Your search keyword '"de Dood, Claudia J."' showing total 48 results

1. Detecting two Schistosoma circulating antigens - CCA and CAA - in urine and serum to improve diagnosis of human schistosomiasis.

Author

Hoekstra, Pytsje T., de Dood, Claudia J., Abdoel, Theresia, Hilt, Stan, van Diepen, Angela, Polman, Katja, Kremsner, Peter, van Lieshout, Lisette, Kreidenweiss, Andrea, Adegnika, Ayola Akim, Fusco, Daniela, Rasomoelina, Tahinamandranto, Andrianarivelo, Mala Rakoto, Rakotozandrindrainy, Raphaël, Rakotoarivelo, Rivo Andry, Sicuri, Elisa, van Dam, Govert J., and Corstjens, Paul L. A. M.

Subjects

*SCHISTOSOMA, *SCHISTOSOMIASIS, *ANTIGENS, *SCHISTOSOMATIDAE, *SERUM

Abstract

Background: Schistosomiasis is caused by infection with parasitic Schistosoma worms and affects more than 250 million people globally. The detection of schistosome derived circulating cathodic and anodic antigens (CCA and CAA) has proven highly valuable for detecting active Schistosoma infections, causing both intestinal and urinary schistosomiasis. Aim: The combined detection of CCA and CAA was explored to improve accuracy in detecting Schistosoma infections. Methods: Parallel detection of CCA and CAA was performed on two banked sample sets with matching serum and urine samples from Schistosoma mansoni (Sm) and S. haematobium (Sh) infected individuals using the non-concentration based lateral flow (LF) test comprising the sensitive luminescent up-converting reporter particle (UCP) technology. Results: Parallel detection of CCA and CAA increased the positivity rate for detecting both Sm and Sh infections compared to the detection of either antigen separately, demonstrating the added value of detecting both antigens in a single sample to confirm diagnosis, independent from the Schistosoma species. Significantly higher CCA concentrations in urine were observed in Sm infected individuals compared to Sh infected individuals, while serum CCAconcentrations were similar between species. CAA concentrations were higher in serum compared to those in urine, irrespective of species. When exploring the relationship of CCA and CAA in urine, the CCA/CAA ratio in Sm infected individuals was significantly higher than in Sh infected individuals, while no differences were observed in serum. Discussion and conclusion: Parallel detection of CCA and CAA via the UCP-LF platform showed added diagnostic value through an increased positivity rate for the detection of Sm and Sh infections, compared to only detecting either of the antigens. The combined and quantitative detection of CCA and CAA is indicative for identifying the infecting species, but needs further exploration. [ABSTRACT FROM AUTHOR]

Published

2024

2. Cervicovaginal bacterial communities in reproductive-aged Tanzanian women with Schistosoma mansoni, Schistosoma haematobium, or without schistosome infection

Author

Bullington, Brooke W., Lee, Myung Hee, Mlingi, Jane, Paul, Ndalloh, Aristide, Christine, Fontana, Emily, Littmann, Eric R., Mukerebe, Crispin, Shigella, Peter, Kashangaki, Philibert, Kalluvya, Samuel E., de Dood, Claudia J., van Dam, Govert J., Corstjens, Paul L.A.M., Fitzgerald, Daniel W., Pamer, Eric G., and Downs, Jennifer A.

Published

2021

3. Rhesus macaques self-curing from a schistosome infection can display complete immunity to challenge

Author

Amaral, Murilo Sena, Santos, Daisy Woellner, Pereira, Adriana S. A., Tahira, Ana Carolina, Malvezzi, João V. M., Miyasato, Patrícia Aoki, Freitas, Rafaela de Paula, Kalil, Jorge, Tjon Kon Fat, Elisa M., de Dood, Claudia J., Corstjens, Paul L. A. M., van Dam, Govert J., Nakano, Eliana, Castro, Simone de Oliveira, Mattaraia, Vânia Gomes de Moura, Augusto, Ronaldo de Carvalho, Grunau, Christoph, Wilson, R. Alan, and Verjovski-Almeida, Sergio

Published

2021

4. A controlled human Schistosoma mansoni infection model to advance novel drugs, vaccines and diagnostics

Author

Langenberg, Marijke C. C., Hoogerwerf, Marie-Astrid, Koopman, Jan Pieter R., Janse, Jacqueline J., Kos-van Oosterhoud, Janneke, Feijt, Carola, Jochems, Simon P., de Dood, Claudia J., van Schuijlenburg, Roos, Ozir-Fazalalikhan, Arifa, Manurung, Mikhael D., Sartono, Erliyani, van der Beek, Martha T., Winkel, Béatrice M. F., Verbeek-Menken, Petra H., Stam, Koen A., van Leeuwen, Fijs W. B., Meij, Pauline, van Diepen, Angela, van Lieshout, Lisette, van Dam, Govert J., Corstjens, Paul L. A. M., Hokke, Cornelis H., Yazdanbakhsh, Maria, Visser, Leo G., and Roestenberg, Meta

Published

2020

5. Schistosoma mansoni infection alters the host pre-vaccination environment resulting in blunted Hepatitis B vaccination immune responses

Author

Muir, Roshell, primary, Metcalf, Talibah, additional, Fourati, Slim, additional, Bartsch, Yannic, additional, Kyosiimire-Lugemwa, Jacqueline, additional, Canderan, Glenda, additional, Alter, Galit, additional, Muyanja, Enoch, additional, Okech, Brenda, additional, Namatovu, Teddy, additional, Namara, Irene, additional, Namuniina, Annemarie, additional, Ssetaala, Ali, additional, Mpendo, Juliet, additional, Nanvubya, Annet, additional, Kitandwe, Paul Kato, additional, Bagaya, Bernard S., additional, Kiwanuka, Noah, additional, Nassuna, Jacent, additional, Biribawa, Victoria Menya, additional, Elliott, Alison M., additional, de Dood, Claudia J., additional, Senyonga, William, additional, Balungi, Priscilla, additional, Kaleebu, Pontiano, additional, Mayanja, Yunia, additional, Odongo, Matthew, additional, Connors, Jennifer, additional, Fast, Pat, additional, Price, Matt A., additional, Corstjens, Paul L. A. M., additional, van Dam, Govert J., additional, Kamali, Anatoli, additional, Sekaly, Rafick Pierre, additional, and Haddad, Elias K., additional

Published

2023

6. Sensitivity and specificity of human point-of-care circulating cathodic antigen (POC-CCA) test in African livestock for rapid diagnosis of schistosomiasis: A Bayesian latent class analysis

Author

Calvo-Urbano, Beatriz, primary, Léger, Elsa, additional, Gabain, Isobel, additional, De Dood, Claudia J., additional, Diouf, Nicolas D., additional, Borlase, Anna, additional, Rudge, James W., additional, Corstjens, Paul L. A. M., additional, Sène, Mariama, additional, Van Dam, Govert J., additional, Walker, Martin, additional, and Webster, Joanne P., additional

