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An experimental target-based platform in yeast for screeningPlasmodium vivaxdeoxyhypusine synthase inhibitors

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ABSTRACTThe enzyme deoxyhypusine synthase (DHS) catalyzes the first step in the post-translational modification of the eukaryotic translation factor 5A (eIF5A). This is the only protein known to contain the amino acid hypusine, which results from this modification. Both eIF5A and DHS are essential for cell viability in eukaryotes, and inhibiting DHS can be a promising strategy for the development of new therapeutic alternatives. The human and parasitic orthologous proteins are different enough to render selective targeting against infectious diseases; however, no DHS inhibitor selective for the parasite ortholog has previously been reported. Here, we established a yeast surrogate genetics platform to identify inhibitors of DHS fromPlasmodium vivax,one of the major causative agents of malaria. We constructed genetically modifiedSaccharomyces cerevisiaestrains expressing DHS genes fromHomo sapiens(HsDHS) orP. vivax(PvDHS) in place of the endogenous DHS gene fromS. cerevisiae. This new strain background was ∼60-fold more sensitive to an inhibitor of human DHS than the one previously used. Initially, a virtual screen using datasets from the ChEMBL-NTD database was performed. Candidate ligands were tested in growth assays using the newly generated yeast strains expressing heterologous DHS genes. Among these, two showed promise by preferentially reducing the growth of the PvDHS-expressing strain. Further, in a robotized assay, we screened 400 compounds from the Pathogen Box library using the sameS. cerevisiaestrains, and one compound preferentially reduced the growth of the PvDHS-expressing yeast strain. Western blot revealed that these compounds significantly reduced eIF5A hypusination in yeast. Our study demonstrates that this yeast-based platform is suitable for identifying and verifying candidate small molecule DHS inhibitors, selective for the parasite over the human ortholog.
Title: An experimental target-based platform in yeast for screeningPlasmodium vivaxdeoxyhypusine synthase inhibitors
Description:
ABSTRACTThe enzyme deoxyhypusine synthase (DHS) catalyzes the first step in the post-translational modification of the eukaryotic translation factor 5A (eIF5A).
This is the only protein known to contain the amino acid hypusine, which results from this modification.
Both eIF5A and DHS are essential for cell viability in eukaryotes, and inhibiting DHS can be a promising strategy for the development of new therapeutic alternatives.
The human and parasitic orthologous proteins are different enough to render selective targeting against infectious diseases; however, no DHS inhibitor selective for the parasite ortholog has previously been reported.
Here, we established a yeast surrogate genetics platform to identify inhibitors of DHS fromPlasmodium vivax,one of the major causative agents of malaria.
We constructed genetically modifiedSaccharomyces cerevisiaestrains expressing DHS genes fromHomo sapiens(HsDHS) orP.
vivax(PvDHS) in place of the endogenous DHS gene fromS.
cerevisiae.
This new strain background was ∼60-fold more sensitive to an inhibitor of human DHS than the one previously used.
Initially, a virtual screen using datasets from the ChEMBL-NTD database was performed.
Candidate ligands were tested in growth assays using the newly generated yeast strains expressing heterologous DHS genes.
Among these, two showed promise by preferentially reducing the growth of the PvDHS-expressing strain.
Further, in a robotized assay, we screened 400 compounds from the Pathogen Box library using the sameS.
cerevisiaestrains, and one compound preferentially reduced the growth of the PvDHS-expressing yeast strain.
Western blot revealed that these compounds significantly reduced eIF5A hypusination in yeast.
Our study demonstrates that this yeast-based platform is suitable for identifying and verifying candidate small molecule DHS inhibitors, selective for the parasite over the human ortholog.

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