Abstract

African trypanosomiasis, also called African sleeping sickness, infects tens of thousands of individuals yearly in endemic areas, and is accompanied by continuing high social and economic cost. Existing treatments for trypanosomiasis are woefully inadequate, due both to the emergence of drug resistance that results in high treatment failures rates (30% in some areas), and high toxicity resulting in significant morbidity (10%) and drug-related mortality (5%). There thus remains an outstanding need for rational design of new trypanocidal therapies, particularly those that minimize host toxicity by targeting unique trypanosome biology. Glucose metabolism is the sole source of ATP for the infectious lifecycle stage of the African trypanosome, Trypanosoma brucei, and enzymes central to sugar metabolism are housed in the glycosome, an organelle not found in the parasite's mammalian host(s). Hence, both glycosome function and the control mechanisms governing enzyme activity inside the glycosome are important targets for drug design. We have demonstrated that ATP production in this organism is sensitive to environmentally-influenced changes in glycosomal solution conditions, including pH. Characterizing the intraglycosomal environment is therefore a necessary step in understanding essential glycolytic pathways, and would lay the groundwork for development of anti-trypanosome therapies that target control of glucose metabolism. However, this information is currently lacking at the most basic level. Neither pH nor glucose has been quantified inside the glycosome and their environmentally influenced dynamic range(s) are unknown, a paucity that reflects the historical lack of methodologies to allow quantitative intraglycosomal measurement. Here we propose development of peptide-targeted small molecule and recombinant protein-based sensors to quantitatively determine intraglycosomal pH and glucose levels. Our preliminary data indicates that such sensors can be delivered to the glycosomes of live parasites. Developed sensors can be subsequently modified for measurement of other glycosomal solutes, including ATP, and used to investigate control of glycolysis as a response to other potentially important environmental and developmental conditions, including glucose and divalent salt concentrations, nutrient depletion, and calcium signaling. Resulting findings will illuminate the mechanisms of dynamic regulation of the glycosomal environment, reveal conditions that influence the activity of this essential metabolic pathway, and introduce methodologies likely facilitate a series of new approaches to understanding and testing parasite metabolism. Notably, techniques pioneered in this study can be extended to analysis of other pathogenic kinetoplastid parasites, such as Trypanasoma cruzi and Leishmania spp. that also localize ATP production in glycosomes. In addition, the methodologies can be modified to evaluate the intraorganellar environment in other important subcellular compartments such as the mitochondria, endoplasmic reticulum, and Golgi apparatus. The work is therefore likely to have impact(s) beyond African trypanosomiasis.

Public Health Relevance

Glucose metabolism is the sole source of ATP for the infectious lifecycle stage of the African trypanosome, Trypanosoma brucei, and occurs exclusively in the glycosome. The proposed research would use both recombinant protein-based probes and peptide-bearing small molecule sensors to quantitatively observe intraglycosomal pH and glucose levels in live parasites, as a means to probe the mechanism of ATP production and reveal regulatory mechanisms suitable for therapeutic targeting of glucose metabolism. This work is a necessary first step in the design of mechanism-based therapeutics that target glycosomal pathways and is therefore relevant to NIH's mission to promote public health.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Exploratory/Developmental Grants (R21)
Project #
7R21AI105656-03
Application #
9077835
Study Section
Pathogenic Eukaryotes Study Section (PTHE)
Program Officer
Mcgugan, Glen C
Project Start
2013-12-12
Project End
2016-11-30
Budget Start
2015-08-01
Budget End
2016-11-30
Support Year
3
Fiscal Year
2015
Total Cost
$183,936
Indirect Cost
$32,102

  Institution

Name
Brigham Young University
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
009094012
City
Provo
State
UT
Country
United States
Zip Code
84602

  Publications

Voyton, Charles M; Morris, Meredith T; Ackroyd, P Christine et al. (2018) FRET Flow Cytometry-Based High Throughput Screening Assay To Identify Disrupters of Glucose Levels in Trypanosoma brucei. ACS Infect Dis 4:1058-1066
Voyton, Charles M; Qiu, Yijian; Morris, Meredith T et al. (2018) A FRET flow cytometry method for monitoring cytosolic and glycosomal glucose in living kinetoplastid parasites. PLoS Negl Trop Dis 12:e0006523
Gordhan, Heeren M; Milanes, Jillian E; Qiu, Yijian et al. (2017) A targeted delivery strategy for the development of potent trypanocides. Chem Commun (Camb) 53:8735-8738
Lin, Sheng; Voyton, Charles; Morris, Meredith T et al. (2017) pH regulation in glycosomes of procyclic form Trypanosoma brucei. J Biol Chem 292:7795-7805
Gordhan, Heeren M; Patrick, Stephen L; Swasy, Maria I et al. (2017) Evaluation of substituted ebselen derivatives as potential trypanocidal agents. Bioorg Med Chem Lett 27:537-541