Transcriptome Profiling of Trypanosoma brucei Development in the Tsetse Fly Vector Glossina morsitans

Savage, Amy F.; Franklin, Joseph B.; Vigneron, Aurélien; Aksoy, Serap; Tschudi, Christian

doi:10.1371/journal.pone.0168877

Cited by 59 publications

(109 citation statements)

References 60 publications

(66 reference statements)

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“…biological replicas, were prepared from PF and MF cells and isolation of poly(A) 1 mRNA, library preparation and sequencing on an Illumina HiSeq4000 platform were performed at the Yale Center for Genome Analysis. The resulting reads of 75 nt in length were mapped to the T. brucei 11 megabase chromosomes (GeneDB version 5) using the Lasergene 13.1 software package from DNASTAR as described (Savage et al, 2016). Briefly, the SeqMan NGen layout algorithm by DNASTAR is based on a local match percentage and the match percentage threshold has to be met in each overlapping window of 50 bases.…”

Section: Rna Preparation Rna-seq Read Processing and Data Analysismentioning

confidence: 99%

“…Two different statistical methods were used for differential gene expression analysis: DESeq2 package version 1.16.1 (Love et al, 2014) and the Lasergene 13.1 software package from DNASTAR (Savage et al, 2016) with an excellent correlation of 0.97. For DESeq2 the quantified transcript read files were imported into Bioconductor (version 3.5), an open-source software project based on the R programming language (Gentleman et al, 2004).…”

Section: Rna Preparation Rna-seq Read Processing and Data Analysismentioning

confidence: 99%

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The proteome and transcriptome of the infectious metacyclic form of Trypanosoma brucei define quiescent cells primed for mammalian invasion

Christiano

Shi

Ullu

et al. 2017

Molecular Microbiology

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103

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Summary The infectious metacyclic forms of Trypanosoma brucei result from a complex development in the tsetse fly vector. When they infect mammals, they cause African sleeping sickness in humans. Due to scarcity of biological material and difficulties of the tsetse fly as an experimental system, very limited information is available concerning the gene expression profile of metacyclic forms. We used an in vitro system based on expressing the RNA binding protein 6 to obtain infectious metacyclics and determined their protein and mRNA repertoires by mass-spectrometry (MS) based proteomics and mRNA sequencing (RNA-Seq) in comparison to non-infectious procyclic trypanosomes. We showed that metacyclics are quiescent cells, and propose this influences the choice of a monocistronic variant surface glycoprotein expression site. Metacyclics have a largely bloodstream-form type transcriptome, and thus are programmed to translate a bloodstream-form type proteome upon entry into the mammalian host and resumption of cell division. Genes encoding cell surface components showed the largest changes between procyclics and metacyclics, observed at both the transcript and protein levels. Genes encoding metabolic enzymes exhibited expression in metacyclics with features of both procyclic and bloodstream forms, suggesting that this intermediate-type metabolism is dictated by the availability of nutrients in the tsetse fly vector.

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Section: Rna Preparation Rna-seq Read Processing and Data Analysismentioning

confidence: 99%

Section: Rna Preparation Rna-seq Read Processing and Data Analysismentioning

confidence: 99%

The proteome and transcriptome of the infectious metacyclic form of Trypanosoma brucei define quiescent cells primed for mammalian invasion

Christiano

Shi

Ullu

et al. 2017

Molecular Microbiology

Self Cite

103

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“…In contrast with other eukaryotes, T. brucei protein-coding genes can also be transcribed by RNA Pol I, including procyclin and VSG. DRIP-seq enrichment was notably greater in the VSG expression sites (ES) that are actively transcribed in BSF T. brucei compared with the procyclin loci or metacyclic VSG expression sites ( Fig.3A), from which gene expression is repressed in this life cycle stage (89). In addition, loss of TbRH1 caused a more pronounced increase in signal at the bloodstream VSG ES ( Fig.3A), perhaps suggesting R-loops predominantly form co-transcriptionally at RNA Pol I loci.…”

