function to those of enterovirus 2B. In contrast, 2B proteins of hepatitis A virus, foot-and-mouth disease virus, and encephalomyocarditis virus, all of which are more distantly related to enteroviruses, show a different localization and have little, if any, effects on Ca(2+) homeostasis and intracellular protein trafficking. Our data suggest that the 2B proteins of enterovirus and rhinovirus share the same function in virus replication, while the other picornavirus 2B proteins support the viral life cycle in a different manner. Moreover, we show that an enterovirus 2B protein that is retained in the ER is unable to modify Ca(2+) homeostasis and inhibit protein trafficking, demonstrating the importance of Golgi complex localization for its functioning.

Published
2008

46. The thiazolobenzimidazole TBZE-029 inhibits enterovirus replication by targeting a short region immediately downstream from motif C in the nonstructural protein 2C.

Author

Palma, A.M. De, Heggermont, W., Lanke, K.H.W., Coutard, B., Bergmann, M., Monforte, A.M., Canard, B., Clercq, E. De, Chimirri, A., Purstinger, G., Rohayem, J., Kuppeveld, F.J.M. van, Neyts, J., Palma, A.M. De, Heggermont, W., Lanke, K.H.W., Coutard, B., Bergmann, M., Monforte, A.M., Canard, B., Clercq, E. De, Chimirri, A., Purstinger, G., Rohayem, J., Kuppeveld, F.J.M. van, and Neyts, J.

Abstract

Contains fulltext : 70668.pdf (publisher's version ) (Open Access), TBZE-029 {1-(2,6-difluorophenyl)-6-trifluoromethyl-1H,3H-thiazolo[3,4-a]benzimidazole} is a novel selective inhibitor of the replication of several enteroviruses. We show that TBZE-029 exerts its antiviral activity through inhibition of viral RNA replication, without affecting polyprotein processing. To identify the viral target of TBZE-029, drug-resistant coxsackievirus B3 (CVB3) was selected. Genotyping of resistant clones led to the identification of three amino acid mutations in nonstructural protein 2C, clustered at amino acid positions 224, 227, and 229, immediately downstream of NTPase/helicase motif C. The mutations were reintroduced, either alone or combined, into an infectious full-length CVB3 clone. In particular the mutations at positions 227 and 229 proved essential for the altered sensitivity of CVB3 to TBZE-029. Resistant virus exhibited cross-resistance to the earlier-reported antienterovirus agents targeting 2C, namely, guanidine hydrochloride, HBB [2-(alpha-hydroxybenzyl)-benzimidazole], and MRL-1237 {1-(4-fluorophenyl)-2-[(4-imino-1,4-dihydropyridin-1-yl)methyl]benzimidazole hydrochloride}. The ATPase activity of 2C, however, remained unaltered in the presence of TBZE-029.

Published
2008

47. Molecular determinants of the interaction between coxsackievirus protein 3A and guanine nucleotide exchange factor GBF1.

Author

Wessels, E., Duijsings, D., Lanke, K.H.W., Melchers, W.J.G., Jackson, C.L., Kuppeveld, F.J.M. van, Wessels, E., Duijsings, D., Lanke, K.H.W., Melchers, W.J.G., Jackson, C.L., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 52098.pdf (publisher's version ) (Open Access), The 3A protein of coxsackievirus B3 (CVB3), a small membrane protein that forms homodimers, inhibits endoplasmic reticulum-to-Golgi complex transport. Recently, we described the underlying mechanism by showing that the CVB3 3A protein binds to and inhibits the function of GBF1, a guanine nucleotide exchange factor for ADP-ribosylation factor 1 (Arf1), thereby interfering with Arf1-mediated COP-I recruitment. This study was undertaken to gain more insight into the molecular determinants underlying the interaction between 3A and GBF1. Here we show that 3A mutants that have lost the ability to dimerize are no longer able to bind to GBF1 and trap it on membranes. Moreover, we identify a conserved region in the N terminus of 3A that is crucial for GBF1 binding but not for 3A dimerization. Analysis of the binding domain in GBF1 showed that the extreme N terminus, the dimerization/cyclophilin binding domain, and the homology upstream of Sec7 domain are required for the interaction with 3A. In contrast to that of full-length GBF1, overexpression of a GBF1 mutant lacking its extreme N terminus failed to rescue the effects of 3A. Together, these data provide insight into the molecular requirements of the interaction between 3A and GBF1.