Published

2023

7. Association of schistosome infection with adiposity in Tanzania

Author

Pham, Khanh, PrayGod, George, Faurholt-Jepsen, Daniel, Olsen, Mette Frahm, Kavishe, Bazil, Kitilya, Brenda, Corstjens, Paul L A M, de Dood, Claudia J, Friis, Henrik, Filteau, Suzanne, Downs, Jennifer A, Peck, Robert N, Pham, Khanh, PrayGod, George, Faurholt-Jepsen, Daniel, Olsen, Mette Frahm, Kavishe, Bazil, Kitilya, Brenda, Corstjens, Paul L A M, de Dood, Claudia J, Friis, Henrik, Filteau, Suzanne, Downs, Jennifer A, and Peck, Robert N

Abstract

Background: Observational studies in humans have reported a link between schistosome infection and lower adiposity, but this may be explained by socioeconomic and demographic factors, intensity of infection, or common co-infections such as HIV.Methods: This was a cross-sectional study that investigated the relationship between schistosome infection and adiposity in a large, well-described cohort of Tanzanian adults living with and without HIV. Cross-sectional data were collected among adults living in Mwanza, Tanzania who were enrolled in the Chronic Infections, Co-morbidities and Diabetes in Africa (CICADA) cohort study. Schistosome circulating anodic antigen, secreted by both Schistosoma mansoni and haematobium which are endemic to Tanzania, was quantified from stored samples. Schistosome infection diagnosed by serum circulating anodic antigen levels. The primary outcome was fat mass measured by bioimpedance analysis. Secondary outcomes included fat-free mass, waist circumference, mid-upper arm circumference, and body mass index.Results: The study enrolled 1,947 adults, of whom 1,923 (98.8%) had serum available for schistosome testing. Of these, 873 (45.4%) had a serum circulating anodic antigen ≥30 pg/mL, indicating schistosome infection. Compared to uninfected individuals, those with schistosome infections had -1.1 kg [95% CI -1.9 to -0.3] lower fat mass after adjusting for age, sex, physical activity, tobacco use, education level, and socioeconomic status. Infected participants also had lower waist circumference, mid-upper arm circumference, and body mass index. Fat-free mass was not different between the two groups. Neither being HIV-infected, nor receiving antiretroviral therapy, modified associations between schistosome infection and adiposity. These associations were also not affected by Schistosoma worm burden.Conclusions: Schistosome infection was associated with lower fat mass and less cen

Published

2023

8. HIV-seroconversion among HIV-1 serodiscordant married couples in Tanzania: a cohort study

Author

Colombe, Soledad, Beard, James, Mtenga, Baltazar, Lutonja, Peter, Mngara, Julius, de Dood, Claudia J., van Dam, Govert J., Corstjens, Paul L. A. M., Kalluvya, Samuel, Urassa, Mark, Todd, Jim, and Downs, Jennifer A.

Published

2019

9. Schistosomiasis and HIV-1 viral load in HIV-infected outpatients with immunological failure in Tanzania: a case-control study

Author

Masikini, Peter, Colombe, Soledad, Marti, Amon, Desderius, Bernard, de Dood, Claudia J., Corstjens, Paul L. A. M., van Dam, Govert J., Seugendo, Mwanaisha, Kalluvya, Samuel, and Downs, Jennifer A.

Published

2019

10. Association of schistosome infection with adiposity in Tanzania

Author

Pham, Khanh, primary, PrayGod, George, additional, Faurholt-Jepsen, Daniel, additional, Olsen, Mette F., additional, Kavishe, Bazil, additional, Kitilya, Brenda, additional, Corstjens, Paul L. A. M., additional, de Dood, Claudia J., additional, Friis, Henrik, additional, Filteau, Suzanne, additional, Downs, Jennifer A., additional, and Peck, Robert N., additional

Published

2023

11. Latent class analysis to evaluate performance of point-of-care CCA for low-intensity Schistosoma mansoni infections in Burundi

Author

Clements, Michelle N., Corstjens, Paul L. A. M., Binder, Sue, Campbell, Jr, Carl H., de Dood, Claudia J., Fenwick, Alan, Harrison, Wendy, Kayugi, Donatien, King, Charles H., Kornelis, Dieuwke, Ndayishimiye, Onesime, Ortu, Giuseppina, Lamine, Mariama Sani, Zivieri, Antonio, Colley, Daniel G., and van Dam, Govert J.

Published

2018

12. Sensitive Diagnosis and Post-Treatment Follow-Up of Schistosoma mansoni Infections in Asymptomatic Eritrean Refugees by Circulating Anodic Antigen Detection and Polymerase Chain Reaction

Author

Hoekstra, Pytsje T., primary, Chernet, Afona, additional, de Dood, Claudia J., additional, Brienen, Eric A. T., additional, Corstjens, Paul L. A. M., additional, Labhardt, Niklaus D., additional, Nickel, Beatrice, additional, Wammes, Linda J., additional, van Dam, Govert J., additional, Neumayr, Andreas, additional, and van Lieshout, Lisette, additional

Published

2022

13. Excretion patterns of Schistosoma mansoni antigens CCA and CAA by adult male and female worms, using a mouse model and ex vivo parasite cultures

Author

Casacuberta-Partal, Miriam, primary, van Lieshout, Lisette, additional, van Diepen, Angela, additional, Sijtsma, Jeroen, additional, Ozir-Fazalalikhan, Arifa, additional, Koopman, Jan Pieter R., additional, de Dood, Claudia J., additional, Corstjens, Paul L.A.M., additional, van Dam, Govert J., additional, Hokke, Cornelis H., additional, and Roestenberg, Meta, additional

Published

2021

14. A rapid assay for on-site monitoring of infliximab trough levels: a feasibility study

Author

Corstjens, Paul L. A. M., Fidder, Herma H., Wiesmeijer, Karien C., de Dood, Claudia J., Rispens, Theo, Wolbink, Gert-Jan, Hommes, Daniel W., and Tanke, Hans J.

Published

2013

15. Sensitive diagnosis and post-treatment follow-up of Schistosoma mansoni infections in asymptomatic Eritrean refugees by Circulating Anodic Antigen (CAA) detection and PCR

Author

Hoekstra, Pytsje T., Chernet, Afona, de Dood, Claudia J., Brienen, Eric A. T., Corstjens, Paul L. A. M., Labhardt, Niklaus D., Nickel, Beatrice, Wammes, Linda, van Dam, Govert J., Neumayr, Andreas, and van Lieshout, Lisette

Abstract

The increasing number of refugees coming from or passing through Schistosoma-endemic areas and arriving in Europe highlights the importance of screening for schistosomiasis on arrival, and focuses attention on the choice of diagnostic test. We evaluate the diagnostic performance of circulating anodic antigen (CAA) detection in 92 asymptomatic refugees from Eritrea. Results were compared with already-available stool microscopy, serology, and urine point-of-care circulating cathodic antigen (POC-CCA) data. For a full diagnostic comparison, real-time polymerase chain reaction (PCR) and the POC-CCA were included. All outcomes were compared against a composite reference standard. Urine and serum samples were subjected to the ultra-sensitive and highly specific up-converting particle lateral flow CAA test, Schistosoma spp. real-time PCR was performed on urine and stool, and the POC-CCA was used on urine using the G-score method. CAA was detected in 43% of urine and in 40% of serum samples. Urine PCR was negative in all 92 individuals, whereas 25% showed Schistosoma DNA in stool. POC-CCA was positive in 30% of individuals. The CAA test confirmed all microscopy positives, except for two cases that were also negative by all other diagnostic procedures. Post-treatment, a significant reduction in the number of positives and infection intensity was observed, in particular regarding CAA levels. Our findings confirm that microscopy, serology, and POC-CCA lack the sensitivity to detect all active Schistosoma infections. Accuracy of stool PCR was similar to microscopy, indicating that this method also lacks sensitivity. The CAA test appeared to be the most accurate method for screening active Schistosoma infections and for monitoring treatment efficacy.

