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Stability and suitability of housekeeping genes in phlebotomine sand flies
F. Sassù, B. Vomáčková Kykalová, CS. Vieira, P. Volf, E. Loza Telleria
Language English Country England, Great Britain
Document type Journal Article
Grant support
16_019/0000759
European Regional Development Fund
16_019/0000759
European Regional Development Fund
16_019/0000759
European Regional Development Fund
16_019/0000759
European Regional Development Fund
101067053
Marie Sklodowska-Curie Postdoctoral Fellowship, Horizon Europe 2021
731060
Infravec 2, Horizon Europe 2020
731060
Infravec 2, Horizon Europe 2020
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- MeSH
- Genes, Essential * MeSH
- Insect Vectors genetics MeSH
- Genes, Insect MeSH
- Larva genetics MeSH
- Leishmania genetics MeSH
- Phlebotomus * genetics MeSH
- Psychodidae genetics MeSH
- Gene Expression Profiling methods MeSH
- Animals MeSH
- Check Tag
- Male MeSH
- Female MeSH
- Animals MeSH
- Publication type
- Journal Article MeSH
We investigated gene expression patterns in Lutzomyia and Phlebotomus sand fly vectors of leishmaniases. Using quantitative PCR, we assessed the expression stability of potential endogenous control genes commonly used in dipterans. We analyzed Lutzomyia longipalpis and Phlebotomus papatasi samples from L3 and L4 larval stages, adult sand flies of different sexes, diets, dsRNA injection, and Leishmania infection. Six genes were evaluated: actin, α-tubulin, GAPDH, 60 S ribosomal proteins L8 and L32 (RiboL8 and RiboL32), and elongation factor 1-α (EF1-α). EF1-α was among the most stably expressed along with RiboL8 in L. longipalpis larvae and RiboL32 in adults. In P. papatasi, EF1-α and RiboL32 were the top in larvae, while EF1-α and actin were the most stable in adults. RiboL8 and actin were the most stable genes in dissected tissues and infected guts. Additionally, five primer pairs designed for L. longipalpis or P. papatasi were effective in PCR with Lutzomyia migonei, Phlebotomus duboscqi, Phlebotomus perniciosus, and Sergentomyia schwetzi cDNA. Furthermore, L. longipalpis RiboL32 and P. papatasi α-tubulin primers were suitable for qPCR with cDNA from the other four species. Our research provides tools to enhance relative gene expression studies in sand flies, facilitating the selection of endogenous control for qPCR.
References provided by Crossref.org
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