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2. Zoonotic Ancylostoma ceylanicum Hookworm Infections, Ecuador

Author

Sears, William J., Cardenas, Jorge, Kubofcik, Joseph, Nutman, Thomas B., and Cooper, Philip J.

Subjects
Zoonoses -- Risk factors, Disease transmission -- Risk factors, Hookworm disease -- Risk factors, Health
Abstract

Ancylostoma ceylanicum hookworms can infect humans and have been increasingly recognized as endemic among humans living or traveling to the Asia-Pacific region (1). Although A. ceylanicum hookworms are known to [...]

Published
2022
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4. Isolation of Onchocerca lupi in dogs and black flies, California, USA

Author

Hassan, Hassan K., Bolcen, Shanna, Kubofcik, Joseph, Nutman, Thomas B., Eberhard, Mark L., Middleton, Kelly, Wekesa, Joseph Wakoli, Ruedas, Gimena, Nelson, Kimberly J., Dubielzig, Richard, De Lombaert, Melissa, Silverman, Bruce, Schorling, Jamie J., Adler, Peter H., Unnasch, Thomas R., and Beeler, Emily S.

Subjects
Cytochrome oxidase -- Analysis -- Health aspects, Dogs -- Analysis -- Health aspects, RNA -- Analysis -- Health aspects, Health
Abstract

Onchocerca lupi is a zoonotic parasite capable of infecting dogs, cats, and humans. Human infection was first suspected in 2002, when a case of human subconjunctival filariasis was found to [...]

Published
2015
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7. A randomized trial of doxycycline for mansonella perstans infection

Author

Coulibaly, Yaya I., Dembele, Benoit, Diallo, Abdallah A., Lipner, Ettie M., Doumbia, Salif S., Coulibaly, Siaka Y., Konate, Siaka, Diallo, Dapa A., Yalcouye, Daniel, Kubofcik, Joseph, Doumbo, Ogobara K., Traore, Sekou F., Keita, Adama D., Fay, Michael P., Nutman, Thomas B., and Kilion, Amy D.

Subjects
Doxycycline -- Usage, Roundworm infections -- Care and treatment
Abstract

A study was conducted to evaluate the efficacy of doxycycline in the treatment of mansonella perstans infection. Results indicated that doxycycline was found to be an effective treatment option for the ailment, and also that mansonella perstans infection does contain bacterial endosymbionts.

Published
2009

9. Inherited Resistance to HIV-1 Conferred by an Inactivating Mutation in CC Chemokine Receptor 5: Studies in Populations with Contrasting Clinical Phenotypes, Defined Racial Background, and Quantified Risk

Author

Zimmerman, Peter A., Buckler-White, Alicia, Alkhatib, Ghalib, Spalding, Todd, Kubofcik, Joseph, Combadiere, Christophe, Weissman, Drew, Cohen, Oren, Rubbert, Andrea, Lam, Gordon, Vaccarezza, Mauro, Kennedy, Paul E., Kumaraswami, V., Giorgi, Janis V., Detels, Roger, Hunter, Jay, Chopek, Michael, Berger, Edward A., Fauci, Anthony S., Nutman, Thomas B., and Murphy, Philip M.

Published
1997
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13. Loa loa Microfilariae in Skin Snips: Consequences for Onchocerciasis Monitoring and Evaluation in L. loa–Endemic Areas.

Author

Nana-Djeunga, Hugues C, Fossuo-Thotchum, Floribert, Pion, Sébastien D, Chesnais, Cédric B, Kubofcik, Joseph, Mackenzie, Charles D, Klion, Amy D, Boussinesq, Michel, Nutman, Thomas B, and Kamgno, Joseph

Subjects
FILARIASIS, MOLECULAR diagnosis, ONCHOCERCIASIS, SKIN tests
Abstract

The specificity of skin snips for onchocerciasis diagnoses is considered to be almost 100%. Our molecular methods revealed that microfilariae emerging from skin snips collected from highly microfilaremic Loa loa– infected individuals were largely misidentified as Onchocerca volvulus. This has important implications for onchocerciasis diagnostic testing in Loa -endemic areas. [ABSTRACT FROM AUTHOR]

Published
2019
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15. Comparison of antigen and antibody responses in repeat lymphatic filariasis transmission assessment surveys in American Samoa.

