4.5 Article

Homeostasis of extracellular ATP in uninfected RBCs from a Plasmodium falciparum culture and derived microparticles

Journal

BIOCHIMICA ET BIOPHYSICA ACTA-BIOMEMBRANES
Volume 1864, Issue 10, Pages -

Publisher

ELSEVIER
DOI: 10.1016/j.bbamem.2022.183980

Keywords

Red blood cells; Malaria; Extracellular ATP; Ectonucleotidases microparticles

Funding

  1. CONICET [PIP 112 20150100459]
  2. Universidad de Buenos Aires [PICT 2019-0905, A15S01]
  3. Agencia Nacional de Promocion de la Investigacion, el Desarrollo Tecnologico y la Innovacion [PICT 2018-0630, ANR-11-LABX-0051, ANR-11-LABX-005]
  4. Laboratory of Excellence GR-Ex [RGPIN-2016-05867]
  5. French National Research Agency
  6. Natural Sciences and Engineering Research Council of Canada (NSERC)
  7. [200201701001 52BA]
  8. [PDE 45 2020]

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The pathological processes of malaria patients are primarily due to metabolic and structural changes caused by Plasmodium falciparum, while uninfected RBCs and MPs play important roles in the regulation of extracellular ATP, activating ATP release and hydrolyzing eATP.
Plasmodium falciparum, a dangerous parasitic agent causing malaria, invades human red blood cells (RBCs), causing hemolysis and microvascular obstruction. These and other pathological processes of malaria patients are due to metabolic and structural changes occurring in uninfected RBCs. In addition, infection activates the pro-duction of microparticles (MPs). ATP and byproducts are important extracellular ligands modulating purinergic signaling within the intra-vascular space. Here, we analyzed the contribution of uninfected RBCs and MPs to the regulation of extracellular ATP (eATP) of RBCs, which depends on the balance between ATP release by specific transporters and eATP hydrolysis by ectonucleotidases. RBCs were cultured with P. falciparum for 24-48 h prior to experiments, from which uninfected RBCs and MPs were purified. On-line luminometry was used to quantify the kinetics of ATP release. Luminometry, colorimetry and radioactive methods were used to assess the rate of eATP hydrolysis by ectonucleotidases. Rates of ATP release and eATP hydrolysis were also evaluated in MPs. Uninfected RBCs challenged by different stimuli displayed a strong and transient activation of ATP release, together with an elevated rate of eATP hydrolysis. MPs contained ATP in their lumen, which was released upon vesicle rupture, and were able to hydrolyze eATP. Results suggest that uninfected RBCs and MPs can act as important determinants of eATP regulation of RBCs during malaria. The comparison of eATP homeostasis in infected RBCs, ui-RBCs, and MPs allowed us to speculate on the impact of P. falciparum infection on intravascular purinergic signaling and the control of the vascular caliber by RBCs.

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