Profiling the bloodstream form and procyclic form Trypanosoma brucei cell cycle using single-cell transcriptomics

Briggs, Emma; Marques, Catarina A.; Oldrieve, Guy; Hu, Jihua; Otto, Thomas D.; Matthews, Keith R.

doi:10.7554/elife.86325

Cited by 8 publications

(5 citation statements)

References 115 publications

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“…After 24 to 72 h, parasites were moved to liquid nitrogen storage. For Chromium scRNA-seq (single cell RNA sequencing) (10× Genomics), samples were transported on dry ice before slow defrosting to limit cell death using the previously validated protocol ( 47 ). For each sample, parasites were combined from 2 to 3 mice in equal proportion depending on sample viability, only samples with >90% live, motile, parasites were used for sequencing.…”

Section: Methodsmentioning

confidence: 99%

The developmental hierarchy and scarcity of replicative slender trypanosomes in blood challenges their role in infection maintenance

Larcombe,

Briggs,

Savill

et al. 2023

Proc. Natl. Acad. Sci. U.S.A.

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The development of Trypanosoma brucei in its mammalian host is marked by a distinct morphological change as replicative “slender” forms differentiate into cell cycle arrested “stumpy” forms in a quorum-sensing-dependent manner. Although stumpy forms dominate chronic infections at the population level, the proportion of replicative parasites at the individual cell level and the irreversibility of arrest in the bloodstream are unclear. Here, we experimentally demonstrate that developmental cell cycle arrest is definitively irreversible in acute and chronic infections in mice. Furthermore, analysis of replicative capacity and single-cell transcriptome profiling reveal a temporal hierarchy, whereby cell cycle arrest and appearance of a reversible stumpy-like transcriptome precede irreversible commitment and morphological change. Unexpectedly, we show that proliferating parasites are exceptionally scarce in the blood after infections are established. This challenges the ability of bloodstream trypanosomes to sustain infection by proliferation or antigenic variation, these parasites instead being overwhelmingly adapted for transmission.

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Section: Methodsmentioning

confidence: 99%

The developmental hierarchy and scarcity of replicative slender trypanosomes in blood challenges their role in infection maintenance

Larcombe,

Briggs,

Savill

et al. 2023

Proc. Natl. Acad. Sci. U.S.A.

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“…Nonetheless, programming of DNA replication to predominantly initiate from a single origin or locus per chromosome would explain the chromosome size-dependent timing of L. major DNA replication we describe here and previously 82 . As we have argued 70, 81, 141, 142 , it is unlikely that whole genome duplication in Leishmania can be accomplished during S-phase using a single origin per chromosome, and so DNA replication may be supported by further, less efficient initiation activities. Such organisation could then explain Leishmania DNA replication timing, feeding into the other genome features we describe.…”

Section: Discussionmentioning

confidence: 92%

R-loops acted on by RNase H1 are a determinant of chromosome length-associated DNA replication timing and genome stability inLeishmania

Damasceno,

Briggs,

Krasilnikova

et al. 2024

Preprint

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Genomes in eukaryotes normally undergo DNA replication in a choreographed temporal order, resulting in early and late replicating chromosome compartments. Leishmania, a human protozoan parasite, displays an unconventional DNA replication program in which the timing of DNA replication completion is chromosome size-dependent: larger chromosomes complete replication later then smaller ones. Here we show that both R-loops and RNase H1, a ribonuclease that resolves RNA-DNA hybrids, accumulate in Leishmania major chromosomes in a pattern that reflects their replication timing. Furthermore, we demonstrate that such differential organisation of R-loops, RNase H1 and DNA replication timing across the parasite chromosomes correlates with size-dependent differences in chromatin accessibility, G quadruplex distribution and sequence content. Using conditional gene excision, we show that loss of RNase H1 leads to transient growth perturbation and permanently abrogates the differences in DNA replication timing across chromosomes, as well as altering levels of aneuploidy and increasing chromosome instability in a size-dependent manner. This work provides a link between R-loop homeostasis and DNA replication timing in a eukaryotic parasite and demonstrates that orchestration of DNA replication dictates levels of genome plasticity in Leishmania.

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“…To further investigate whether SUMO chain mutants are primed for differentiation to stumpy forms, we challenged the parasites with high concentrations of cis -aconitate (CA) at low temperature to stimulate differentiation to PF, which is thought to occur via a stumpy-like intermediate stage [ 23 , 24 ]. During this transformation, the VSG coat is released and replaced by a different coat consisting of invariant GPEET and EP procyclins.…”

Section: Resultsmentioning

confidence: 99%

Depolymerization of SUMO chains induces slender to stumpy differentiation in T. brucei bloodstream parasites

Iribarren,

Di Marzio,

Berazategui

et al. 2024

PLoS Pathog

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Trypanosoma brucei are protozoan parasites that cause sleeping sickness in humans and nagana in cattle. Inside the mammalian host, a quorum sensing-like mechanism coordinates its differentiation from a slender replicative form into a quiescent stumpy form, limiting growth and activating metabolic pathways that are beneficial to the parasite in the insect host. The post-translational modification of proteins with the Small Ubiquitin-like MOdifier (SUMO) enables dynamic regulation of cellular metabolism. SUMO can be conjugated to its targets as a monomer but can also form oligomeric chains. Here, we have investigated the role of SUMO chains in T. brucei by abolishing the ability of SUMO to polymerize. We have found that parasites able to conjugate only SUMO monomers are primed for differentiation. This was demonstrated for monomorphic lines that are normally unable to produce stumpy forms in response to quorum sensing signaling in mice, and also for pleomorphic cell lines in which stumpy cells were observed at unusually low parasitemia levels. SUMO chain mutants showed a stumpy compatible transcriptional profile and better competence to differentiate into procyclics. Our study indicates that SUMO depolymerization may represent a coordinated signal triggered during stumpy activation program.

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Profiling the bloodstream form and procyclic form Trypanosoma brucei cell cycle using single-cell transcriptomics

Cited by 8 publications

References 115 publications

The developmental hierarchy and scarcity of replicative slender trypanosomes in blood challenges their role in infection maintenance

The developmental hierarchy and scarcity of replicative slender trypanosomes in blood challenges their role in infection maintenance

R-loops acted on by RNase H1 are a determinant of chromosome length-associated DNA replication timing and genome stability inLeishmania

Depolymerization of SUMO chains induces slender to stumpy differentiation in T. brucei bloodstream parasites

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