Author

Won, Kimberly Y., Robinson, Keri, Hamlin, Katy L., Tufa, Joseph, Seespesara, Margaret, Wiegand, Ryan E., Gass, Katherine, Kubofcik, Joseph, Nutman, Thomas B., Lammie, Patrick J., and Fuimaono, Saipale

Subjects
FILARIASIS, HELMINTHIASIS, NEMATODE infections, SPIRURIDA diseases, LOAIASIS
Abstract

Background: Current WHO recommendations for lymphatic filariasis (LF) surveillance advise programs to implement activities to monitor for new foci of transmission after stopping mass drug administration (MDA). A current need in the global effort to eliminate LF is to standardize diagnostic tools and surveillance activities beyond the recommended transmission assessment survey (TAS). Methodology: TAS was first conducted in American Samoa in 2011 (TAS 1) and a repeat TAS was carried out in 2015 (TAS 2). Circulating filarial antigen (CFA) and serologic results from both surveys were analyzed to determine whether interruption of LF transmission has been achieved in American Samoa. Principal findings: A total of 1,134 and 864 children (5–10 years old) were enrolled in TAS 1 and TAS 2, respectively. Two CFA-positive children were identified in TAS 1, and one CFA-positive child was identified in TAS 2. Results of both surveys were below the threshold for which MDA was warranted. Additionally, 1,112 and 836 dried blood spots from TAS 1 and TAS 2, respectively were tested for antibodies to Wb123, Bm14 and Bm33 by luciferase immunoprecipitation system (LIPS) assay and multiplex bead assay. In 2011, overall prevalence of responses to Wb123, Bm14, and Bm33 was 1.0%, 6.8% and 12.0%, respectively. In 2015, overall prevalence of positive Bm14 and Bm33 responses declined significantly to 3.0% (p<0.001) and 7.8% (p = 0.013), respectively. Conclusions/Significance: Although passing TAS 1 and TAS 2 and an overall decline in the prevalence of antibodies to Bm14 and Bm33 between these surveys suggests decreased exposure and infection among young children, there were persistent responses in some schools. Clustering and persistence of positive antibody responses in schools may be an indication of ongoing transmission. There is a need to better understand the limitations of current antibody tests, but our results suggest that serologic tools can have a role in guiding programmatic decision making. [ABSTRACT FROM AUTHOR]

Published
2018
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16. Measuring changes in transmission of neglected tropical diseases, malaria, and enteric pathogens from quantitative antibody levels.

Author

Arnold, Benjamin F., van der Laan, Mark J., Hubbard, Alan E., Steel, Cathy, Kubofcik, Joseph, Hamlin, Katy L., Moss, Delynn M., Nutman, Thomas B., Priest, Jeffrey W., and Lammie, Patrick J.

Subjects
TROPICAL medicine, MALARIA, PATHOGENIC microorganisms, IMMUNOGLOBULINS, IMMUNOLOGY
Abstract

