Inhibition of Oxidative Phosphorylation Reverses Bone Marrow Hypoxia Visualized in Imageable Syngeneic B-ALL Mouse Model

Mateusz Rytelewski; Karine Harutyunyan; Natalia Baran; Saradhi Mallampati; M Anna Zal; Antonio Cavazos; Jason M Butler; Sergej Konoplev; Mirna El Khatib; Shane Plunkett; Joseph R Marszalek; Michael Andreeff; Tomasz Zal; Marina Konopleva

doi:10.3389/fonc.2020.00991

Inhibition of Oxidative Phosphorylation Reverses Bone Marrow Hypoxia Visualized in Imageable Syngeneic B-ALL Mouse Model

Front Oncol. 2020 Jun 30:10:991. doi: 10.3389/fonc.2020.00991. eCollection 2020.

Authors

Affiliations

¹ Department of Immunology, The University of Texas MD Anderson Cancer Center, Houston, TX, United States.
² Department of Leukemia, The University of Texas MD Anderson Cancer Center, Houston, TX, United States.
³ Translational Molecular Pathology, The University of Texas MD Anderson Cancer Center, Houston, TX, United States.
⁴ Weill Cornell Medicine, Medical School of Biological Sciences, Center for Discovery and Innovation, Hackensack University Medical Center, Nutley, NJ, United States.
⁵ Department of Hematopathology, The University of Texas MD Anderson Cancer Center, Houston, TX, United States.
⁶ Department of Biochemistry and Biophysics, The University of Pennsylvania, Philadelphia, PA, United States.
⁷ TRACTION, The University of Texas MD Anderson Cancer Center, Houston, TX, United States.

Abstract

Abnormally low level of interstitial oxygen, or hypoxia, is a hallmark of tumor microenvironment and a known promoter of cancer chemoresistance. Inside a solid tumor mass, the hypoxia stems largely from inadequate supply of oxygenated blood through sparse or misshapen tumor vasculature whilst oxygen utilization rates are low in typical tumor's glycolytic metabolism. In acute leukemias, however, markers of intracellular hypoxia such as increased pimonidazole adduct staining and HIF-1α stabilization are observed in advanced leukemic bone marrows (BM) despite an increase in BM vasculogenesis. We utilized intravital fast scanning two-photon phosphorescence lifetime imaging microscopy (FaST-PLIM) in a BCR-ABL B-ALL mouse model to image the extracellular oxygen concentrations (pO₂) in leukemic BM, and we related the extracellular oxygen levels to intracellular hypoxia, vascular markers and local leukemia burden. We observed a transient increase in BM pO₂ in initial disease stages with intermediate leukemia BM burden, which correlated with an expansion of blood-carrying vascular network in the BM. Yet, we also observed increased formation of intracellular pimonidazole adducts in leukemic BM at the same time. This intermediate stage was followed by a significant decrease of extracellular pO₂ and further increase of intracellular hypoxia as leukemia cellularity overwhelmed BM in disease end-stage. Remarkably, treatment of leukemic mice with IACS-010759, a pharmacological inhibitor of mitochondrial Complex I, substantially increased pO₂ in the BM with advanced B-ALL, and it alleviated intracellular hypoxia reported by pimonidazole staining. High rates of oxygen consumption by B-ALL cells were confirmed by Seahorse assay including in ex vivo cells. Our results suggest that B-ALL expansion in BM is associated with intense oxidative phosphorylation (OxPhos) leading to the onset of metabolic BM hypoxia despite increased BM vascularization. Targeting mitochondrial respiration may be a novel approach to counteract BM hypoxia in B-ALL and, possibly, tumor hypoxia in other OxPhos-reliant malignancies.

Keywords: acute lymphobastic leukemia; bone marrow; hypoxia; leukemia; oxidative phosphorylation; oxygen; vascularity.

Abstract

Grants and funding