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Parasite antigens in sera and urine of patients with bancroftian and brugian filariasis detected by sandwich ELISA with monoclonal antibodies.

Identifieur interne : 009897 ( Ncbi/Checkpoint ); précédent : 009896; suivant : 009898

Parasite antigens in sera and urine of patients with bancroftian and brugian filariasis detected by sandwich ELISA with monoclonal antibodies.

Auteurs : H J Zheng ; Z H Tao ; M V Reddy ; B C Harinath ; W F Piessens

Source :

RBID : pubmed:3555138

Descripteurs français

English descriptors

Abstract

We developed a sandwich enzyme-linked immunosorbent assay to detect circulating parasite antigens in human lymphatic filariasis. The assay utilizes a polyclonal rabbit antifilarial antiserum to capture, and a monoclonal antibody to identify, circulating parasite antigen. Using this assay, we found that greater than 95% of sera from microfilaremic donors with bancroftian or brugian filariasis, approximately 60% of sera from microfilaremic patients with hydroceles, chyluria, or elephantiasis, and 15%-20% of sera from asymptomatic residents of filariasis-endemic areas evidently contain filarial antigens. Antigen was also detected in the urine of some microfilaremic patients. Serum levels of antigen detected with one monoclonal antibody, ES34, correlated well with microfilarial density in night blood. In contrast, less than 5% of sera from residents of areas where lymphatic filariasis is not endemic reacted in the assay, even though approximately one-third of the donors whose sera were tested were known to be infected with intestinal nematodes. The assay was designed to be flexible enough to allow the parallel use of multiple monoclonal antibodies with different specificities and simple enough to be applicable in most areas where lymphatic filariasis is endemic.

PubMed: 3555138


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pubmed:3555138

Le document en format XML

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<term>Antigens, Helminth (analysis)</term>
<term>Antigens, Helminth (urine)</term>
<term>Brugia (immunology)</term>
<term>Elephantiasis, Filarial (immunology)</term>
<term>Enzyme-Linked Immunosorbent Assay</term>
<term>Microfilariae</term>
<term>Wuchereria (immunology)</term>
<term>Wuchereria bancrofti (immunology)</term>
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<term>Anticorps monoclonaux</term>
<term>Antigènes d'helminthe (analyse)</term>
<term>Antigènes d'helminthe (urine)</term>
<term>Brugia (immunologie)</term>
<term>Filariose lymphatique (immunologie)</term>
<term>Microfilaria</term>
<term>Test ELISA</term>
<term>Wuchereria (immunologie)</term>
<term>Wuchereria bancrofti (immunologie)</term>
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<term>Antigens, Helminth</term>
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<keywords scheme="MESH" type="chemical" qualifier="urine" xml:lang="en">
<term>Antigens, Helminth</term>
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<keywords scheme="MESH" type="chemical" xml:lang="en">
<term>Antibodies, Monoclonal</term>
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<term>Antigènes d'helminthe</term>
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<keywords scheme="MESH" qualifier="immunologie" xml:lang="fr">
<term>Brugia</term>
<term>Filariose lymphatique</term>
<term>Wuchereria</term>
<term>Wuchereria bancrofti</term>
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<keywords scheme="MESH" qualifier="immunology" xml:lang="en">
<term>Brugia</term>
<term>Elephantiasis, Filarial</term>
<term>Wuchereria</term>
<term>Wuchereria bancrofti</term>
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<div type="abstract" xml:lang="en">We developed a sandwich enzyme-linked immunosorbent assay to detect circulating parasite antigens in human lymphatic filariasis. The assay utilizes a polyclonal rabbit antifilarial antiserum to capture, and a monoclonal antibody to identify, circulating parasite antigen. Using this assay, we found that greater than 95% of sera from microfilaremic donors with bancroftian or brugian filariasis, approximately 60% of sera from microfilaremic patients with hydroceles, chyluria, or elephantiasis, and 15%-20% of sera from asymptomatic residents of filariasis-endemic areas evidently contain filarial antigens. Antigen was also detected in the urine of some microfilaremic patients. Serum levels of antigen detected with one monoclonal antibody, ES34, correlated well with microfilarial density in night blood. In contrast, less than 5% of sera from residents of areas where lymphatic filariasis is not endemic reacted in the assay, even though approximately one-third of the donors whose sera were tested were known to be infected with intestinal nematodes. The assay was designed to be flexible enough to allow the parallel use of multiple monoclonal antibodies with different specificities and simple enough to be applicable in most areas where lymphatic filariasis is endemic.</div>
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