Background: Serological antibody levels are a sensitive marker of pathogen exposure, and advances in multiplex assays have created enormous potential for large-scale, integrated infectious disease surveillance. Most methods to analyze antibody measurements reduce quantitative antibody levels to seropositive and seronegative groups, but this can be difficult for many pathogens and may provide lower resolution information than quantitative levels. Analysis methods have predominantly maintained a single disease focus, yet integrated surveillance platforms would benefit from methodologies that work across diverse pathogens included in multiplex assays. Methods/Principal findings: We developed an approach to measure changes in transmission from quantitative antibody levels that can be applied to diverse pathogens of global importance. We compared age-dependent immunoglobulin G curves in repeated cross-sectional surveys between populations with differences in transmission for multiple pathogens, including: lymphatic filariasis (Wuchereria bancrofti) measured before and after mass drug administration on Mauke, Cook Islands, malaria (Plasmodium falciparum) before and after a combined insecticide and mass drug administration intervention in the Garki project, Nigeria, and enteric protozoans (Cryptosporidium parvum, Giardia intestinalis, Entamoeba histolytica), bacteria (enterotoxigenic Escherichia coli, Salmonella spp.), and viruses (norovirus groups I and II) in children living in Haiti and the USA. Age-dependent antibody curves fit with ensemble machine learning followed a characteristic shape across pathogens that aligned with predictions from basic mechanisms of humoral immunity. Differences in pathogen transmission led to shifts in fitted antibody curves that were remarkably consistent across pathogens, assays, and populations. Mean antibody levels correlated strongly with traditional measures of transmission intensity, such as the entomological inoculation rate for P. falciparum (Spearman’s rho = 0.75). In both high- and low transmission settings, mean antibody curves revealed changes in population mean antibody levels that were masked by seroprevalence measures because changes took place above or below the seropositivity cutoff. Conclusions/Significance: Age-dependent antibody curves and summary means provided a robust and sensitive measure of changes in transmission, with greatest sensitivity among young children. The method generalizes to pathogens that can be measured in high-throughput, multiplex serological assays, and scales to surveillance activities that require high spatiotemporal resolution. Our results suggest quantitative antibody levels will be particularly useful to measure differences in exposure for pathogens that elicit a transient antibody response or for monitoring populations with very high- or very low transmission, when seroprevalence is less informative. The approach represents a new opportunity to conduct integrated serological surveillance for neglected tropical diseases, malaria, and other infectious diseases with well-defined antigen targets. [ABSTRACT FROM AUTHOR]

Published
2017
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18. Extended Result Reading Window in Lateral Flow Tests Detecting Exposure to Onchocerca volvulus: A New Technology to Improve Epidemiological Surveillance Tools.

Author

Golden, Allison, Steel, Cathy, Yokobe, Lindsay, Jackson, Emily, Barney, Rebecca, Kubofcik, Joseph, Peck, Roger, Unnasch, Thomas R., Nutman, Thomas B., de los Santos, Tala, and Domingo, Gonzalo J.

Subjects
ONCHOCERCIASIS, TROPICAL medicine, ONCHOCERCA volvulus, EPIDEMIOLOGY, PUBLIC health surveillance, PARASITES, IMMUNOGLOBULIN G, DISEASE risk factors
Abstract

Onchocerciasis is a neglected tropical disease caused by infection with the parasite Onchocerca volvulus (Ov). An estimated 180 million people are at risk for Ov infection, and 37 million people are infected, mostly in Africa. A lateral flow-based assay to detect human IgG4 antibodies to the Ov-specific antigen Ov-16 was developed as a rapid tool to detect exposure to Ov. The test, when performed on 449 sera specimens from patients with microfiladermia and Ov-negative patients, has a sensitivity of 89.1% (95% confidence interval: 86.2%–92.0%), and specificity of 97% (95% confidence interval: 95.4%–98.6%). Because the intended use of the test is for surveillance, it is highly desirable to have a stable, long-lasting result. An extended read window is thus desirable for a high-volume, busy workflow and facilitates post-surveillance quality assurance. The main restriction on achieving an extended read window for this assay was the erythrocyte lysis that can alter the signal-to-noise ratio, especially in those with low IgG4 levels (weak positives). We describe a test housing that incorporates a user-independent feature driven by assay fluid and an expanding wick that detaches the blood separation membrane from the nitrocellulose used in the assay, but before hemolysis occurs. We demonstrated material functionality at extreme operational conditions (37°C, 80% relative humidity) and a read window of a minimum of 70 days. The fluid-driven assay device performs equally as well with whole blood as with plasma, as demonstrated with 100 spiked clinical specimens (with a correlation coefficient of 0.96). We show a novel, inexpensive, and simple approach to actuating the detachment of the blood separation membrane from the nitrocellulose test with no impact on the performance characteristics of the test. [ABSTRACT FROM AUTHOR]

Published
2013
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19. Antibody to the Filarial Antigen Wb123 Reflects Reduced Transmission and Decreased Exposure in Children Born following Single Mass Drug Administration (MDA).

