BioTechniques (Mar 2004)

Dual-function stem molecular beacons to assess mRNA expression in AT-rich transcripts of Plasmodium falciparum

  • Leyla Y. Bustamante,
  • Almudena Crooke,
  • Joaquín Martínez,
  • Amalia Díez,
  • José M. Bautista

DOI
https://doi.org/10.2144/04363RN04
Journal volume & issue
Vol. 36, no. 3
pp. 488 – 494

Abstract

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The genome of the human malaria parasite Plasmodium falciparum is extremely AT-rich such that it is particularly difficult to design standard probes to identify and quantify specific transcripts. Biased AT genome contents (70%–80%) lead to a high proportion of short repetitions and a low free energy of binding between target sequences and their specific probes during hybridization. This causes nonspecific annealing and high background noise. We constructed molecular beacon probes with dual-function stems to avoid nonspecific detection and establish identical melting patterns for use with several fluorescent probes for the analysis of mRNA expression in P. falciparum in real-time reverse transcription PCR (RT-PCR) assays. The method proved highly efficient at detecting low transcript levels in P. falciparum microcultures. Conditions were established for two types of real-time instruments, demonstrating that molecular beacons with dual-function stems are a useful tool for the functional analysis of high AT genomes. The procedure could be adapted to high-throughput gene expression protocols for the biomolecular screening of the P. falciparum and other AT-rich genomes.