Control of XPR1-dependent cellular phosphate efflux by InsP8 is an exemplar for functionally-exclusive inositol pyrophosphate signaling.
Xingyao Li,Chunfang Gu,Sarah Hostachy,Soumyadip Sahu,Christopher Wittwer,Henning J. Jessen,Dorothea Fiedler,Huanchen Wang,Stephen B. Shears +8 more
TL;DR: It is demonstrated that a major cellular phosphate export protein, XPR1, is regulated by the most “energetic” of cell signaling molecules—1,5-bisdiphosphoinositol 1,2,3,4-tetrakisphosphate (InsP8) and proposed that mutations in gene products that regulate InsP8 synthesis might compromise XPR 1 function, with pathological consequences for bone maintenance and ectopic calcification.
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Abstract: Homeostasis of cellular fluxes of inorganic phosphate (Pi) supervises its structural roles in bones and teeth, its pervasive regulation of cellular metabolism, and its functionalization of numerous organic compounds. Cellular Pi efflux is heavily reliant on Xenotropic and Polytropic Retrovirus Receptor 1 (XPR1), regulation of which is largely unknown. We demonstrate specificity of XPR1 regulation by a comparatively uncharacterized member of the inositol pyrophosphate (PP-InsP) signaling family: 1,5-bis-diphosphoinositol 2,3,4,6-tetrakisphosphate (InsP8). XPR1-mediated Pi efflux was inhibited by reducing cellular InsP8 synthesis, either genetically (knockout [KO] of diphosphoinositol pentakisphosphate kinases [PPIP5Ks] that synthesize InsP8) or pharmacologically [cell treatment with 2.5 µM dietary flavonoid or 10 µM N2-(m-trifluorobenzyl), N6-(p-nitrobenzyl) purine], to inhibit inositol hexakisphosphate kinases upstream of PPIP5Ks. Attenuated Pi efflux from PPIP5K KO cells was quantitatively phenocopied by KO of XPR1 itself. Moreover, Pi efflux from PPIP5K KO cells was rescued by restoration of InsP8 levels through transfection of wild-type PPIP5K1; transfection of kinase-dead PPIP5K1 was ineffective. Pi efflux was also rescued in a dose-dependent manner by liposomal delivery of a metabolically resistant methylene bisphosphonate (PCP) analog of InsP8; PCP analogs of other PP-InsP signaling molecules were ineffective. High-affinity binding of InsP8 to the XPR1 N-terminus (Kd = 180 nM) was demonstrated by isothermal titration calorimetry. To derive a cellular biology perspective, we studied biomineralization in the Soas-2 osteosarcoma cell line. KO of PPIP5Ks or XPR1 strongly reduced Pi efflux and accelerated differentiation to the mineralization end point. We propose that catalytically compromising PPIP5K mutations might extend an epistatic repertoire for XPR1 dysregulation, with pathological consequences for bone maintenance and ectopic calcification.
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Citations
Importance of Dietary Phosphorus for Bone Metabolism and Healthy Aging.
Juan Serna,Clemens Bergwitz +1 more
TL;DR: How dietary phosphorus is absorbed in the gut, current knowledge about Pi sensing, and endocrine regulation of Pi levels are examined to examine the roles of Pi in different tissues, the consequences of low and high dietary phosphorus in these tissues, and the implications for healthy aging.
108
Role of Inositols and Inositol Phosphates in Energy Metabolism.
Saimai Chatree,Nanthaphop Thongmaen,Kwanchanit Tantivejkul,Chantacha Sitticharoon,Ivana Vucenik +4 more
TL;DR: Evidence showed that inositol phosphates might enhance the browning of white adipocytes and directly improve insulin sensitivity through adipocytes, and inositl pyrophosphates containing high-energy phosphate bonds are considered in increasing cellular energetics.
108
Hormonal regulation of biomineralization.
Andrew Arnold,Elaine M. Dennison,Christopher S. Kovacs,Michael Mannstadt,René Rizzoli,Maria-Luisa Brandi,Bart L. Clarke,Rajesh V. Thakker +7 more
TL;DR: How developmental stresses in the fetus and neonate, and in the mother during pregnancy and lactation, invoke alternative hormonal regulatory pathways to control mineral delivery, skeletal metabolism and biomineralization is summarized.
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The social and structural architecture of the yeast protein interactome.
André C. Michaelis,Andreas D. Brunner,Maximilian Zwiebel,Florian Meier,Maximillian T. Strauss,Isabell Bludau,Matthias Mann +6 more
TL;DR: A protein interaction network constructed with data from high-throughput affinity enrichment coupled to mass spectrometry provides a highly saturated yeast interactome with 31,004 interactions, including low-abundance complexes, membrane protein complexes and non-taggable protein complexes.
49
Inositol Pyrophosphates: Signaling Molecules with Pleiotropic Actions in Mammals.
TL;DR: This review summarizes the current understanding of how PP-IPs control mammalian cellular signaling networks in physiology and disease.
47
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281
Mutations in XPR1 cause primary familial brain calcification associated with altered phosphate export
Andrea Legati,Donatella Giovannini,Gaël Nicolas,Uriel López-Sánchez,Beatriz Quintáns,João Ricardo Mendes de Oliveira,Renee L. Sears,Renee L. Sears,Eliana Marisa Ramos,Elizabeth Spiteri,María Jesús Sobrido,Angel Carracedo,Cristina Castro-Fernández,Stéphanie Cubizolle,Brent L. Fogel,Cyril Goizet,Joanna C. Jen,Suppachok Kirdlarp,Anthony E. Lang,Zosia Miedzybrodzka,Witoon Mitarnun,Martin Paucar,Henry L. Paulson,Jérémie Pariente,Anne Claire Richard,Naomi Salins,Sheila A Simpson,Pasquale Striano,Per Svenningsson,François Tison,Vivek K. Unni,Olivier Vanakker,Marja W. Wessels,Suppachok Wetchaphanphesat,Michele Yang,François Boller,Dominique Campion,Didier Hannequin,Marc Sitbon,Daniel H. Geschwind,Jean-Luc Battini,Giovanni Coppola +41 more
TL;DR: This work has identified in multiple families with PFBC mutations in XPR1, a gene encoding a retroviral receptor with phosphate export function that alters phosphate export, implicating X PR1 and phosphate homeostasis in PFBC.
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