Author

Steel, Cathy, Kubofcik, Joseph, Ottesen, Eric A., and Nutman, Thomas B.

Subjects
*DRUG administration, *ANTIGENS, *IMMUNOGLOBULINS, *FILARIASIS, *FILARIAL worms
Abstract

Background: Antibody (Ab) to the Wuchereria bancrofti (Wb) infective larval (L3) antigen Wb123, using a Luciferase Immunoprecipitation System (LIPS) assay, has been shown to be a species-specific, early marker of infection developed for potential use as a surveillance tool following transmission interruption post mass drug administration. To examine its usefulness in a single filarial-endemic island assessed at two time points with markedly different levels of transmission, Ab to Wb123 was measured in sera collected from subjects from Mauke, Cook Islands in 1975 (no previous treatment) and 1992 (5 years after a one time island-wide treatment with diethylcarbamazine [DEC]). Findings: Between 1975 and 1992, Wb transmission decreased dramatically as evidenced by reduced prevalences of microfilariae (31% vs. 5%) and circulating Ag (CAg, 49% vs. 16%). Age specific prevalence analysis showed a dramatic reduction in Wb123 Ab positivity from 54% (25/46) in 1975 to 8% (3/38) in 1992 in children 1–5 years (p<0.0001), reflecting the effects of single-dose treatment five years earlier. By 1992, Wb123 Ab prevalence in children 6–10 years had fallen from 75% (42/56) in 1975 to 42% (33/79) consistent with a lower cumulative transmission potential. In the whole population, Wb123 seropositivity decreased from 86% to 60% between 1975 and 1992. In CAg+ subjects the levels of Wb123 Ab were indistinguishable between the 2 time points but differed in those who were CAg− (p<0.0001). In paired sample analysis, individuals who were CAg+ in 1975 but became CAg− in 1992 had significantly lower Ab levels in 1992 (p<0.0001), with 9/40 (23%) becoming seronegative for Wb123. Conclusions: The relationship between reduction in Wb123 Ab prevalence and the reduction of transmission, seen most clearly in young children, strongly advocates for the continuing assessment and rapid development of Wb123 as a surveillance tool to detect potential transmission of bancroftian filariasis in treated endemic areas. Author Summary: Lymphatic filariasis (LF) causes an enormous disease burden throughout the tropics and subtropics. The Global Programme to Eliminate Lymphatic Filariasis was begun in 2000 following the advent of large donations from drug companies for treating LF and the development of a rapid antigen assay for detection of infection. As more countries undergo mass drug administration (MDA), the driving need is for development of a highly sensitive and specific antibody assay for detecting ongoing exposure to vector-borne filaria following MDA. The target group for such surveillance is children born during or following MDA. Current assays, while sensitive, are not specific enough where non-LF filaria species are co-endemic. Recently, we developed an antibody assay based upon the highly specific larval antigen Wb123 using the Luciferase Immunoprecipitation System (LIPS). In the current study, we determined that the Wb123 LIPS assay detects a reduction in LF transmission on an endemic island following a one-time island wide MDA with diethylcarbamazine, with the most pronounced reduction in prevalence of antibody to Wb123 occurring in young children born just prior to and following this MDA. We propose that Wb123 can be an extremely useful surveillance tool following MDA and should be developed into a rapid test format. [ABSTRACT FROM AUTHOR]

Published
2012
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20. Identification of Wb123 as an Early and Specific Marker of Wuchereria bancrofti Infection.

Author

Kubofcik, Joseph, Fink, Doran L., and Nutman, Thomas B.