Published

2021

16. High prevalence of Schistosoma mansoni infection and stunting among school age children in communities along the Albert-Nile, Northern Uganda: A cross sectional study.

Author

Mulindwa, Julius, Namulondo, Joyce, Kitibwa, Anna, Nassuuna, Jacent, Nyangiri, Oscar Asanya, Kimuda, Magambo Phillip, Boobo, Alex, Nerima, Barbara, Busingye, Fred, Candia, Rowel, Namukuta, Annet, Ssenyonga, Ronald, Ukumu, Noah, Ajal, Paul, Adriko, Moses, Noyes, Harry, de Dood, Claudia J., Corstjens, Paul L. A. M., van Dam, Govert J., and Elliott, Alison M.

Subjects

STUNTED growth, SCHOOL children, SCHISTOSOMA mansoni, SHORELINES, CHILD nutrition, FRESH water, GIRLS

Abstract

Background: Knowing the prevalence of schistosomiasis is key to informing programmes to control and eliminate the disease as a public health problem. It is also important to understand the impact of infection on child growth and development in order to allocate appropriate resources and effort to the control of the disease. Methods: We conducted a survey to estimate the prevalence of schistosomiasis among school aged children in villages along the Albert-Nile shore line in the district of Pakwach, North Western Uganda. A total of 914 children aged between 10–15 years were screened for Schistosoma mansoni using the POC-CCA and Kato Katz (KK) techniques. The infection intensities were assessed by POC-CCA and KK as well as CAA tests. The KK intensities were also correlated with POC-CCA and with CAA intensity. Anthropometric measurements were also taken and multivariate analysis was carried out to investigate their association with infection status. Results: The prevalence of schistosomiasis using the POC-CCA diagnostic test was estimated at 85% (95% CI: 83–87), being highest amongst children living closer to the Albert-Nile shoreline. Visual scoring of the POC-CCA results was more sensitive than the Kato Katz test and was positively correlated with the quantified infection intensities by the CAA test. The majority of the children were underweight (BMI<18.5), and most notably, boys had significantly lower height for age (stunting) than girls in the same age range (p < 0.0001), but this was not directly associated with S. mansoni infection. Conclusion: High prevalence of S. mansoni infection in the region calls for more frequent mass drug administration with praziquantel. We observed high levels of stunting which was not associated with schistosomiasis. There is a need for improved nutrition among the children in the area. Author summary: Schistosomiasis is a neglected but frequent disease that is caused by schistosomes, with over 290 million people worldwide at risk of infection. The major mode of transmission is through contact with fresh water sources infested with infected snails (the intermediate host). In this study, using the point of care test (POC-CCA), we screened 914 school aged children (10–15 years) living in the rural communities along the Lake Albert- River Nile shores of Pakwach district in Northern Uganda. We observed a very high prevalence of S. mansoni infections (over 80%) although the prevalence dropped to 40% in communities that were further from the lake shores. This high prevalence was also coupled with Kato Katz light schistosome infection intensities as categorised by WHO guidelines. We further compared the POC-CCA and Kato Katz tests to the more sensitive CAA assay and this revealed that even though both tests gave good probability of positive prediction, the POC-CCA had higher sensitivity in screening for S. mansoni infections than Kato Katz assay. The study also revealed high levels of stunting within the children, more so amongst boys. Frequent screening and mass treatment of these communities with praziquantel will reduce on the infection rates. But in addition, improved hygiene and sanitation will be required for a sustainable reduction in the prevalence and morbidity of schistosomiasis in the Albert-Nile communities along with dietary intervention for optimal child health. [ABSTRACT FROM AUTHOR]

Published

2022

17. Specificity of the Point-of-Care Urine Strip Test for Schistosoma Circulating Cathodic Antigen (POC-CCA) Tested in Non-Endemic Pregnant Women and Young Children

Author

Casacuberta-Partal, Miriam, primary, Beenakker, Margreet, additional, de Dood, Claudia J., additional, Hoekstra, Pytsje T., additional, Kroon, Lisa, additional, Kornelis, Dieuwke, additional, Corstjens, Paul, additional, Hokke, Cornelis H., additional, van Dam, Govert J., additional, Roestenberg, Meta, additional, and van Lieshout, Lisette, additional

Published

2021

18. Circulating Anodic Antigen (CAA): A Highly Sensitive Diagnostic Biomarker to Detect Active Schistosoma Infections—Improvement and Use during SCORE

Author

Corstjens, Paul L. A. M., primary, de Dood, Claudia J., additional, Knopp, Stefanie, additional, Clements, Michelle N., additional, Ortu, Giuseppina, additional, Umulisa, Irenee, additional, Ruberanziza, Eugene, additional, Wittmann, Udo, additional, Kariuki, Thomas, additional, LoVerde, Philip, additional, Secor, William Evan, additional, Atkins, Lydia, additional, Kinung’hi, Safari, additional, Binder, Sue, additional, Campbell, Carl H., additional, Colley, Daniel G., additional, and van Dam, Govert J., additional

Published

2020

19. Excretion patterns of Schistosoma mansoni antigens CCA and CAA by adult male and female worms, using a mouse model and ex vivo parasite cultures.

Author

Casacuberta-Partal, Miriam, van Lieshout, Lisette, van Diepen, Angela, Sijtsma, Jeroen C., Ozir-Fazalalikhan, Arifa, Koopman, Jan Pieter R., de Dood, Claudia J., Corstjens, Paul L.A.M., van Dam, Govert J., Hokke, Cornelis H., and Roestenberg, Meta

Subjects

SCHISTOSOMA mansoni, LABORATORY mice, EXCRETION, ANIMAL disease models, WORMS

Abstract

Assays which enable the detection of schistosome gut-associated circulating anodic (CAA) and cathodic (CCA) antigen in serum or urine are increasingly used as a diagnostic tool for schistosome infection. However, little is known about the production and clearance of these circulating antigens in relation to the sex and reproductive maturity of the parasite. Here we describe CAA and CCA excretion patterns by exploring a mouse model after exposure to 36 male-only, female-only and mixed (male/female) Schistosoma mansoni cercariae. We found that serum and urine CAA levels, analysed at 3 weeks intervals, peaked at 6 weeks post-infection. Worms recovered after perfusion at 14 weeks were cultured ex vivo. Male parasites excreted more circulating antigens than females, in the mouse model as well as ex vivo. In mixed infections (supporting egg production), serum CAA levels correlated to the number of recovered worms, whereas faecal egg counts or Schistosoma DNA in stool did not. No viable eggs and no inflammation were seen in the livers from mice infected with female worms only. Ex vivo, CAA levels were higher than CCA levels. Our study confirms that CAA levels reflect worm burden and allows detection of low-level single-sex infections. [ABSTRACT FROM AUTHOR]

Published

2022

20. Refining Diagnosis of Schistosoma haematobium Infections: Antigen and Antibody Detection in Urine

Author

de Dood, Claudia J., Hoekstra, Pytsje T., Mngara, Julius, Kalluvya, Samuel E., van Dam, Govert J., Downs, Jennifer A., and Corstjens, Paul L. A. M.

