Your search keyword '"Adrian Benito"' showing total 12 results

1. Indisulam targets RNA splicing and metabolism to serve as a therapeutic strategy for high-risk neuroblastoma

Author

Anke Nijhuis, Arti Sikka, Orli Yogev, Lili Herendi, Cristina Balcells, Yurui Ma, Evon Poon, Clare Eckold, Gabriel N. Valbuena, Yuewei Xu, Yusong Liu, Barbara Martins da Costa, Michael Gruet, Chiharu Wickremesinghe, Adrian Benito, Holger Kramer, Alex Montoya, David Carling, Elizabeth J. Want, Yann Jamin, Louis Chesler, and Hector C. Keun

Subjects

Science

Abstract

The prognosis of high-risk neuroblastoma is poor despite the availability of multimodal treatment. Here the authors show that high-risk neuroblastoma is sensitive to indisulam, a selective degrader of the splicing factor RBM39 through the dual targeting of RNA splicing and metabolism.

Published

2022

2. Glutamine Modulates Expression and Function of Glucose 6-Phosphate Dehydrogenase via NRF2 in Colon Cancer Cells

Author

Ibrahim H. Polat, Míriam Tarrado-Castellarnau, Adrian Benito, Claudia Hernandez-Carro, Josep Centelles, Silvia Marin, and Marta Cascante

Subjects

cancer cell metabolism, glucose-6-phosphate dehydrogenase, pentose phosphate pathway, colon cancer, oxidative stress, Therapeutics. Pharmacology, RM1-950

Abstract

Nucleotide pools need to be constantly replenished in cancer cells to support cell proliferation. The synthesis of nucleotides requires glutamine and 5-phosphoribosyl-1-pyrophosphate produced from ribose-5-phosphate via the oxidative branch of the pentose phosphate pathway (ox-PPP). Both PPP and glutamine also play a key role in maintaining the redox status of cancer cells. Enhanced glutamine metabolism and increased glucose 6-phosphate dehydrogenase (G6PD) expression have been related to a malignant phenotype in tumors. However, the association between G6PD overexpression and glutamine consumption in cancer cell proliferation is still incompletely understood. In this study, we demonstrated that both inhibition of G6PD and glutamine deprivation decrease the proliferation of colon cancer cells and induce cell cycle arrest and apoptosis. Moreover, we unveiled that glutamine deprivation induce an increase of G6PD expression that is mediated through the activation of the nuclear factor (erythroid-derived 2)-like 2 (NRF2). This crosstalk between G6PD and glutamine points out the potential of combined therapies targeting oxidative PPP enzymes and glutamine catabolism to combat colon cancer.

Published

2021

3. Oxidative Pentose Phosphate Pathway Enzyme 6-Phosphogluconate Dehydrogenase Plays a Key Role in Breast Cancer Metabolism

Author

Ibrahim H. Polat, Míriam Tarrado-Castellarnau, Rohit Bharat, Jordi Perarnau, Adrian Benito, Roldán Cortés, Philippe Sabatier, and Marta Cascante

Subjects

breast cancer, pentose phosphate pathway, cancer metabolism, 6PGD, Biology (General), QH301-705.5

Abstract

The pentose phosphate pathway (PPP) plays an essential role in the metabolism of breast cancer cells for the management of oxidative stress and the synthesis of nucleotides. 6-phosphogluconate dehydrogenase (6PGD) is one of the key enzymes of the oxidative branch of PPP and is involved in nucleotide biosynthesis and redox maintenance status. Here, we aimed to analyze the functional importance of 6PGD in a breast cancer cell model. Inhibition of 6PGD in MCF7 reduced cell proliferation and showed a significant decrease in glucose consumption and an increase in glutamine consumption, resulting in an important alteration in the metabolism of these cells. No difference in reactive oxygen species (ROS) production levels was observed after 6PGD inhibition, indicating that 6PGD, in contrast to glucose 6-phosphate dehydrogenase, is not involved in redox balance. We found that 6PGD inhibition also altered the stem cell characteristics and mammosphere formation capabilities of MCF7 cells, opening new avenues to prevent cancer recurrance after surgery or chemotherapy. Moreover, inhibition of 6PGD via chemical inhibitor S3 resulted in an induction of senescence, which, together with the cell cycle arrest and apoptosis induction, might be orchestrated by p53 activation. Therefore, we postulate 6PGD as a novel therapeutic target to treat breast cancer.

Published

2021

4. β-Hydroxybutyrate Oxidation Promotes the Accumulation of Immunometabolites in Activated Microglia Cells

Author

Adrian Benito, Nabil Hajji, Kevin O’Neill, Hector C. Keun, and Nelofer Syed

Subjects

microglia, β-hydroxybutyrate, metabolic reprogramming, stable-isotope tracing, metabolomics, Microbiology, QR1-502

Abstract

Metabolic regulation of immune cells has arisen as a critical set of processes required for appropriate response to immunological signals. While our knowledge in this area has rapidly expanded in leukocytes, much less is known about the metabolic regulation of brain-resident microglia. In particular, the role of alternative nutrients to glucose remains poorly understood. Here, we use stable-isotope (13C) tracing strategies and metabolomics to characterize the oxidative metabolism of β-hydroxybutyrate (BHB) in human (HMC3) and murine (BV2) microglia cells and the interplay with glucose in resting and LPS-activated BV2 cells. We found that BHB is imported and oxidised in the TCA cycle in both cell lines with a subsequent increase in the cytosolic NADH:NAD+ ratio. In BV2 cells, stimulation with LPS upregulated the glycolytic flux, increased the cytosolic NADH:NAD+ ratio and promoted the accumulation of the glycolytic intermediate dihydroxyacetone phosphate (DHAP). The addition of BHB enhanced LPS-induced accumulation of DHAP and promoted glucose-derived lactate export. BHB also synergistically increased LPS-induced accumulation of succinate and other key immunometabolites, such as α-ketoglutarate and fumarate generated by the TCA cycle. Finally, BHB upregulated the expression of a key pro-inflammatory (M1 polarisation) marker gene, NOS2, in BV2 cells activated with LPS. In conclusion, we identify BHB as a potentially immunomodulatory metabolic substrate for microglia that promotes metabolic reprogramming during pro-inflammatory response.