Subjects
*RENILLA luciferase, *FILARIASIS, *ONCHOCERCA volvulus, *CHIMERIC proteins, *ANTIBODY titer
Abstract

Background: The current antibody tests used for monitoring in lymphatic filariasis (LF) elimination programs suffer from poor specificity because of the considerable geographical overlap with other filarial infections such as Loa loa (Ll), Onchocerca volvulus (Ov), and Mansonella perstans (Mp). Methods: Using bioinformatics to assemble into contigs 2048 expressed sequence tags (ESTs) from the L3 infective larvae of W. bancrofti (Wb), these were next assessed for homology to known proteins and nucleotides and to similar assemblies of L3 larval ESTs of B. malayi (Bm – n = 5068), Ov (n = 4166), and Ll (n = 3315). Nineteen potential L3- and Wb- and/or Bm-specific antigens were identified. Sixteen of the 19 antigens could be expressed as fusion proteins with Renilla luciferase (Ruc); these were used in a rapid Luciferase Immunopreciptation System (LIPS) assay. Results: One of the 16 expressed antigens (Wb123) was both highly immunogenic and specific for Wb. Using Wb123-based IgG and IgG4 LIPS assays on well-defined sera from normal North Americans and those infected exclusively with intestinal helminths, we could detect all of the Wb-infected individuals (from diverse geographic regions) with 100% sensitivity and 100% specificity. Using sera from exclusively Ll-infected, Ov-infected Mp-infected or Bm-infected subjects as the negative comparator, the sensitivities were between 98–100% and the specificities ranged between 84–100% (for IgG anti-Wb123) and between 98–100% (for IgG4 anti-Wb123). Blinded assessments using panels of sera from various Wb-, Bm- or non-Wb helminth-infected subjects demonstrated equally high degrees of sensitivity and specificity. Significance: We have identified a Wb-encoded antigen that can be used both as a rapid, high throughput tool to diagnose individual Wb infections and as a sensitive method for early detection of recrudescent infections in areas of control and for mapping new areas of Wb transmission. Author Summary: To address an unmet need for a surveillance tool to detect transmission of Wuchereria bancrofti (Wb), a causative agent of lymphatic filariasis, following mass drug administration (MDA) control measures, we used a novel bioinformatic approach to identify Wb-specific antigens expressed primarily by the infective stage larvae of Wb that could be used as the basis for a rapid, high throughput antibody assay. From 19 potential candidates, we identified one, termed Wb123, that could be used as the basis for the rapid detection of IgG and IgG4 reactivity in a luciferase immunoprecipitation system (LIPS) assay. These anti-Wb123 IgG and IgG4 antibodies were only present in those with Wb infection and not in those infected with closely related filarial parasites (e.g. Onchocerca volvulus, Loa loa, Mansonella perstans) that share the same geographical niches with Wb. Our data suggest that this rapid Wb123 assay has the potential to be used in for large scale detection of recrudescent Wb infection and thereby may provide a new tool for the monitoring of transmission control measures. [ABSTRACT FROM AUTHOR]

Published
2012
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21. Longitudinal Monitoring of the Development of Antifilarial Antibodies and Acquisition of Wuchereria bancrofti in a Highly Endemic Area of Haiti.

Author

Hamlin, Katy L., Moss, Delynn M., Priest, Jeffrey W., Roberts, Jacquelin, Kubofcik, Joseph, Gass, Katherine, Streit, Thomas G., Nutman, Thomas B., Eberhard, Mark L., and Lammie, Patrick J.

Subjects
ANTIBODY formation, IMMUNOGLOBULINS, ANTIBODY titer, CELL surface antigens, INFECTIOUS disease transmission
Abstract

