Hostname: page-component-586b7cd67f-rdxmf Total loading time: 0 Render date: 2024-11-27T21:32:07.184Z Has data issue: false hasContentIssue false

Detection of Onchocerca volvulus infection in Simulium ochraceum sensu lato: comparison of a PCR assay and fly dissection in a Mexican hypoendemic community

Published online by Cambridge University Press:  16 October 2009

M. A. RODRÍGUEZ-PÉREZ
Affiliation:
Centro de Investigaciones sobre Enfermedades Infecciosas, Instituto Nacional de Salud Pública, Cuernavaca 62508, México Department of Biological Sciences, University of Salford, Salford M5 4WT, UK
R. DANIS-LOZANO
Affiliation:
Centro de Investigación de Paludismo, Instituto Nacional de Salud Pública, Tapachula 30700, México
M. H. RODRÍGUEZ
Affiliation:
Centro de Investigaciones sobre Enfermedades Infecciosas, Instituto Nacional de Salud Pública, Cuernavaca 62508, México
T. R. UNNASCH
Affiliation:
Division of Geographic Medicine, University of Alabama at Birmingham, USA
J. E. BRADLEY
Affiliation:
Department of Biological Sciences, University of Salford, Salford M5 4WT, UK

Abstract

Detection of Onchocerca volvulus larvae in vector populations is of prime importance in the assessment of the effectiveness of onchocerciasis control programmes. Traditionally, detection of larvae is attained by the dissection of flies, but this time-consuming method cannot easily discriminate between species of Onchocerca. The genome of all Onchocerca species has a unique 150 bp repeat, which can be amplified by PCR, and O. volvulus-specific DNA probes can detect these products by Southern blot (SB). This study optimizes a PCR/SB assay, and compares it with fly dissection to estimate the prevalence (p) and intensity of infection (m) in the local vector population of a Mexican community that has become hypoendemic as a result of 7 years of treatment with ivermectin and nodulectomy. The PCR detected 1 infected fly in a pool of 99 uninfected flies, but the optimal pool size was 50 flies. At the community level, 1 out of 10550 flies was positive (p=0·0095%, 95% confidence intervals CI=0·00024–07·05280%; m=0·00027 larvae/parous fly, CI=−0·00026–0·00081) by PCR, and 4 out of 10772 flies (p=0·0371%, CI=0·01012–0.09505%; m=0·00107 larvae/parous fly, 95% CI=0·00002–0·00212) by dissection (observed m=0·0005). Both methods produce statistically similar estimates of the prevalence and intensity, indicating that pool screening is a viable alternative for entomological surveillance in areas where the intensity of transmission is becoming extremely low as a result of control interventions.

Type
Research Article
Copyright
© 1999 Cambridge University Press

Access options

Get access to the full version of this content by using one of the access options below. (Log in options will check for institutional or personal access. Content may require purchase if you do not have access.)