Preliminary antigenic characterisation of an adult worm vomit preparation of Fasciola hepatica by infected human sera

Almeida, María Alejandra De; Ferreira, Maria B.; Planchart, Sandra; Terashima, Angélica; Maco, Vicente; Marcos, Luis A.; Gotuzzo, Eduardo; Sánchez, Elizabeth; Náquira, César; Scorza, J. V.; Incani, Renzo Nino

doi:10.1590/s0036-46652007000100006

Cited by 14 publications

(15 citation statements)

References 26 publications

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“…Differences in number and molecular weight of reported protein bands of ES or In study of Gonence and Sarimehmetoglu (2004) serum of infected sheep, with F. hepatica, reacted with protein bands of 24,33,35,[44][45][46][47][48][49][50][51][52][53][54][55], and 66 kDa of F. hepatica somatic antigen, and protein bands of 24, 33, 39.5, 42 and 44-55 kDa of F. hepatica ES antigen. In other study, serum of human infected with F. hepatica reacted with bands of 8, 12, 15, and 24 kDa in western blotting on F. hepatica vomiting antigen (De Almeida et al 2007). In our study, rabbit polyclonal antibodies to F. hepatica ES antigen detected 11 bands in F. hepatica somatic and ES antigen, most of them are different from those reported by De Almeida et al (2007).…”

Section: Discussionmentioning

confidence: 77%

“…In other study, serum of human infected with F. hepatica reacted with bands of 8, 12, 15, and 24 kDa in western blotting on F. hepatica vomiting antigen (De Almeida et al 2007). In our study, rabbit polyclonal antibodies to F. hepatica ES antigen detected 11 bands in F. hepatica somatic and ES antigen, most of them are different from those reported by De Almeida et al (2007).…”

Section: Discussionmentioning

confidence: 77%

“…Eight protein bands reported in their study are common with those that we are seeing in the current study. De Almeida et al (2007) reported 17 protein bands (ranging from 2 to 80 kDa) in F. hepatica somatic antigen (De Almeida et al 2007). Meshgi et al (2008) reported six common protein bands (ranging from 15 to 42 kDa) for SDS PAGE pattern of both F. hepatica and F. gigantica ES antigens.…”

Section: Discussionmentioning

confidence: 99%

“…In a study by Gonenc et al (2004) 23 protein bands (ranging from 6.5 to 205 kDa) for F. hepatica ES antigen have been reported. De Almeida et al reported 19 protein bands (ranging from 2 to 80 kDa) for F. hepatica vomiting antigen (ES antigen) (De Almeida et al 2007). In the current study, five and nine protein bands have been respectively detected in F. hepatica and F. gigantica ES antigens.…”

Section: Discussionmentioning

confidence: 99%

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Detection of Fasciola hepatica and Fasciola gigantica common and uncommon antigens, using rabbit hyper immune serum raised against their excretory–secretory and somatic antigens

Khabisi

Sarkari

2016

J Parasit Dis

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Fasciolosis is an important neglected helminth disease caused by two liver flukes, Fasciola hepatica and Fasciola gigantica. The two species of Fasciola are usually different in their morphological and molecular features. They have also common and uncommon antigens in both their somatic and excretory secretory metabolites. In this study, we compared somatic and excretory-secretory (ES) antigens of F. hepatica and F. gigantica, by using rabbit hyper immune serum raised against these antigens. Adult worms were collected from bile ducts of infected animals and species of the fluke was confirmed by RFLP-PCR. ES and somatic antigens of both species were prepared. Rabbits were subcutaneously immunized with either ES or somatic antigens to produce antibodies against these antigens. SDS-PAGE pattern of F. hepatica and F. gigantica somatic antigens was similar and both of them revealed 30 protein bands, ranging from 18 to 180 kDa. In contrast, SDS-PAGE pattern of ES antigen of the two species was different. While protein bands with molecular weight of 18, 27, 29, 48, and 62 kDa were common in both species, bands of 19, 45, 55 and 58 kDa were only noticed in F. hepatica ES antigen. Rabbit polyclonal antibodies, raised against F. hepatica and F. gigantica ES antigen, reacted with main five protein bands, 25, 27, 29, 62 and 67 kDa and polyclonal antibodies raised against somatic antigens of both species reacted with three protein bands, 25, 27 and 72 kDa. Thus, the 25, 27 and 29 kDa protein bands may serve as immunodominant antigens, which might be considered for serodiagnosis of fasciolosis. Moreover, bands of 62 and 67 kDa in ES antigen and 72 kDa in somatic antigens of both species were immunodominant and might be suitable candidate for development of serological assays for diagnosis of fasciolosis.