Subjects

Immunology, Immunology and Allergy

Published

2018

21. Insufficiency of annual praziquantel treatment to control Schistosoma mansoni infections in adult women: A longitudinal cohort study in rural Tanzania

Author

Mishra, Pallavi, primary, Colombe, Soledad, additional, Paul, Ndalloh, additional, Mlingi, Jane, additional, Tosiri, Inobena, additional, Aristide, Christine, additional, Gao, Joanna, additional, Kashangaki, Philibert, additional, Nagai, Honest, additional, Kalluvya, Samuel E., additional, de Dood, Claudia J., additional, Corstjens, Paul L., additional, Mngara, Julius, additional, van Dam, Govert J., additional, and Downs, Jennifer A., additional

Published

2019

22. Performance of an Ultra-Sensitive Assay Targeting the Circulating Anodic Antigen (CAA) for Detection of Schistosoma mansoni Infection in a Low Endemic Area in Brazil

Author

Sousa, Mariana Silva, primary, van Dam, Govert J., additional, Pinheiro, Marta Cristhiany Cunha, additional, de Dood, Claudia J., additional, Peralta, Jose Mauro, additional, Peralta, Regina Helena Saramago, additional, Daher, Elizabeth de Francesco, additional, Corstjens, Paul L. A. M., additional, and Bezerra, Fernando Schemelzer Moraes, additional

Published

2019

23. Gene Expression Differences in Host Response to Schistosoma haematobium Infection

Author

Dupnik, Kathryn M., primary, Reust, Mary Juliet, additional, Vick, Kaitlin M., additional, Yao, Benjamin, additional, Miyaye, Donald, additional, Lyimo, Eric, additional, Mukerebe, Crispin, additional, Mngara, Julius, additional, Kalluvya, Samuel E., additional, de Dood, Claudia J., additional, Corstjens, Paul L. A. M., additional, van Dam, Govert J., additional, Zhang, Tuo, additional, Xiang, Jenny, additional, Lee, Myung Hee, additional, and Downs, Jennifer A., additional

Published

2019

24. Effect of schistosomiasis on the outcome of patients infected with HIV-1 starting antiretroviral therapy in rural Tanzania

Author

Stete, Katarina, primary, Glass, Tracy R., additional, van Dam, Govert J., additional, Ntamatungiro, Alex, additional, Letang, Emilio, additional, de Dood, Claudia J., additional, Corstjens, Paul L. A. M., additional, Ndege, Robert, additional, Mapesi, Herry, additional, Kern, Winfried V., additional, Hatz, Christoph, additional, Weisser, Maja, additional, Utzinger, Jürg, additional, and Müller, Matthias C., additional

Published

2018

25. HIV-1 Viral Loads Are Not Elevated in Individuals Co-infected With Schistosoma spp. After Adjustment for Duration of HIV-1 Infection

Author

Colombe, Soledad, primary, Corstjens, Paul L. A. M., additional, de Dood, Claudia J., additional, Miyaye, Donald, additional, Magawa, Ruth G., additional, Mngara, Julius, additional, Kalluvya, Samuel E., additional, van Lieshout, Lisette, additional, van Dam, Govert J., additional, and Downs, Jennifer A., additional

Published

2018

26. Impact of schistosome infection on long-term HIV/AIDS outcomes

Author

Colombe, Soledad, primary, Machemba, Richard, additional, Mtenga, Baltazar, additional, Lutonja, Peter, additional, Kalluvya, Samuel E., additional, de Dood, Claudia J., additional, Hoekstra, Pytsje T., additional, van Dam, Govert J., additional, Corstjens, Paul L. A. M., additional, Urassa, Mark, additional, Changalucha, John M., additional, Todd, Jim, additional, and Downs, Jennifer A., additional

Published

2018

27. Decreased Sensitivity of Schistosoma sp. Egg Microscopy in Women and HIV-Infected Individuals

Author

Colombe, Soledad, primary, Mngara, Julius, additional, de Dood, Claudia J., additional, Hoekstra, Pytsje T., additional, Masikini, Peter J., additional, Corstjens, Paul L. A. M., additional, van Lieshout, Lisette, additional, Lee, Myung Hee, additional, Downs, Jennifer A., additional, and van Dam, Govert J., additional

Published

2018

28. Rapid clearance of Schistosoma mansoni circulating cathodic antigen after treatment shown by urine strip tests in a Ugandan fishing community :Relevance for monitoring treatment efficacy and re-infection

Author

Kildemoes, Anna O., Vennervald, Birgitte J., Tukahebwa, Edridah M., Kabatereine, Narcis B., Magnussen, Pascal, De Dood, Claudia J., Deelder, André M., Wilson, Shona, Van Dam, Govert J., Kildemoes, Anna O., Vennervald, Birgitte J., Tukahebwa, Edridah M., Kabatereine, Narcis B., Magnussen, Pascal, De Dood, Claudia J., Deelder, André M., Wilson, Shona, and Van Dam, Govert J.

Abstract

Schistosomiasis control and elimination has priority in public health agendas in several sub-Saharan countries. However, achieving these goals remains a substantial challenge. In order to assess progress of interventions and treatment efficacy it is pertinent to have accurate, feasible and affordable diagnostic tools. Detection of Schistosoma mansoni infection by circulating cathodic antigen (CCA) in urine is an attractive option as this measure describes live worm infection noninvasively. In order to interpret treatment efficacy and re-infection levels, knowledge about clearance of this antigen is necessary. The current study aims to investigate, whether antigen clearance as a proxy for decreasing worm numbers is reflected in decreasing CCA levels in urine shortly after praziquantel treatment. Here CCA levels are measured 24 hours post treatment in response to both a single and two treatments. The study was designed as a series of cross-sectional urine and stool sample collections from 446 individuals nested in a two-arm randomised single blinded longitudinal clinical trial cohort matched by gender and age (ClinicalTrials.gov Identifier: NCT00215267) receiving one or two praziquantel treatments. CCA levels in urine were determined by carbon-conjugated monoclonal antibody lateral flow strip assay and eggs per gram faeces for S. mansoni and soil-transmitted helminths by Kato-Katz. Significant correlations between CCA levels and S. mansoni egg count at every measured time point were found and confirmed the added beneficial effect of a second treatment at two weeks after baseline. Furthermore, presence of hookworm was found not to be a confounder for CCA test specificity. Twenty-four hours post treatment measures of mean CCA scores showed significant reductions. In conclusion, removal of CCA in response to treatment is detectable as a decline in CCA in urine already after 24 hours. This has relevance for use and interpretation of laboratory based and point-of-care CCA

Published

2017

29. Rapid clearance of Schistosoma mansoni circulating cathodic antigen after treatment shown by urine strip tests in a Ugandan fishing community – Relevance for monitoring treatment efficacy and re-infection

