A high-throughput sequencing assay to comprehensively detect and characterize unicellular eukaryotes and helminths from biological and environmental samples

Abstract: BackgroundSeveral of the most devastating human diseases are caused by eukaryotic parasites transmitted by arthropod vectors or through food and water contamination. These pathogens only represent a fraction of all unicellular eukaryotes and helminths that are present in the environment and many uncharacterized organisms might have subtle but pervasive effects on health, including by modifying the microbiome where they reside. Unfortunately, while we have modern molecular tools to characterize bacterial and, t… Show more

“…DNA extracted from each mosquito was ampli ed using primers targeting bacterial 16S rRNA primers [32], mosquito kdr-west (L1014F) [33], cox1 and S200 × 6.1 [34] loci, mammalian mitochondrial 16S rRNA sequences, as well as eukaryotic parasite and virus primers [35] (Additional le 1: Table S1).…”

“…Only 35 cycles were used to amplify bacterial 16S rRNA. All PCR products generated from one DNA sample (i.e., individual mosquito) were pooled together and reampli ed in a second PCR to add a unique barcode and the Illumina sequencing adaptors [35]. Finally, all barcoded products from all mosquitoes were pooled and sequenced simultaneously on Illumina HiSeq 2500 to generate 300 bp paired-end reads [35].…”

“…Then all concatenated sequences ampli ed with the same primer pair (from all samples) were compared to each other and a single copy of each unique sequence was kept (while the number of times it is observed in each sample was recorded). Unique sequences that were observed less than 10 times across all samples were removed as they likely represent instances of sequences carrying errors [35]. The remaining unique sequences were compared against all DNA sequences annotated on the NCBI nr database using BLAST [35].…”

“…Unique sequences that were observed less than 10 times across all samples were removed as they likely represent instances of sequences carrying errors [35]. The remaining unique sequences were compared against all DNA sequences annotated on the NCBI nr database using BLAST [35]. We then retrieved the taxonomic information of the most similar sequence(s) if it had at least 70% identity over the entire sequence length.…”

“…Finally, we determined whether each mosquito carried a eukaryotic parasite and/or arbovirus using a sequencing-based assay recently developed in our laboratory [35]. After PCR ampli cation, and sequencing of DNA extracted from individual mosquitoes, we identi ed DNA sequences from eukaryotes and viruses from 127 mosquitoes, with on average, 1,876 reads supporting each identi cation in each mosquito.…”

Relative Contributions of Genetic and Non-Genetic Factors on Mosquito Microbiota

“…DNA extracted from each mosquito was ampli ed using primers targeting bacterial 16S rRNA primers [32], mosquito kdr-west (L1014F) [33], cox1 and S200 × 6.1 [34] loci, mammalian mitochondrial 16S rRNA sequences, as well as eukaryotic parasite and virus primers [35] (Additional le 1: Table S1).…”

“…Only 35 cycles were used to amplify bacterial 16S rRNA. All PCR products generated from one DNA sample (i.e., individual mosquito) were pooled together and reampli ed in a second PCR to add a unique barcode and the Illumina sequencing adaptors [35]. Finally, all barcoded products from all mosquitoes were pooled and sequenced simultaneously on Illumina HiSeq 2500 to generate 300 bp paired-end reads [35].…”

“…Then all concatenated sequences ampli ed with the same primer pair (from all samples) were compared to each other and a single copy of each unique sequence was kept (while the number of times it is observed in each sample was recorded). Unique sequences that were observed less than 10 times across all samples were removed as they likely represent instances of sequences carrying errors [35]. The remaining unique sequences were compared against all DNA sequences annotated on the NCBI nr database using BLAST [35].…”

“…Unique sequences that were observed less than 10 times across all samples were removed as they likely represent instances of sequences carrying errors [35]. The remaining unique sequences were compared against all DNA sequences annotated on the NCBI nr database using BLAST [35]. We then retrieved the taxonomic information of the most similar sequence(s) if it had at least 70% identity over the entire sequence length.…”

“…Finally, we determined whether each mosquito carried a eukaryotic parasite and/or arbovirus using a sequencing-based assay recently developed in our laboratory [35]. After PCR ampli cation, and sequencing of DNA extracted from individual mosquitoes, we identi ed DNA sequences from eukaryotes and viruses from 127 mosquitoes, with on average, 1,876 reads supporting each identi cation in each mosquito.…”

Relative Contributions of Genetic and Non-Genetic Factors on Mosquito Microbiota

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