Section: R-loops Are Enriched At Repeated Sequences Including Centromentioning

confidence: 99%

Genome-wide mapping reveals conserved and diverged R-loop activities in the unusual genetic landscape of the African trypanosome genome

Briggs

Hamilton

Crouch

et al. 2018

Preprint

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R-loops are stable RNA-DNA hybrids that have been implicated in transcription initiation and termination, as well as in telomere homeostasis, chromatin formation, and genome replication and instability. RNA Polymerase (Pol) II transcription in the protozoan parasite Trypanosoma brucei is highly unusual: virtually all genes are co-transcribed from multigene transcription units, with mRNAs generated by linked transsplicing and polyadenylation, and transcription initiation sites display no conserved promoter motifs. Here, we describe the genome-wide distribution of R-loops in wild type mammal-infective T. brucei and in mutants lacking RNase H1, revealing both conserved and diverged functions. Conserved localisation was found at centromeres, rRNA genes and retrotransposon-associated genes. RNA Pol II transcription initiation sites also displayed R-loops, suggesting a broadly conserved role despite the lack of promoter conservation or transcription initiation regulation. However, the most abundant sites of R-loop enrichment were within the intergenic regions of the multigene transcription units, where the hybrids coincide with sites of polyadenylation and nucleosome-depletion. Thus, instead of functioning in transcription termination, most T. brucei R-loops act in a novel role, promoting RNA Pol II movement or mRNA processing. Finally, we show there is little evidence for correlation between R-loop localisation and mapped sites of DNA replication initiation.

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“…Stumpy forms are pre-adapted for development in the definitive host, the Tsetse fly, which becomes infected by blood feeding. Within the Tsetse midgut the parasites differentiate to procyclic forms, which have EP and GPEET procyclins on their surface (36) and a mitochondrial energy metabolism that depends on amino acid substrates (37)(38)(39). After a few weeks, with additional differentiation steps, mammalinfective parasites reappear in the salivary glands and can be transmitted at the next blood meal (40).…”

Section: Introductionmentioning

confidence: 99%

The suppressive cap-binding-complex factor 4EIP is required for normal differentiation

Clayton

Terrao

Marucha

et al. 2018

Preprint

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Summary/AbstractTrypanosoma brucei live in mammals as bloodstream forms and in the Tsetse midgut as procyclic forms. Differentiation from one form to the other proceeds via a growth-arrested stumpy form with low mRNA content and translation. The parasites have six eIF4Es and five eIF4Gs. EIF4E1 pairs with the mRNA-binding protein 4EIP but not with any EIF4G. EIF4E1 and 4EIP each inhibit expression when tethered to a reporter mRNA. The 4E-binding motif in 4EIP is required for the interaction with EIF4E1 both in vivo and in a 2-hybrid assay, but not for the suppressive activity of 4EIP when tethered. However, the suppressive activity of EIF4E1 when tethered requires 4EIP. Correspondingly, in growing bloodstream forms, 4EIP is preferentially associated with unstable mRNAs. Trypanosomes lacking 4EIP have a marginal growth disadvantage as cultured bloodstream or procyclic forms. Bloodstream forms without 4EIP cannot make differentiation-competent stumpy forms, but the defect can be complemented by a truncated 4EIP that does not interact with EIF4E1. Bloodstream forms lacking EIF4E1 have a growth defect but can differentiate. We suggest that 4EIP and EIF4E1 fine-tune mRNA levels in growing cells, and that 4EIP is required for mRNA suppression during differentiation to the stumpy form.

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Transcriptome Profiling of Trypanosoma brucei Development in the Tsetse Fly Vector Glossina morsitans

Cited by 59 publications

References 60 publications

The proteome and transcriptome of the infectious metacyclic form of Trypanosoma brucei define quiescent cells primed for mammalian invasion

The proteome and transcriptome of the infectious metacyclic form of Trypanosoma brucei define quiescent cells primed for mammalian invasion

Genome-wide mapping reveals conserved and diverged R-loop activities in the unusual genetic landscape of the African trypanosome genome

The suppressive cap-binding-complex factor 4EIP is required for normal differentiation

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