Author

Kildemoes, Anna O., primary, Vennervald, Birgitte J., additional, Tukahebwa, Edridah M., additional, Kabatereine, Narcis B., additional, Magnussen, Pascal, additional, de Dood, Claudia J., additional, Deelder, André M., additional, Wilson, Shona, additional, and van Dam, Govert J., additional

Published

2017

30. Utilizing the ultrasensitive Schistosoma up-converting phosphor lateral flow circulating anodic antigen (UCP-LF CAA) assay for sample pooling-strategies

Author

Corstjens, Paul L. A. M., primary, Hoekstra, Pytsje T., additional, de Dood, Claudia J., additional, and van Dam, Govert J., additional

Published

2017

31. Effects of schistosomiasis on susceptibility to HIV-1 infection and HIV-1 viral load at HIV-1 seroconversion: A nested case-control study

Author

Downs, Jennifer A., primary, Dupnik, Kathryn M., additional, van Dam, Govert J., additional, Urassa, Mark, additional, Lutonja, Peter, additional, Kornelis, Dieuwke, additional, de Dood, Claudia J., additional, Hoekstra, Pytsje, additional, Kanjala, Chifundo, additional, Isingo, Raphael, additional, Peck, Robert N., additional, Lee, Myung Hee, additional, Corstjens, Paul L. A. M., additional, Todd, Jim, additional, Changalucha, John M., additional, Johnson, Warren D., additional, and Fitzgerald, Daniel W., additional

Published

2017

32. Selecting accurate post-elimination monitoring tools to prevent reemergence of urogenital schistosomiasis in Morocco: a pilot study

Author

Balahbib, Abdelaali, primary, Amarir, Fatima, additional, Corstjens, Paul L.A.M., additional, de Dood, Claudia J., additional, van Dam, Govert J., additional, Hajli, Amina, additional, Belhaddad, Meryem, additional, El Mansouri, Bouchra, additional, Sadak, Abderrahim, additional, Rhajaoui, Mohamed, additional, and Adlaoui, El Bachir, additional

Published

2017

33. Schistosomiasis and Human Immunodeficiency Virus in Men in Tanzania

Author

Downs, Jennifer A., primary, de Dood, Claudia J., additional, Dee, Hannah E., additional, McGeehan, Megan, additional, Khan, Hijab, additional, Marenga, Abena, additional, Adel, Patrick E., additional, Faustine, Edward, additional, Issarow, Benson, additional, Kisanga, Emmanuel F., additional, Kisigo, Godfrey Alfred, additional, Ngahyolerwa, Salvius, additional, Zahoro, Frank, additional, Miyaye, Donald, additional, Magawa, Ruth Gideon, additional, Mngara, Julius, additional, Lee, Myung Hee, additional, Corstjens, Paul L. A. M., additional, van Dam, Govert J., additional, and Fitzgerald, Daniel W., additional

Published

2017

34. A controlled human Schistosoma mansoniinfection model to advance novel drugs, vaccines and diagnostics

Author

Langenberg, Marijke C. C., Hoogerwerf, Marie-Astrid, Koopman, Jan Pieter R., Janse, Jacqueline J., Kos-van Oosterhoud, Janneke, Feijt, Carola, Jochems, Simon P., de Dood, Claudia J., van Schuijlenburg, Roos, Ozir-Fazalalikhan, Arifa, Manurung, Mikhael D., Sartono, Erliyani, van der Beek, Martha T., Winkel, Béatrice M. F., Verbeek-Menken, Petra H., Stam, Koen A., van Leeuwen, Fijs W. B., Meij, Pauline, van Diepen, Angela, van Lieshout, Lisette, van Dam, Govert J., Corstjens, Paul L. A. M., Hokke, Cornelis H., Yazdanbakhsh, Maria, Visser, Leo G., and Roestenberg, Meta

Abstract

Schistosomiasis treatment relies on the use of a single drug, praziquantel, which is insufficient to control transmission in highly endemic areas1. Novel medicines and vaccines are urgently needed2,3. An experimental human model for schistosomiasis could accelerate the development of these products. We performed a dose-escalating clinical safety trial in 17 volunteers with male Schistosoma mansonicercariae, which do not produce eggs (clinicaltrials.gov NCT02755324), at the Leiden University Medical Center, the Netherlands. The primary endpoints were adverse events and infectivity. We found a dose-related increase in adverse events related to acute schistosomiasis syndrome, which occurred in 9 of 17 volunteers. Overall, 5 volunteers (all 3 of the high dose group and 2 of 11 of the medium dose group) reported severe adverse events. Worm-derived circulating anodic antigen, the biomarker of the primary infection endpoint, peaked in 82% of volunteers at 3–10 weeks following exposure. All volunteers showed IgM and IgG1 seroconversion and worm-specific cytokine production by CD4+T cells. All volunteers were cured with praziquantel provided at 12 weeks after exposure. Infection with 20 Schistosoma mansonicercariae led to severe adverse events in 18% of volunteers and high infection rates. This infection model paves the way for fast-track product development for treatment and prevention of schistosomiasis.

Published

2020

35. Quantitative lateral flow strip assays as User-Friendly Tools To Detect Biomarker Profiles For Leprosy

Author

van Hooij, Anouk, primary, Tjon Kon Fat, Elisa M., additional, Richardus, Renate, additional, van den Eeden, Susan J. F., additional, Wilson, Louis, additional, de Dood, Claudia J., additional, Faber, Roel, additional, Alam, Korshed, additional, Richardus, Jan Hendrik, additional, Corstjens, Paul L. A. M., additional, and Geluk, Annemieke, additional

Published

2016

36. Rapid clearance of schistosomal circulating cathodic antigen (CCA) after treatment shown by urine strip tests - importance for monitoring treatment efficacy and re-infection

Author

Kildemoes, Anna M. O., Vennervald, Birgitte J, Kabatereine, Narcis B., Tukahebwa, Edridah M., Magnussen, Pascal, Wilson, Shona, de Dood, Claudia J., Deelder, André M., Dam, Govert J. van, Kildemoes, Anna M. O., Vennervald, Birgitte J, Kabatereine, Narcis B., Tukahebwa, Edridah M., Magnussen, Pascal, Wilson, Shona, de Dood, Claudia J., Deelder, André M., and Dam, Govert J. van

Abstract

Schistosomiasis elimination has reached agendas in many public health sectors; however, reaching this goal remains a substantial challenge. In order to assess the progress of interventions and monitor treatment efficacy, accurate, feasible and affordable diagnostic tools are an absolute requirement. Detection of Schistosoma mansoni by circulating cathodic antigen (CCA) in urine is an attractive option as this measure describes active worm infection noninvasively. In order to interpret treatment efficacy and re-infections, knowledge about clearance of this antigen is necessary. This study aims to investigate whether systemic antigen clearance is reflected in decreasing CCA levels in urine afteronly 24 h in response to both a single and two treatments with praziquantel.The study was designed as a series of cross-sectional sample collections from 426 individuals nested in a two-arm randomised single blinded longitudinal clinical trial cohort matched by gender and age (ClinicalTrials.gov Identifier: NCT00215267). One arm was baseline treatment only, whereas the other arm received a second treatment at 2 weeks. Samples from baseline (urine+stool), baseline+24 h (urine), 2 weeks (urine), 2 weeks+24 h (urine), 9 weeks (urine+stool) and 2 years (urine+stool) were analysed. CCA levels in urine were determined by carbon-conjugated monoclonal antibody lateral flow strip assay and S. mansoni and soil-transmitted helminths eggs per gram (EPG) by Kato-Katz (six slides). Significant correlations between CCA levels and S. mansoniEPG at baseline, 9 weeks and 2 years regardless of treatment arm were observed. Both tests showed significantly lower levels at 9 weeks in the two treatments group compared to those only receiving one treatment. Furthermore, presence of hookworm was found not to be a confounder for CCA specificity. At baseline mean CCA scores were significantly reduced 24 h after treatment (P < 0.001). Again, at 2 weeks CCA scores were significantly lowered (P < 0.001