Antifilarial antibody testing has been established as a sensitive and specific method of diagnosing lymphatic filariasis. However, the development of serological responses to specific filarial antigens and their relationship to acquisition of infection is poorly understood. In order to evaluate whether the development of antigen specific antifilarial antibodies precedes microfilaremia and antigenemia, we compared the antibody responses of serum samples collected between 1990 and 1999 from a cohort of 142 Haitian children followed longitudinally. Antigen status was determined using the Og4C3 ELISA and the presence of microfilaremia was detected using microscopy. Antibody responses to Wb123, a Wuchereria bancrofti L3 antigen, were measured using a Luciferase Immunoprecipitation System (LIPS) assay. Antibody responses to Bm14 and Bm33, Brugia malayi antigens and to a major surface protein (WSP) from Wolbachia were analyzed using a multiplex bead assay. Over follow-up, 80 (56%) of the children became antigen-positive and 30 (21%) developed microfilaremia. Detectable antibody responses to Bm14, Bm33, Wb123, and WSP developed in 95%, 100%, 92%, and 29% of children, respectively. With the exception of WSP, the development of antibody responses generally preceded detection of filarial antigen. Our results show that antifilarial antibody responses can serve as an important epidemiological indicator in a sentinel population of young children and thus, may be valuable as tool for surveillance in the context of lymphatic filariasis elimination programs. Author Summary: Programs to eliminate lymphatic filariasis (LF) are designed to interrupt transmission of the parasite by treating the human reservoir of infection. As infection levels decline, assessing infection and transmission levels becomes more and more challenging. In principle, measuring the level of antibody to filarial antigens in children may provide a sensitive measure of transmission intensity. Here, we used samples collected over time from 142 Haitian children living in an area of intense transmission of LF to determine when they first developed antibody responses to defined filarial antigens compared to when they became infected. Antibody responses were measured to several filarial antigens using sensitive assays based on multiplex and LIPS assay methods. Our results show that antibody responses developed before infection could be detected by conventional tests for the presence of microfilariae or antigen in the blood. These results support the idea that antibody tests can be used to monitor the impact of mass drug administration programs on transmission of LF and to carry out surveillance for LF after drug treatments have stopped. [ABSTRACT FROM AUTHOR]

Published
2012
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22. Longitudinal Monitoring of the Development of Antifilarial Antibodies and Acquisition of Wuchereria bancrofti in a Highly Endemic Area of Haiti

Author

Hamlin, Katy L., Moss, Delynn M., Priest, Jeffrey W., Roberts, Jacquelin, Kubofcik, Joseph, Gass, Katherine, Streit, Thomas G., Nutman, Thomas B., Eberhard, Mark L., and Lammie, Patrick J.

Subjects
FILARIASIS prevention, FILARIAL worms, IMMUNOGLOBULINS, SERODIAGNOSIS, LONGITUDINAL method
Abstract

Antifilarial antibody testing has been established as a sensitive and specific method of diagnosing lymphatic filariasis. However, the development of serological responses to specific filarial antigens and their relationship to acquisition of infection is poorly understood. In order to evaluate whether the development of antigen specific antifilarial antibodies precedes microfilaremia and antigenemia, we compared the antibody responses of serum samples collected between 1990 and 1999 from a cohort of 142 Haitian children followed longitudinally. Antigen status was determined using the Og4C3 ELISA and the presence of microfilaremia was detected using microscopy. Antibody responses to Wb123, a Wuchereria bancrofti L3 antigen, were measured using a Luciferase Immunoprecipitation System (LIPS) assay. Antibody responses to Bm14 and Bm33, Brugia malayi antigens and to a major surface protein (WSP) from Wolbachia were analyzed using a multiplex bead assay. Over follow-up, 80 (56%) of the children became antigen-positive and 30 (21%) developed microfilaremia. Detectable antibody responses to Bm14, Bm33, Wb123, and WSP developed in 95%, 100%, 92%, and 29% of children, respectively. With the exception of WSP, the development of antibody responses generally preceded detection of filarial antigen. Our results show that antifilarial antibody responses can serve as an important epidemiological indicator in a sentinel population of young children and thus, may be valuable as tool for surveillance in the context of lymphatic filariasis elimination programs. [ABSTRACT FROM AUTHOR]

Published
2012
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23. Identification of Wb123 as an Early and Specific Marker of Wuchereria bancrofti Infection

Author

Kubofcik, Joseph, Fink, Doran L., and Nutman, Thomas B.

