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Rapid phenotypic and genotypic change in a laboratory schistosome population.

Kathrin S JutzelerRoy N PlattXue LiMadison MoralesRobbie DiazWinka LE Clec'hFrédéric D ChevalierTimothy J C Anderson
Published in: bioRxiv : the preprint server for biology (2024)
We were able to detect contamination in this case because SmBRE shows distinctive phenotypes. However, this would likely have been missed with phenotypically similar parasites. These results provide a cautionary tale about the importance of tracking the identity of parasite populations, but also showcase a simple approach to monitor changes within populations using molecular profiling of pooled population samples to characterize fixed single nucleotide polymorphisms. We also show that genetic drift results in continuous change even in the absence of contamination, causing parasites maintained in different labs (or sampled from the same lab at different times) to diverge.
Keyphrases
  • plasmodium falciparum
  • risk assessment
  • drinking water
  • health risk
  • human health
  • genome wide
  • single cell
  • single molecule
  • clinical trial
  • dna methylation
  • toxoplasma gondii
  • loop mediated isothermal amplification