Methods and Protocols (May 2019)

Optimization of DNA Extraction from Individual Sand Flies for PCR Amplification

  • Lorena G. Caligiuri,
  • Adolfo E. Sandoval,
  • Jose C. Miranda,
  • Felipe A. Pessoa,
  • María S. Santini,
  • Oscar D. Salomón,
  • Nagila F. C. Secundino,
  • Christina B. McCarthy

DOI
https://doi.org/10.3390/mps2020036
Journal volume & issue
Vol. 2, no. 2
p. 36

Abstract

Read online

Numerous protocols have been published for extracting DNA from phlebotomines. Nevertheless, their small size is generally an issue in terms of yield, efficiency, and purity, for large-scale individual sand fly DNA extractions when using traditional methods. Even though this can be circumvented with commercial kits, these are generally cost-prohibitive for developing countries. We encountered these limitations when analyzing field-collected Lutzomyia spp. by polymerase chain reaction (PCR) and, for this reason, we evaluated various modifications on a previously published protocol, the most significant of which was a different lysis buffer that contained Ca2+ (buffer TESCa). This ion protects proteinase K against autolysis, increases its thermal stability, and could have a regulatory function for its substrate-binding site. Individual sand fly DNA extraction success was confirmed by amplification reactions using internal control primers that amplify a fragment of the cacophony gene. To the best of our knowledge, this is the first time a lysis buffer containing Ca2+ has been reported for the extraction of DNA from sand flies.

Keywords