Identification of clinically approved small molecules that inhibit growth and affect transcript levels of developmentally regulated genes in the African trypanosome

Walsh, Madison Elle; Naudzius, Eleanor Mary; Diaz, Savanah Jessica; Wismar, Theodore William; Shilman, Mikhail Martchenko; Schulz, Danae

doi:10.1371/journal.pntd.0007790

Cited by 8 publications

(15 citation statements)

References 66 publications

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“…As a licensed medicine, clemastine fumarate has proven pharmacokinetic exposure and the high volume of distribution (9.5 ± 3.8 L kg –1 ) could be contributing to the enhanced perfusion of parasite infected cells. As such, it is perhaps not surprising that clemastine fumarate has been identified in other repurposing studies for NTDs, − including those looking for new antileishmanial applications . However, significant antiparasitic activity has not been reported nor has a putative mode-of-action been identified.…”

Section: Discussionmentioning

confidence: 99%

Antileishmanial Chemotherapy through Clemastine Fumarate Mediated Inhibition of the Leishmania Inositol Phosphorylceramide Synthase

et al. 2020

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Current chemotherapeutics for leishmaniasis have multiple deficiencies, and there is a need for new safe, efficacious, and affordable medicines. This study describes a successful drug repurposing approach that identifies the over-the-counter antihistamine, clemastine fumarate, as a potential antileishmanial drug candidate. The screening for inhibitors of the sphingolipid synthase (inositol phosphorylceramide synthase, IPCS) afforded, following secondary screening against Leishmania major (Lmj) promastigotes, 16 active compounds. Further refinement through the dose response against LmjIPCS and intramacrophage L. major amastigotes identified clemastine fumarate with good activity and selectivity with respect to the host macrophage. On target engagement was supported by diminished sensitivity in a sphingolipid-deficient L. major mutant (ΔLmjLCB2) and altered phospholipid and sphingolipid profiles upon treatment with clemastine fumarate. The drug also induced an enhanced host cell response to infection indicative of polypharmacology. The activity was sustained across a panel of Old and New World Leishmania species, displaying an in vivo activity equivalent to the currently used drug, glucantime, in a mouse model of L. amazonensis infection. Overall, these data validate IPCS as an antileishmanial drug target and indicate that clemastine fumarate is a candidate for repurposing for the treatment of leishmaniasis.

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Section: Discussionmentioning

confidence: 99%

Antileishmanial Chemotherapy through Clemastine Fumarate Mediated Inhibition of the Leishmania Inositol Phosphorylceramide Synthase

et al. 2020

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“…Specifically, the EP genes that are downregulated and the BARP genes that are upregulated during the transition to the epimastigote stage do not show significantly altered transcript levels following I-BET151 treatment. We verified that procyclin expression was not altered in procyclic parasites following I-BET151 treatment using a previously validated EP1/GFP reporter parasite line 30 (Supplemental Figure 1). We observed no difference in EP1/GFP expression in I-BET151 treated parasites (Supplemental Figure 2).…”

Section: Resultsmentioning

confidence: 67%

“…In parasites, bromodomain inhibitors have been shown to bind to bromodomain proteins in T. brucei, T. cruzi, P. falciparum, and L. dovani 23,27,[41][42][43][44] . Inhibition of bromodomain proteins in parasites has been shown to affect differentiation processes in multiple parasite systems 23,45,46 , and therapeutic strategies targeting chromatin interacting proteins have also been proposed and/or demonstrated for trypanosomiasis 23,30 , Chagas disease [47][48][49] , schistosomiasis 50,51 , toxoplasmosis 52,53 , leishmaniasis 54 , and malaria 55,56 .…”

Section: Discussionmentioning

confidence: 99%

“…Parasites were treated with 20µM I-BET151 (Sigma-Aldrich). EP1/GFP procyclic reporter parasites were generated as described in 30 . EP1/GFP bloodstream parasites 30 and Single Marker (SM) parasites 77 (used as controls for verification of the EP1/GFP reporter construct) were grown in HMI9 supplemented with 10% FCS and 10% Serum Plus at 37 ºC and 5.0% CO 2 .…”

Section: Methodsmentioning

confidence: 99%

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Chemical inhibition of bromodomain proteins in insect stage African trypanosomes perturbs silencing of the Variant Surface Glycoprotein repertoire and results in widespread changes in the transcriptome