Published

2015

37. Sensitivity and Specificity of a Urine Circulating Anodic Antigen Test for the Diagnosis of Schistosoma haematobium in Low Endemic Settings

Author

Knopp, Stefanie, primary, Corstjens, Paul L. A. M., additional, Koukounari, Artemis, additional, Cercamondi, Colin I., additional, Ame, Shaali M., additional, Ali, Said M., additional, de Dood, Claudia J., additional, Mohammed, Khalfan A., additional, Utzinger, Jürg, additional, Rollinson, David, additional, and van Dam, Govert J., additional

Published

2015

38. Improved sensitivity of the urine CAA lateral-flow assay for diagnosing active Schistosoma infections by using larger sample volumes

Author

Corstjens, Paul LAM, primary, Nyakundi, Ruth K, additional, de Dood, Claudia J, additional, Kariuki, Thomas M, additional, Ochola, Elizabeth A, additional, Karanja, Diana MS, additional, Mwinzi, Pauline NM, additional, and van Dam, Govert J, additional

Published

2015

39. Effects of schistosomiasis on susceptibility to HIV-1 infection and HIV-1 viral load at HIV-1 seroconversion: A nested case-control study.

Author

Dupnik, Kathryn M., Lee, Myung Hee, Jr.Johnson, Warren D., Fitzgerald, Daniel W., Downs, Jennifer A., Peck, Robert N., van Dam, Govert J., Kornelis, Dieuwke, Hoekstra, Pytsje, Urassa, Mark, Lutonja, Peter, Kanjala, Chifundo, Isingo, Raphael, Changalucha, John M., de Dood, Claudia J., Corstjens, Paul L. A. M., and Todd, Jim

Subjects

SCHISTOSOMIASIS, HIV-positive persons, IMMUNOREGULATION, SURVEYS, PATIENTS, DISEASE risk factors

Abstract

Background: Schistosomiasis affects 218 million people worldwide, with most infections in Africa. Prevalence studies suggest that people with chronic schistosomiasis may have higher risk of HIV-1 acquisition and impaired ability to control HIV-1 replication once infected. We hypothesized that: (1) pre-existing schistosome infection may increase the odds of HIV-1 acquisition and that the effects may differ between men and women, and (2) individuals with active schistosome infection at the time of HIV-1 acquisition may have impaired immune control of HIV-1, resulting in higher HIV-1 viral loads at HIV-1 seroconversion. Methology/Principal findings: We conducted a nested case-control study within a large population-based survey of HIV-1 transmission in Tanzania. A population of adults from seven villages was tested for HIV in 2007, 2010, and 2013 and dried blood spots were archived for future studies with participants’ consent. Approximately 40% of this population has Schistosoma mansoni infection, and 2% has S. haematobium. We tested for schistosome antigens in the pre- and post-HIV-1-seroconversion blood spots of people who acquired HIV-1. We also tested blood spots of matched controls who did not acquire HIV-1 and calculated the odds that a person with schistosomiasis would become HIV-1-infected compared to these matched controls. Analysis was stratified by gender. We compared 73 HIV-1 seroconverters with 265 controls. Women with schistosome infections had a higher odds of HIV-1 acquisition than those without (adjusted OR = 2.8 [1.2–6.6], p = 0.019). Schistosome-infected men did not have an increased odds of HIV-1 acquisition (adjusted OR = 0.7 [0.3–1.8], p = 0.42). We additionally compared HIV-1 RNA levels in the post-seroconversion blood spots in HIV-1 seroconverters with schistosomiasis versus those without who became HIV-infected in 2010, before antiretroviral therapy was widely available in the region. The median whole blood HIV-1 RNA level in the 15 HIV-1 seroconverters with schistosome infection was significantly higher than in the 22 without schistosomiasis: 4.4 [3.9–4.6] log10 copies/mL versus 3.7 [3.2–4.3], p = 0.017. Conclusions/Significance: We confirm, in an area with endemic S. mansoni, that pre-existing schistosome infection increases odds of HIV-1 acquisition in women and raises HIV-1 viral load at the time of HIV-1 seroconversion. This is the first study to demonstrate the effect of schistosome infection on HIV-1 susceptibility and viral control, and to differentiate effects by gender. Validation studies will be needed at additional sites. [ABSTRACT FROM AUTHOR]

Published

2017

40. Field-Evaluation of a New Lateral Flow Assay for Detection of Cellular and Humoral Immunity against Mycobacterium leprae

Author

Bobosha, Kidist, primary, Tjon Kon Fat, Elisa M., additional, van den Eeden, Susan J. F., additional, Bekele, Yonas, additional, van der Ploeg-van Schip, Jolien J., additional, de Dood, Claudia J., additional, Dijkman, Karin, additional, Franken, Kees L. M. C., additional, Wilson, Louis, additional, Aseffa, Abraham, additional, Spencer, John S., additional, Ottenhoff, Tom H. M., additional, Corstjens, Paul L. A. M., additional, and Geluk, Annemieke, additional

Published

2014

41. Development of a Generic Microfluidic Device for Simultaneous Detection of Antibodies and Nucleic Acids in Oral Fluids

Author

Chen, Zongyuan, primary, Abrams, William R., additional, Geva, Eran, additional, de Dood, Claudia J., additional, González, Jesús M., additional, Tanke, Hans J., additional, Niedbala, R. Sam, additional, Zhou, Peng, additional, Malamud, Daniel, additional, and Corstjens, Paul L. A. M., additional

Published

2013

42. Association of Schistosomiasis and HIV Infection in Tanzania

Author

Downs, Jennifer A., primary, Changalucha, John M., additional, Andreasen, Aura, additional, Johnson, Warren D., additional, Kalluvya, Samuel E., additional, Fitzgerald, Daniel W., additional, de Dood, Claudia J., additional, Bang, Heejung, additional, Corstjens, Paul L. A. M., additional, van Lieshout, Lisette, additional, Peck, Robert N., additional, and van Dam, Govert J., additional

Published

2012

43. Feasibility of a Lateral Flow Test for Neurocysticercosis Using Novel Up-Converting Nanomaterials and a Lightweight Strip Analyzer.

