Gluconeogenesis is essential for trypanosome development in the tsetse fly vector

Marion Wargnies; Eloïse Bertiaux; Edern Cahoreau; Nicole Ziebart; Aline Crouzols; Pauline Morand; Marc Biran; Stefan Allmann; Jane Hubert; Oriana Villafraz; Yoann Millerioux; Nicolas Plazolles; Corinne Asencio; Loïc Rivière; Brice Rotureau; Michael Boshart; Jean-Charles Portais; Frédéric Bringaud

doi:10.1371/journal.ppat.1007502

Gluconeogenesis is essential for trypanosome development in the tsetse fly vector

PLoS Pathog. 2018 Dec 17;14(12):e1007502. doi: 10.1371/journal.ppat.1007502. eCollection 2018 Dec.

Authors

Marion Wargnies^{1

2}, Eloïse Bertiaux³, Edern Cahoreau⁴, Nicole Ziebart⁵, Aline Crouzols³, Pauline Morand², Marc Biran², Stefan Allmann^{1

5}, Jane Hubert⁴, Oriana Villafraz¹, Yoann Millerioux^{1

2}, Nicolas Plazolles¹, Corinne Asencio¹, Loïc Rivière¹, Brice Rotureau³, Michael Boshart⁵, Jean-Charles Portais⁴, Frédéric Bringaud^{1

2}

Affiliations

¹ Laboratoire de Microbiologie Fondamentale et Pathogénicité (MFP), Université de Bordeaux, CNRS UMR-5234, Bordeaux, France.
² Centre de Résonance Magnétique des Systèmes Biologiques (RMSB), Université de Bordeaux, CNRS UMR-5536, Bordeaux, France.
³ Trypanosome Transmission Group, Trypanosome Cell Biology Unit, Department of Parasites and Insect Vectors and INSERM U1201, Institut Pasteur, Paris, France.
⁴ LISBP, Université de Toulouse, CNRS, INRA, INSA, Toulouse, France.
⁵ Fakultät für Biologie, Genetik, Ludwig-Maximilians-Universität München, Martinsried, Germany.

Abstract

In the glucose-free environment that is the midgut of the tsetse fly vector, the procyclic form of Trypanosoma brucei primarily uses proline to feed its central carbon and energy metabolism. In these conditions, the parasite needs to produce glucose 6-phosphate (G6P) through gluconeogenesis from metabolism of non-glycolytic carbon source(s). We showed here that two phosphoenolpyruvate-producing enzymes, PEP carboxykinase (PEPCK) and pyruvate phosphate dikinase (PPDK) have a redundant function for the essential gluconeogenesis from proline. Indeed, incorporation of 13C-enriched proline into G6P was abolished in the PEPCK/PPDK null double mutant (Δppdk/Δpepck), but not in the single Δppdk and Δpepck mutant cell lines. The procyclic trypanosome also uses the glycerol conversion pathway to feed gluconeogenesis, since the death of the Δppdk/Δpepck double null mutant in glucose-free conditions is only observed after RNAi-mediated down-regulation of the expression of the glycerol kinase, the first enzyme of the glycerol conversion pathways. Deletion of the gene encoding fructose-1,6-bisphosphatase (Δfbpase), a key gluconeogenic enzyme irreversibly producing fructose 6-phosphate from fructose 1,6-bisphosphate, considerably reduced, but not abolished, incorporation of 13C-enriched proline into G6P. In addition, the Δfbpase cell line is viable in glucose-free conditions, suggesting that an alternative pathway can be used for G6P production in vitro. However, FBPase is essential in vivo, as shown by the incapacity of the Δfbpase null mutant to colonise the fly vector salivary glands, while the parental phenotype is restored in the Δfbpase rescued cell line re-expressing FBPase. The essential role of FBPase for the development of T. brucei in the tsetse was confirmed by taking advantage of an in vitro differentiation assay based on the RNA-binding protein 6 over-expression, in which the procyclic forms differentiate into epimastigote forms but not into mammalian-infective metacyclic parasites. In total, morphology, immunofluorescence and cytometry analyses showed that the differentiation of the epimastigote stages into the metacyclic forms is abolished in the Δfbpase mutant.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Disease Vectors
Gluconeogenesis / physiology*
Trypanosoma brucei brucei / metabolism*
Trypanosomiasis, African
Tsetse Flies / parasitology*

Grants and funding

The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript. FB's and BR's group were funded by the Agence Nationale de la Recherche (ANR) through GLYCONOV (grant number ANR-15-CE15-0025-01) of the ANR-BLANC-2015 call. FB's group was supported by the Centre National de la Recherche Scientifique (CNRS), the Université de Bordeaux, the ANR through the grants ACETOTRYP (grant number ANR-2010-BLAN-1319-02) of the ANR-BLANC-2010 call, the Laboratoire d’Excellence (LabEx) ParaFrap ANR-11-LABX-0024 and the ParaMet PhD programme of Marie Curie Initial Training Network. BR’s group was supported by the Institut Pasteur, the Institut National de la Santé et de la Recherche Médicale (INSERM). EB is funded by a doctoral fellowship from French National Ministry for Research and Technology (Doctoral School CDV515). MB was funded by the University of Munich and MB and FB were supported by a research cooperation grant of the Franco-Bavarian University Cooperation Center (BFHZ/CCUFB).