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Section: Discussionmentioning

confidence: 77%

Section: Discussionmentioning

confidence: 77%

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

See 2 more Smart Citations

Detection of Fasciola hepatica and Fasciola gigantica common and uncommon antigens, using rabbit hyper immune serum raised against their excretory–secretory and somatic antigens

Khabisi

Sarkari

2016

J Parasit Dis

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“…Algunos análisis electroforéticos y bioquímicos del antígeno total AgMFhE/S de F. hepatica, mostraron 31 bandas de naturaleza polipeptídica en rango de 10-116 KDa, dentro de los cuales destacan un grupo de siete polipéptidos entre 66-116 KDa; un segundo grupo de nueve polipéptidos entre 60-31 KDa, un tercero con seis polipéptidos entre 29-17 KDa, y una agrupación de nueve polipéptidos entre 10-15 KDa (3,4) . Estos antígenos son utilizados en pruebas serológicas con enfoque diagnóstico, con valores variables de sensibilidad y especificidad (5,6) . Se conocen cuatro bandas de diagnóstico específicas (8, 12, 15 y 24kDa) en pacientes infectados con F. hepatica (6) .…”

Section: Introductionunclassified

Purificación de la fracción antigénica 27-28 KDA a partir del antígeno metabólico secretado excretado de Fasciola hepatica

Antitupa

Quispe

Mayo

et al. 2014

Rev Peru Med Exp Salud Publica

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Citar como: Antitupa I, Quispe W, Mayo J, Valverde F, Sanchez E. Purificación de la fracción antigénica 27-28 KDa a partir del antígeno metabólico secretadoexcretado de Fasciola hepatica. Rev Peru Med Exp Salud Publica. 2014;31(2) RESUMENEn el presente estudio, las fracciones antigénicas de 27-28 KDa de Fasciola hepatica fueron purificadas por cromatografía de exclusión molecular para su aplicación en el diagnóstico de la fascioliasis humana. Se obtuvieron antígenos de excreción y secreción a partir de fasciolas adultas vivas obtenida de hígado de ovino y bovino, y cultivados en medio mínimo esencial. La reactividad y eficacia del antígeno purificado fueron evaluadas por la prueba de inmunoblot empleando cuatro sueros con fascioliasis humana; cuatro sueros con otras parasitosis, y dos sueros negativos. Se concluye que las fracciones antigénicas purificadas no presentan reacción cruzada con otras parasitosis, por inmunoblot, por lo que se considera a las proteínas purificadas como potenciales candidatas a ser utilizadas para el diagnóstico de fascioliasis humana.Palabras clave: Fasciola hepatica; Purificación; Cromatografía (fuente: DeCS BIREME). PURIFICATION OF ANTIGENIC FRACTION 27-28 kDa from the metabolic ANTIGEN FROM METABOLIC secreted-excreted from Fasciola hepatica ABSTRACTAntigenic fractions of 27-28 kDa from Fasciola hepatica were purified by size-exclusion chromatography for use in the diagnosis of human fasciolosis. Excretion and secretion antigens were obtained from living adult flukes collected from sheep and cattle liver, and cultured in minimum essential medium. The reactivity of the purified antigen and efficacy were assessed by immunoblot test using four sera with human fascioliasis; four sera with other parasites, and two negative sera. We conclude that the purified antigenic fractions do not cross-react with other parasites by immunoblot. Therefore, purified proteins are considered as potential candidates to be used for the diagnosis of human fascioliasis.

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Evaluation of the diagnostic efficacy of Fasciola adult worm vomit for serodiagnosis of human fasciolosis

et al. 2013

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The diagnostic efficacy of Fasciola gigantica adult worm vomit (AWV) preparation in diagnosis of human fasciolosis was evaluated using conventional enzyme-linked immunosorbent assay (ELISA) and Falcon assay screening test (FAST)-ELISA in comparison with F. gigantica adult total soluble extract (TSE). Sera of fasciolosis patients, patients with other parasitic diseases (hydatid disease, schistosomiasis, toxoplasmosis, and amebiasis), and sera of healthy individuals were enrolled in this study. The results showed that the sensitivity of both conventional ELISA and FAST-ELISA was improved from 95 % using TSE to 100 % when using AWV. The specificity of conventional ELISA was 93.3 % using TSE and increased to 96.7 % using AWV. The specificity of FAST-ELISA using TSE was 96.7 % and became 100 % AWV antigen. The diagnostic accuracy of conventional ELISA was 94 % using TSE and increased to 98 % using AWV. The diagnostic accuracy of FAST-ELISA was 96 % using TSE and increased to 100 % using AWV. It is concluded that both TSE and AWV antigenic preparations are efficient for use in the serodiagnosis of human fasciolosis.

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Preliminary antigenic characterisation of an adult worm vomit preparation of Fasciola hepatica by infected human sera

Cited by 14 publications

References 26 publications

Detection of Fasciola hepatica and Fasciola gigantica common and uncommon antigens, using rabbit hyper immune serum raised against their excretory–secretory and somatic antigens

Detection of Fasciola hepatica and Fasciola gigantica common and uncommon antigens, using rabbit hyper immune serum raised against their excretory–secretory and somatic antigens

Purificación de la fracción antigénica 27-28 KDA a partir del antígeno metabólico secretado excretado de Fasciola hepatica

Evaluation of the diagnostic efficacy of Fasciola adult worm vomit for serodiagnosis of human fasciolosis

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