PCR detection of malaria parasites in desiccated Anopheles mosquitoes is uninhibited by storage time and temperature

Authors

Mark A. Rider, Tulane University of Louisiana
Brian D. Byrd, Western Carolina University
Joseph Keating, Tulane University of Louisiana
Dawn M. Wesson, Tulane University of Louisiana
Kevin A. Caillouet, Virginia Commonwealth University

Document Type

Article

Original Publication Date

2012

Journal/Book/Conference Title

Malaria Journal

Volume

11

DOI of Original Publication

10.1186/1475-2875-11-193

Comments

Originally published at http://dx.doi.org/10.1186/1475-2875-11-193.

Date of Submission

August 2014

Abstract

Background

Reliable methods to preserve mosquito vectors for malaria studies are necessary for detectingPlasmodium parasites. In field settings, however, maintaining a cold chain of storage from the time of collection until laboratory processing, or accessing other reliable means of sample preservation is often logistically impractical or cost prohibitive. As the Plasmodium infection rate of Anophelesmosquitoes is a central component of the entomological inoculation rate and other indicators of transmission intensity, storage conditions that affect pathogen detection may bias malaria surveillance indicators. This study investigated the effect of storage time and temperature on the ability to detect Plasmodium parasites in desiccated Anophelesmosquitoes by real-time polymerase chain reaction (PCR).

Methods

Laboratory-infected Anopheles stephensi mosquitoes were chloroform-killed and stored over desiccant for 0, 1, 3, and 6 months while being held at four different temperatures: 28, 37, -20 and -80°C. The detection of Plasmodium DNA was evaluated by real-time PCR amplification of a 111 base pair region of block 4 of the merozoite surface protein.

Results

Varying the storage time and temperature of desiccated mosquitoes did not impact the sensitivity of parasite detection. A two-way factorial analysis of variance suggested that storage time and temperature were not associated with a loss in the ability to detect parasites. Storage of samples at 28°C resulted in a significant increase in the ability to detect parasite DNA, though no other positive associations were observed between the experimental storage treatments and PCR amplification.

Conclusions

Cold chain maintenance of desiccated mosquito samples is not necessary for real-time PCR detection of parasite DNA. Though field-collected mosquitoes may be subjected to variable conditions prior to molecular processing, the storage of samples over an inexpensive and logistically accessible desiccant will likely ensure accurate assessment of malaria parasite presence without diminishing PCR-detection of parasites in mosquitoes stored for at least six months.

Rights

© 2012 Rider et al.; licensee BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

Is Part Of

VCU Biostatistics Publications