AI Article Synopsis

  • The genus Fusarium has over 200 species, with 73 associated with human infections and classified as opportunistic pathogens.
  • Species identification is best achieved using a combination of molecular techniques involving specific protein-coding genes, as traditional methods like the internal transcribed spacers (ITS) may be limited in distinguishing closely related species.
  • Recent research highlights the effectiveness of new DNA barcode loci, TOP1 and PGK, alongside TEF1, in accurately analyzing 144 Fusarium strains from 52 species, confirming the validity of the phylogenetic relationships among recognized Fusarium species.

Article Abstract

The genus Fusarium includes more than 200 species of which 73 have been isolated from human infections. Fusarium species are opportunistic human pathogens with variable aetiology. Species determination is best made with the combined phylogeny of protein-coding genes such as elongation factor (TEF1), RNA polymerase (RPB2) and the partial β-tubulin (BT2) gene. The internal transcribed spacers 1, 2 and 5.8S rRNA gene (ITS) have also been used, however, ITS cannot discriminate several closely related species and has nonorthologous copies in Fusarium. Currently, morphological approaches and tree-building methods are in use to define species and to discover hitherto undescribed species. Aftter a species is defined, DNA barcoding approaches can be used to identify species by the presence or absence of discrete nucleotide characters. We demonstrate the potential of two recently discovered DNA barcode loci, topoisomerase I (TOP1) and phosphoglycerate kinase (PGK), in combination with other routinely used markers such as TEF1, in an analysis of 144 Fusarium strains belonging to 52 species. Our barcoding study using TOP1 and PKG provided concordance of molecular data with TEF1. The currently accepted Fusarium species sampled were well supported in phylogenetic trees of both new markers.

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Source
http://dx.doi.org/10.1016/j.funbio.2015.08.006DOI Listing

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