Ashby

Havens

Hardin

et al. 2023

Preprint

Self Cite

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The eukaryotic protozoan parasite Trypanosoma brucei, spp. is transmitted by the tsetse fly to both humans and animals, where it causes a fatal disease called African trypanosomiasis. While the parasite lacks canonical DNA sequence specific transcription factors, it does possess histones, histone modifications, and proteins that write, erase, and read histone marks. Chemical inhibition of chromatin interacting bromodomain proteins has previously been shown to perturb bloodstream specific trypanosome processes, including silencing of the Variant Surface Glycoprotein genes (VSGs) and immune evasion. Transcriptomic changes that occur in bromodomain inhibited bloodstream parasites mirror many of the changes that occur as parasites developmentally progress from the bloodstream to the insect stage. We performed RNA-seq timecourses to determine the effects of chemical bromodomain inhibition in insect stage parasites using the compound I-BET151. We found that treatment with I-BET151 causes large changes in the transcriptome of insect stage parasites, and also perturbs silencing of VSG genes. The transcriptomes of bromodomain inhibited parasites share some features with early metacyclic stage parasites in the fly salivary gland, implicating bromodomain proteins as important for regulating transcript levels for developmentally relevant genes. However, the downregulation of surface procyclin protein that typically accompanies developmental progression is absent in bromodomain inhibited insect stage parasites. We conclude that chemical modulation of bromodomain proteins causes widespread transcriptomic changes in multiple trypanosome life cycle stages. Understanding the gene regulatory processes that facilitate transcriptome remodeling in this highly diverged eukaryote may shed light on how these mechanisms evolved.

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“…The authors of that study showed that clemastine treatment reduces Plasmodium tubulin levels and inhibits replication. Clemastine also inhibits the kinetoplastid parasites Leishmania (amastigotes), Trypanosoma cruzi (amastigotes), and Trypanosoma brucei (bloodstream forms) with EC 50 values of 180 nM, 400 nM, and 3.7 µM, respectively [ 38 , 39 , 40 ]. The Leishmania study proposes inositol phosphoryl-ceramide synthase as the target: clemastine inhibits purified IPCS enzyme activity, with an IC 50 of 2.90 μM; parasites with an IPCS gene knockout have reduced drug sensitivity, and clemastine-treated amastigotes show altered lipid profiles [ 38 ].…”

Section: Discussionmentioning

confidence: 99%

Systematic Analysis of Clemastine, a Candidate Apicomplexan Parasite-Selective Tubulin-Targeting Agent

Abbaali

Truong

Day

et al. 2021

IJMS

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Apicomplexan parasites, such as Toxoplasma gondii, Plasmodium spp., Babesia spp., and Cryptosporidium spp., cause significant morbidity and mortality. Existing treatments are problematic due to toxicity and the emergence of drug-resistant parasites. Because protozoan tubulin can be selectively disrupted by small molecules to inhibit parasite growth, we assembled an in vitro testing cascade to fully delineate effects of candidate tubulin-targeting drugs on Toxoplasma gondii and vertebrate host cells. Using this analysis, we evaluated clemastine, an antihistamine that has been previously shown to inhibit Plasmodium growth by competitively binding to the CCT/TRiC tubulin chaperone as a proof-of-concept. We concurrently analyzed astemizole, a distinct antihistamine that blocks heme detoxification in Plasmodium. Both drugs have EC50 values of ~2 µM and do not demonstrate cytotoxicity or vertebrate microtubule disruption at this concentration. Parasite subpellicular microtubules are shortened by treatment with either clemastine or astemizole but not after treatment with pyrimethamine, indicating that this effect is not a general response to antiparasitic drugs. Immunoblot quantification indicates that the total α-tubulin concentration of 0.02 pg/tachyzoite does not change with clemastine treatment. In conclusion, the testing cascade allows profiling of small-molecule effects on both parasite and vertebrate cell viability and microtubule integrity.

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Identification of clinically approved small molecules that inhibit growth and affect transcript levels of developmentally regulated genes in the African trypanosome

Cited by 8 publications

References 66 publications

Antileishmanial Chemotherapy through Clemastine Fumarate Mediated Inhibition of the Leishmania Inositol Phosphorylceramide Synthase

Antileishmanial Chemotherapy through Clemastine Fumarate Mediated Inhibition of the Leishmania Inositol Phosphorylceramide Synthase

Chemical inhibition of bromodomain proteins in insect stage African trypanosomes perturbs silencing of the Variant Surface Glycoprotein repertoire and results in widespread changes in the transcriptome

Systematic Analysis of Clemastine, a Candidate Apicomplexan Parasite-Selective Tubulin-Targeting Agent

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