Subjects
FILARIASIS, ONCHOCERCA volvulus, BIOINFORMATICS, TROPICAL medicine, RECEIVER operating characteristic curves
Abstract

Background: The current antibody tests used for monitoring in lymphatic filariasis (LF) elimination programs suffer from poor specificity because of the considerable geographical overlap with other filarial infections such as Loa loa (Ll), Onchocerca volvulus (Ov), and Mansonella perstans (Mp). Methods: Using bioinformatics to assemble into contigs 2048 expressed sequence tags (ESTs) from the L3 infective larvae of W. bancrofti (Wb), these were next assessed for homology to known proteins and nucleotides and to similar assemblies of L3 larval ESTs of B. malayi (Bm – n = 5068), Ov (n = 4166), and Ll (n = 3315). Nineteen potential L3- and Wb- and/or Bm-specific antigens were identified. Sixteen of the 19 antigens could be expressed as fusion proteins with Renilla luciferase (Ruc); these were used in a rapid Luciferase Immunopreciptation System (LIPS) assay. Results: One of the 16 expressed antigens (Wb123) was both highly immunogenic and specific for Wb. Using Wb123-based IgG and IgG4 LIPS assays on well-defined sera from normal North Americans and those infected exclusively with intestinal helminths, we could detect all of the Wb-infected individuals (from diverse geographic regions) with 100% sensitivity and 100% specificity. Using sera from exclusively Ll-infected, Ov-infected Mp-infected or Bm-infected subjects as the negative comparator, the sensitivities were between 98–100% and the specificities ranged between 84–100% (for IgG anti-Wb123) and between 98–100% (for IgG4 anti-Wb123). Blinded assessments using panels of sera from various Wb-, Bm- or non-Wb helminth-infected subjects demonstrated equally high degrees of sensitivity and specificity. Significance: We have identified a Wb-encoded antigen that can be used both as a rapid, high throughput tool to diagnose individual Wb infections and as a sensitive method for early detection of recrudescent infections in areas of control and for mapping new areas of Wb transmission. [ABSTRACT FROM AUTHOR]

Published
2012
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24. Molecular identification of Wolbachia from the filarial nematode Mansonella perstans

Author

Keiser, Paul B., Coulibaly, Yaya, Kubofcik, Joseph, Diallo, Abdallah A., Klion, Amy D., Traoré, Sekou F., and Nutman, Thomas B.

Subjects
*WOLBACHIA, *NUCLEIC acids, *NEMATODES, *FILARIASIS
Abstract

Abstract: Wolbachiae are bacterial endosymbionts of insects and many filarial nematodes whose products trigger inflammation in filarial infections. The dependence of the parasites on their endosymbionts has also led to the use of antibiotics directed against the Wolbachiae, therapy that has been demonstrated to have a profound salutary effect on filarial infections. The identification of Wolbachiae in Mansonella species has been conclusively shown for Mansonella ozzardi (Mo), but not for Mansonella perstans (Mp). Using primers known to amplify the 16S ribosomal DNA of other filarial Wolbachiae, an identical 1393bp band was found in all samples tested. Sequence analysis of these samples demonstrated a single consensus sequence for Mp Wolbachia 16S rDNA that was most similar to Wolbachia sequences from other filarial nematodes. When aligned with the only other Mansonella Wolbachia sequence (Mo) there were only 8 nucleotide differences in the 1369bp overlapping sequence. Phylogenetic dendrograms, examining the relationship of the Mp Wolbachia to other Wolbachia 16S rDNA, showed that the Wolbachia tracked almost identically to the 5S rRNA of their parasite host. Wolbachia surface protein (WSP) was also demonstrated in protein extracted from Mp-containing whole blood. In advance of a treatment trial of Mp, a method for the quantitation of Mp Wolbachia was developed and used to demonstrate not only a relationship between microfilarial numbers and Wolbachia copy numbers, but also to demonstrate the effect of antibiotic on ridding Mp of Wolbachia. [Copyright &y& Elsevier]

Published
2008
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