Published
2007

48. PDTC inhibits picornavirus polyprotein processing and RNA replication by transporting zinc ions into cells.

Author

Lanke, K.H.W., Krenn, B.M., Melchers, W.J.G., Seipelt, J., Kuppeveld, F.J.M. van, Lanke, K.H.W., Krenn, B.M., Melchers, W.J.G., Seipelt, J., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 52333.pdf (publisher's version ) (Closed access), Previously, it was shown that pyrrolidine dithiocarbamate (PDTC) inhibits proteolytic polyprotein processing and replication of human rhinovirus by transporting metal ions into cells. Here, it is shown that PDTC also inhibits replication of two other picornaviruses: coxsackievirus B3 (CVB3), a closely related virus that belongs to the genus Enterovirus, and mengovirus, an encephalomyocarditis virus strain that belongs to the genus Cardiovirus, and that this inhibition is due to the dithiocarbamate moiety of the compound. Making use of subgenomic replicons, evidence is provided that PDTC inhibits replication of these two viruses by disturbing viral RNA synthesis. Furthermore, it is shown that PDTC transports zinc ions into cells and that these zinc ions play an important role in the antiviral activity mediated by PDTC. Finally, it is shown that PDTC interferes with proteolytic processing of the polyproteins of both CVB3 and mengovirus, but that the underlying mechanism between these two viruses differs. In CVB3-infected cells, PDTC interferes strongly with the proteolytic activity of 3CD(pro), as shown by the impaired production of the mature capsid proteins as well as the autocleavage of 3CD(pro) into 3C(pro) and 3D(pol). In mengovirus-infected cells, however, PDTC had no effect on the proteolytic production of capsid proteins or the autocleavage of 3CD(pro). Instead, PDTC caused the accumulation of a high-molecular-mass precursor protein, due to an impairment in the primary 'break' that normally occurs at the 2A-2B junction. Thus, PDTC disturbs polyprotein processing and replication of two groups of picornaviruses, enteroviruses and cardioviruses, but the underlying mechanism is different.

Published
2007

49. Effects of picornavirus 3A Proteins on Protein Transport and GBF1-dependent COP-I recruitment.

Author

Wessels, E., Duijsings, D.M., Lanke, K.H.W., Dooren, S.H.J. van, Jackson, C.L., Melchers, W.J.G., Kuppeveld, F.J.M. van, Wessels, E., Duijsings, D.M., Lanke, K.H.W., Dooren, S.H.J. van, Jackson, C.L., Melchers, W.J.G., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 35907.pdf (publisher's version ) (Open Access), The 3A protein of the coxsackievirus B3 (CVB3), an enterovirus that belongs to the family of the picornaviruses, inhibits endoplasmic reticulum-to-Golgi transport. Recently, we elucidated the underlying mechanism by showing that CVB3 3A interferes with ADP-ribosylation factor 1 (Arf1)-dependent COP-I recruitment to membranes by binding and inhibiting the function of GBF1, a guanine nucleotide exchange factor that is required for the activation of Arf1 (E. Wessels et al., Dev. Cell 11:191-201, 2006). Here, we show that the 3A protein of poliovirus, another enterovirus, is also able to interfere with COP-I recruitment through the same mechanism. No interference with protein transport or COP-I recruitment was observed for the 3A proteins of any of the other picornaviruses tested here (human rhinovirus [HRV], encephalomyocarditis virus, foot-and-mouth disease virus, and hepatitis A virus). We show that the 3A proteins of HRV, which are the most closely related to the enteroviruses, are unable to inhibit COP-I recruitment, due to a reduced ability to bind GBF1. When the N-terminal residues of the HRV 3A proteins are replaced by those of CVB3 3A, chimeric proteins are produced that have gained the ability to bind GBF1 and, by consequence, to inhibit protein transport. These results show that the N terminus of the CVB3 3A protein is important for binding of GBF1 and its transport-inhibiting function. Taken together, our data demonstrate that the activity of the enterovirus 3A protein to inhibit GBF1-dependent COP-I recruitment is unique among the picornaviruses.

Published
2006

50. A viral protein that blocks Arf1-mediated COP-I assembly by inhibiting the guanine nucleotide exchange factor GBF1.

Author

Wessels, E., Duijsings, D.M., Niu, T.K., Neumann, S., Oorschot, V.M., Lange, F. de, Lanke, K.H.W., Klumperman, J., Henke, A., Jackson, C.L., Melchers, W.J.G., Kuppeveld, F.J.M. van, Wessels, E., Duijsings, D.M., Niu, T.K., Neumann, S., Oorschot, V.M., Lange, F. de, Lanke, K.H.W., Klumperman, J., Henke, A., Jackson, C.L., Melchers, W.J.G., and Kuppeveld, F.J.M. van

Abstract

Contains fulltext : 49596.pdf (publisher's version ) (Closed access), Many viruses modify cellular processes for their own benefit. The enterovirus 3A protein inhibits endoplasmic reticulum (ER)-to-Golgi transport, a function previously suggested to be important for viral suppression of immune responses. Here, we show that a virus carrying a 3A protein defective in inhibiting ER-to-Golgi transport is indeed less virulent in mice, and we unravel the mechanism by which 3A inhibits this trafficking step. Evidence is provided that 3A inhibits the activation of the GTPase ADP-ribosylation factor 1 (Arf1), which regulates the recruitment of the COP-I coat complex to membranes. 3A specifically inhibits the function of GBF1, a guanine nucleotide exchange factor for Arf1, by interacting with its N terminus. By specifically interfering with GBF1-mediated Arf1 activation, 3A may prove a valuable tool in dissecting the early steps of the secretory pathway.

Published
2006

Catalog

Books, media, physical & digital resources
See catalog results