Author

Corstjens, Paul L. A. M., de Dood, Claudia J., Priest, Jeffrey W., Tanke, Hans J., and Handali, Sukwan

Subjects

*NEUROCYSTICERCOSIS, *INFRARED technology, *PARASITIC diseases, *BACTERIAL antigens, *SERUM, *ANTIBODY titer, *NANOSTRUCTURED materials

Abstract

Neurocysticercosis is a frequent parasitic infection of the human brain, occurring in most of the world, and requires imaging of the brain to diagnose. To determine the burden of disease and to simplify diagnosis, a field-friendly rapid lateral flow (LF) based antibody screening test was developed. The assay utilizes novel nano-sized up-converting phosphor (UCP) reporter particles in combination with a portable lightweight analyzer and detects antibodies in serum samples reactive with bacterial-expressed recombinant (r) T24H, a marker for detecting neurocysticercosis cases. Three sequential flow steps allow enrichment of antibodies on the Test (T) line and consecutive binding of protein-A coated UCP reporter particles. Antibody binding was determined by measuring 550 nm emission after excitation of the UCP label with a 980 nm infrared (IR) diode. Clinical sensitivity and specificity of the assay to detect cases of human neurocysticercosis with 2 or more viable brain cysts were 96% and 98%, respectively, using a sample set comprised of sera from 63 confirmed cases and 170 healthy parasite-naïve non-endemic controls. In conclusion: Proof-of-principle, of a rapid UCP-LF screening assay for neurocysticercosis was demonstrated. The assay utilized bacterial-expressed rT24H as a potential alternative for baculovirus-expressed rT24H. Performance of the UCP-LF assay was excellent, although further studies need to confirm that bacterial expressed antigen can entirely replace previously used baculovirus antigen. In addition, the increasing availability of commercial sources for UCP reporter materials as well as the accessibility of affordable semi-handheld scanners may allow UCP-based bioanalytical systems for point-of-care to evolve at an even faster pace. Author Summary: A field-friendly screening tool to simplify serological diagnosis of neurocysticercosis was developed. The assay utilizes a rapid lateral flow based test platform in combination with unique fluorescent label, up-converting phosphor (UCP) reporter particles. The UCP reporter technology uses infrared excitation and emission of higher energy visible light. Total absence of autofluorescence provides the label with a distinctive advantage compared to common fluorescent labels. The developed assay detects antibodies against an established marker for detecting neurocysticercosis cases, recombinant T24H. In this study rT24H was produced by a bacterial expression system, a less cumbersome method compared to the previously used baculovirus expression system. With a sample set comprised of 63 confirmed neurocysticercosis cases and 170 healthy controls, clinical sensitivity and specificity were 96% and 98%, respectively. The study shows proof-of-principle that the designed UCP-rT24H assay can provide an on-site rapid screening method utilizing a mobile lightweight scanner and 40 nm yttrium fluoride UCP particles. A semi-handheld UCP reader and nano-sized UCP particles performed as good as previously used 'research and development'-only tools. Availability of commercial sources for UCP reporter materials as well as the accessibility to affordable scanners may allow UCP-based bioanalytical systems for point-of-care to evolve at an even faster pace. [ABSTRACT FROM AUTHOR]

Published

2014

44. Field-Evaluation of a New Lateral Flow Assay for Detection of Cellular and Humoral Immunity against Mycobacterium leprae.

Author

Bobosha, Kidist, Tjon Kon Fat, Elisa M., van den Eeden, Susan J. F., Bekele, Yonas, van der Ploeg-van Schip, Jolien J., de Dood, Claudia J., Dijkman, Karin, Franken, Kees L. M. C., Wilson, Louis, Aseffa, Abraham, Spencer, John S., Ottenhoff, Tom H. M., Corstjens, Paul L. A. M., and Geluk, Annemieke

Subjects

MYCOBACTERIUM, MYCOBACTERIA, MYCOBACTERIOSIS, CELLULAR immunity, TROPICAL medicine

Abstract

Background: Field-applicable tests detecting asymptomatic Mycobacterium leprae (M. leprae) infection or predicting progression to leprosy, are urgently required. Since the outcome of M. leprae infection is determined by cellular- and humoral immunity, we aim to develop diagnostic tests detecting pro-/anti-inflammatory and regulatory cytokines as well as antibodies against M. leprae. Previously, we developed lateral flow assays (LFA) for detection of cytokines and anti-PGL-I antibodies. Here we evaluate progress of newly developed LFAs for applications in resource-poor settings. Methods: The combined diagnostic value of IP-10, IL-10 and anti-PGL-I antibodies was tested using M. leprae-stimulated blood of leprosy patients and endemic controls (EC). For reduction of the overall test-to-result time the minimal whole blood assay time required to detect distinctive responses was investigated. To accommodate LFAs for field settings, dry-format LFAs for IP-10 and anti-PGL-I antibodies were developed allowing storage and shipment at ambient temperatures. Additionally, a multiplex LFA-format was applied for simultaneous detection of anti-PGL-I antibodies and IP-10. For improved sensitivity and quantitation upconverting phosphor (UCP) reporter technology was applied in all LFAs. Results: Single and multiplex UCP-LFAs correlated well with ELISAs. The performance of dry reagent assays and portable, lightweight UCP-LF strip readers indicated excellent field-robustness. Notably, detection of IP-10 levels in stimulated samples allowed a reduction of the whole blood assay time from 24 h to 6 h. Moreover, IP-10/IL-10 ratios in unstimulated plasma differed significantly between patients and EC, indicating the feasibility to identify M. leprae infection in endemic areas. Conclusions: Dry-format UCP-LFAs are low-tech, robust assays allowing detection of relevant cytokines and antibodies in response to M. leprae in the field. The high levels of IP-10 and the required shorter whole blood assay time, render this cytokine useful to discriminate between leprosy patients and EC. [ABSTRACT FROM AUTHOR]

Published

2014

45. Development of a Generic Microfluidic Device for Simultaneous Detection of Antibodies and Nucleic Acids in Oral Fluids.

Author

Zongyuan Chen, Abrams, William R., Geva, Eran, de Dood, Claudia J., González, Jesús M., Tanke, Hans J., Niedbala, R. Sam, Peng Zhou, Malamud, Daniel, and Corstjens, Paul L. A. M.

Abstract

A prototype dual-path microfluidic device (Rheonix CARD) capable of performing simultaneously screening (antigen or antibody) and confirmatory (nucleic acid) detection of pathogens is described. The device fully integrates sample processing, antigen or antibody detection, and nucleic acid amplification and detection, demonstrating rapid and inexpensive "sample-to-result" diagnosis with performance comparable to benchtop analysis. For the chip design, a modular approach was followed allowing the optimization of individual steps in the sample processing process. This modular design provides great versatility accommodating different disease targets independently of the production method. In the detection module, a lateral flow (LF) protocol utilizing upconverting phosphor (UCP) reporters was employed. The nucleic acid (NA) module incorporates a generic microtube containing dry reagents. Lateral flow strips and PCR primers determine the target or disease that is diagnosed. Diagnosis of HIV infection was used as a model to investigate the simultaneous detection of both human antibodies against the virus and viral RNA. The serological result is available in less than 30 min, and the confirmation by RNA amplification takes another 60 min. This approach combines a core serological portable diagnostic with a nucleic acid-based confirmatory test. [ABSTRACT FROM AUTHOR]

Published

2013

46. Gene Expression Differences in Host Response to Schistosoma haematobiumInfection

Author

Dupnik, Kathryn M., Reust, Mary Juliet, Vick, Kaitlin M., Yao, Benjamin, Miyaye, Donald, Lyimo, Eric, Mukerebe, Crispin, Mngara, Julius, Kalluvya, Samuel E., de Dood, Claudia J., Corstjens, Paul L. A. M., van Dam, Govert J., Zhang, Tuo, Xiang, Jenny, Lee, Myung Hee, and Downs, Jennifer A.

