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Large-scale entomological assessment of Wuchereria bancrofti transmission by dissection and PCR-ELISA in Gampaha district, Sri Lanka

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dc.contributor.author Wijegunawardana, N.D.A.D.
dc.contributor.author Gunawardene, Y.I.N.S. en
dc.contributor.author Manamperi, A. en
dc.contributor.author Hapuarachchi, H.A.C. en
dc.contributor.author Bandara, K.B.A.T. en
dc.contributor.author Abeyewickreme, W. en
dc.date.accessioned 2015-07-31T11:17:30Z
dc.date.available 2015-07-31T11:17:30Z
dc.date.issued 2008
dc.identifier.citation Proceedings of the Sri Lanka Association for the Advancement of Science. 2008; 64 (Part I): 9 en_US
dc.identifier.uri http://repository.kln.ac.lk/handle/123456789/9072
dc.description Sri Lanka Association for the Advancement of Science, 64th Annual Sessions Abstracts(009A), 1st-6th December 2008. Colombo. en_US
dc.description.abstract Entomological surveys are important tools for monitoring progress of lymphatic filariasis (Lf) eradication programs. In this study, dissection of Culex quinquefasciatus was compared with a Polymerase Chain Reaction - Enzyme Linked Immunosorbent Assay (PCR-ELISA) for pooled mosquitoes to assess filarial infection levels in the major vector of Wuchereria bancrofti in Gampaha district, following mass-treatment programme with diethylcarbamazine (DEC) and albendazole. Mosquitoes were collected in 30 sentinel and 15 non-sentinel sites in 15 Medical Officer of Health (MOH) areas of Gampaha district known for the presence of W. bancrofti transmission. Captured mosquitoes were dissected to determine the W. bancrofti larvae (L1, L2, L3). PCR was carried out using Deoxyribonucleic acid (DNA) extracted from mosquito pools (15 body parts/pool) utilizing primers specific for the Wb-SspI repeat. PCR products were analyzed by hybridization ELISA using fluorescein-labeled wild type specific probes. The prevalence of infected/infective mosquitoes in PCR pools (3pools/site) was estimated using the PoolScreenTM algorithm and a novel probability-based method. The prevalence of infected mosquitoes with L1-L2 larvae of W. bancrofti ranged from 0%-8.54% by dissection and point estimates of infection prevalence as assayed by PCR-ELISA, ranged from 0% - 25.4%. Mosquitoes collected from all MOH areas (80%, N = 12), except for Minuwangoda, Dompe and Ragama, were positive for W. bancrofti larvae, with a prevalence rate ranging from 0.78% to 16.97% in both methods. Of 30 sentinel sites, 43.3% (N = 13) were positive for W. bancrofti transmission whereas it was evident in 40% (N = 6) of non-sentinel sites. The proportion of positive pools detected by the PCR-ELISA assay was higher than that obtained by the dissection indicating that PCR-ELISA assay is more sensitive than the dissection method in detecting infected/infective mosquitoes. Also results of this study showed that autochthonous transmission of W. bancrofti continues in the Gampaha district despite completion of the 5 year mass drug administration (MDA) programme. Therefore, we emphasize the use of more sensitive tools such as PCR-ELISA to monitor the impact of the MDA programme on disease transmission. This study also emphasizes that control measures should be further continued until the microfilareamic population is reduced to a level which could interrupt transmission in the area. Financial assistance received from WHO/SEARO/TDR (grant no. SN 1152) and University of Kelaniya (Grant no. RP/03/04/06/01/2006) is acknowledged en_US
dc.language.iso en en_US
dc.publisher Sri Lanka Association for the Advancement of Science en_US
dc.subject Filariasis en_US
dc.subject Elephantiasis, Filarial en_US
dc.subject Wuchereria bancrofti en_US
dc.subject Polymerase Chain Reaction en_US
dc.subject Polymerase Chain Reaction-methods en_US
dc.subject Enzyme-Linked Immunosorbent Assay en_US
dc.subject Enzyme-Linked Immunosorbent Assay-methods en_US
dc.subject Elephantiasis, Filarial-diagnosis en_US
dc.title Large-scale entomological assessment of Wuchereria bancrofti transmission by dissection and PCR-ELISA in Gampaha district, Sri Lanka en_US
dc.type Conference Abstract en_US


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