Abstract

Schistosome worms infect over 200 million people worldwide. They live in the host’s bloodstream and alter host immunity.

Published

2018

47. Concurrent evaluation of cytokines improves the accuracy of antibodies against Mycobacterium tuberculosis antigens in the diagnosis of active tuberculosis

Author

Ruschca Jacobs, Dolapo O. Awoniyi, Ralf Baumann, Kim Stanley, Shirley McAnda, Susanne Kaempfer, Stephanus T. Malherbe, Mahavir Singh, Gerhard Walzl, Novel N. Chegou, Magdalena Kriel, Gian van der Spuy, Andre G. Loxton, Belinda Kriel, Jayne S. Sutherland, Olumuyiwa Owolabi, Abdou Sillah, Joseph Mendy, Awa Gindeh, Simon Donkor, Toyin Togun, Martin Ota, Amelia C. Crampin, Felanji Simukonda, Alemayehu Amberbir, Femia Chilongo, Rein Houben, Desta Kassa, Atsbeha Gebrezgeabher, Getnet Mesfin, Yohannes Belay, Gebremedhin Gebremichael, Yodit Alemayehu, Marieta van der Vyver, Faustina N. Amutenya, Josefina N. Nelongo, Lidia Monye, Jacob A. Sheehama, Scholastica Iipinge, Harriet Mayanja-Kizza, Anna Ritah Namuganga, Grace Muzanye, Mary Nsereko, Pierre Peters, Rawleigh Howe, Adane Mihret, Yonas Bekele, Bamlak Tessema, Lawrence Yamuah, Tom H.M. Ottenhoff, Annemieke Geluk, Kees Franken, Jolien J. van der Ploeg-van Schip, Paul L.A.M. Corstjens, Elisa M. Tjon Kon Fat, Claudia J. de Dood, Ida Rosenkrands, Claus Aagaard, Stefan H.E. Kaufmann, Maria M. Esterhuyse, Jacqueline M. Cliff, Hazel M. Dockrell, AE-TBC Consortium, Walzl, Gerhard, Chegou, Novel N., Kriel, Magdalena, van der Spuy, Gian, Loxton, Andre G., Stanley, Kim, Malherbe, Stephanus T., Kriel, Belinda, Sutherland, Jayne S., Owolabi, Olumuyiwa, Sillah, Abdou, Mendy, Joseph, Gindeh, Awa, Donkor, Simon, Togun, Toyin, Ota, Martin, Crampin, Amelia C., Simukonda, Felanji, Amberbir, Alemayehu, Chilongo, Femia, Houben, Rein, Kassa, Desta, Gebrezgeabher, Atsbeha, Mesfin, Getnet, Belay, Yohannes, Gebremichael, Gebremedhin, Alemayehu, Yodit, van der Vyver, Marieta, Amutenya, Faustina N., Nelongo, Josefina N., Monye, Lidia, Sheehama, Jacob A., Iipinge, Scholastica, Mayanja-Kizza, Harriet, Namuganga, Anna Ritah, Muzanye, Grace, Nsereko, Mary, Peters, Pierre, Howe, Rawleigh, Mihret, Adane, Bekele, Yonas, Tessema, Bamlak, Yamuah, Lawrence, Ottenhoff, Tom H. M., Geluk, Annemieke, Franken, Kees, van der Ploeg-van Schip, Jolien J., Corstjens, Paul L. A. M., Tjon Kon Fat, Elisa M., de Dood, Claudia J., Rosenkrands, Ida, Aagaard, Claus, Kaufmann, Stefan H. E., Esterhuyse, Maria M., Cliff, Jacqueline M., and Dockrell, Hazel M.

Subjects

Microbiology (medical), Antigens, Bacterial, diagnosis, Immunology, biomarkers, Enzyme-Linked Immunosorbent Assay, Mycobacterium tuberculosis, Antibodies, Bacterial, Sensitivity and Specificity, Microbiology, cytokines, Antibodies, Immunoglobulin A, Infectious Diseases, tuberculosis, antigens, Diagnosis, Humans, antibodies, Tuberculosis, Cytokines, Antigens, Biomarkers

Abstract

Tuberculosis 133, 102169 (2022). doi:10.1016/j.tube.2022.102169, Published by Churchill Livingstone, Edinburgh

Published

2022

48. Field-Evaluation of a New Lateral Flow Assay for Detection of Cellular and Humoral Immunity against Mycobacterium leprae.

Author

Bobosha, Kidist, Tjon Kon Fat, Elisa M., van den Eeden, Susan J. F., Bekele, Yonas, van der Ploeg-van Schip, Jolien J., de Dood, Claudia J., Dijkman, Karin, Franken, Kees L. M. C., Wilson, Louis, Aseffa, Abraham, Spencer, John S., Ottenhoff, Tom H. M., Corstjens, Paul L. A. M., and Geluk, Annemieke

Subjects

*MYCOBACTERIUM, *MYCOBACTERIA, *MYCOBACTERIOSIS, *CELLULAR immunity, *TROPICAL medicine

Abstract

Background: Field-applicable tests detecting asymptomatic Mycobacterium leprae (M. leprae) infection or predicting progression to leprosy, are urgently required. Since the outcome of M. leprae infection is determined by cellular- and humoral immunity, we aim to develop diagnostic tests detecting pro-/anti-inflammatory and regulatory cytokines as well as antibodies against M. leprae. Previously, we developed lateral flow assays (LFA) for detection of cytokines and anti-PGL-I antibodies. Here we evaluate progress of newly developed LFAs for applications in resource-poor settings. Methods: The combined diagnostic value of IP-10, IL-10 and anti-PGL-I antibodies was tested using M. leprae-stimulated blood of leprosy patients and endemic controls (EC). For reduction of the overall test-to-result time the minimal whole blood assay time required to detect distinctive responses was investigated. To accommodate LFAs for field settings, dry-format LFAs for IP-10 and anti-PGL-I antibodies were developed allowing storage and shipment at ambient temperatures. Additionally, a multiplex LFA-format was applied for simultaneous detection of anti-PGL-I antibodies and IP-10. For improved sensitivity and quantitation upconverting phosphor (UCP) reporter technology was applied in all LFAs. Results: Single and multiplex UCP-LFAs correlated well with ELISAs. The performance of dry reagent assays and portable, lightweight UCP-LF strip readers indicated excellent field-robustness. Notably, detection of IP-10 levels in stimulated samples allowed a reduction of the whole blood assay time from 24 h to 6 h. Moreover, IP-10/IL-10 ratios in unstimulated plasma differed significantly between patients and EC, indicating the feasibility to identify M. leprae infection in endemic areas. Conclusions: Dry-format UCP-LFAs are low-tech, robust assays allowing detection of relevant cytokines and antibodies in response to M. leprae in the field. The high levels of IP-10 and the required shorter whole blood assay time, render this cytokine useful to discriminate between leprosy patients and EC. [ABSTRACT FROM AUTHOR]

Published

2014