Published

2020

5. Efecto De Diferentes Concentraciones De Fructosa Sobre La Producción De Celulosa Bacteriana En Cultivo Estático

Author

Ruben Jaramillo, Olga Perna, Adrian Benito Revollo, Carlos Arrieta, and Edgardo Escamilla

Subjects

celulosa bacteriana, fructosa, Gluconacetobacter xylinus IFO, cultivo estático., Agriculture, Agriculture (General), S1-972, Animal culture, SF1-1100

Abstract

En la síntesis de celulosa bacteriana se han usado diversas fuentes de carbono, distintas configuraciones de biorreactores y estrategias de cultivo. En este estudio se compara la producción de celulosa bacteriana evaluando el efecto de diferentes concentraciones de fructosa en la producción de celulosa bacteriana (CB) por Gluconacetobacter xylinus IFO en un cultivo estático. El estudio se llevó a cabo en biorreactores cilíndricos de 750 ml, con 200 ml de medio que contenían concentraciones iniciales de 1, 5, 10, 15 % p/v de fructosa a pH 5,6. El volumen del inoculo fue el 10% v/v del volumen de medio de cultivo. La síntesis de celulosa se realizó a temperatura ambiente y a distintos tiempos de incubación que iban de 1,5 hasta 28 días, tiempo en el que se determinaron propiedades fisicoquímicas y mecánicas de la celulosa bacteriana, así como también el consumo de fructosa en función del tiempo para las diferentes concentraciones iniciales de fructosa. Los resultados indican que al 10% p/v de fructosa se obtiene el valor mas alto para la síntesis de CB en gramos de celulosa húmeda por litro de medio de cultivo y se obtuvo el máximo grosor con una disminución del volumen remanente de cultivo; además, se observó un consumo de fructosa hasta de un 90% de la concentración inicial. La comprensibilidad fue menor a un mayor grosor de la película de celulosa. El pH del medio se mantuvo en una región óptima para la síntesis de la CB.

Published

2013

6. Oxidative Pentose Phosphate Pathway Enzyme 6-Phosphogluconate Dehydrogenase Plays a Key Role in Breast Cancer Metabolism

Author

Adrian Benito, Jordi Perarnau, Marta Cascante, Ibrahim H. Polat, Philippe Sabatier, Roldán Cortés, Míriam Tarrado-Castellarnau, and Rohit Bharat

Subjects

pentose phosphate pathway, cancer metabolism, Oxidative phosphorylation, Pentose phosphate pathway, Biology, medicine.disease_cause, Cicle de la pentosa-fosfat, Article, General Biochemistry, Genetics and Molecular Biology, Càncer de mama, Breast cancer, breast cancer, medicine, lcsh:QH301-705.5, General Immunology and Microbiology, Cell growth, Cancer, Metabolism, Cell cycle, 6PGD, medicine.disease, Cell biology, Glutamine, lcsh:Biology (General), General Agricultural and Biological Sciences, Oxidative stress

Abstract

Simple Summary Cancer cells alter their metabolism to maintain their high need for energy, produce enough macromolecules for biosynthesis, and preserve their redox status. The investigation of cancer cell-specific metabolic alterations has vital importance to identify targets to be exploited for therapeutic development. The pentose phosphate pathway (PPP) is often highly activated in tumor cells to maintain redox level, as this pathway takes an important role in reactive oxygen species detoxification. PPP also yields ribose-5-phosphate, a five-carbon sugar essential for synthesizing nucleotides necessary for DNA replication and cell proliferation. In this study, we inhibited one of the key enzymes of this biochemical pathway and observed the main functions of this enzyme in breast cancer cells. We have demonstrated that inhibition of this enzyme reduces cell proliferation and leads to cell cycle arrest and apoptosis. Besides that, we showed that the inhibition of this enzyme causes an alteration in cellular metabolism. All these findings indicate that targeting this enzyme with specific pharmacological inhibitors is an effective strategy in fighting cancer. Abstract The pentose phosphate pathway (PPP) plays an essential role in the metabolism of breast cancer cells for the management of oxidative stress and the synthesis of nucleotides. 6-phosphogluconate dehydrogenase (6PGD) is one of the key enzymes of the oxidative branch of PPP and is involved in nucleotide biosynthesis and redox maintenance status. Here, we aimed to analyze the functional importance of 6PGD in a breast cancer cell model. Inhibition of 6PGD in MCF7 reduced cell proliferation and showed a significant decrease in glucose consumption and an increase in glutamine consumption, resulting in an important alteration in the metabolism of these cells. No difference in reactive oxygen species (ROS) production levels was observed after 6PGD inhibition, indicating that 6PGD, in contrast to glucose 6-phosphate dehydrogenase, is not involved in redox balance. We found that 6PGD inhibition also altered the stem cell characteristics and mammosphere formation capabilities of MCF7 cells, opening new avenues to prevent cancer recurrance after surgery or chemotherapy. Moreover, inhibition of 6PGD via chemical inhibitor S3 resulted in an induction of senescence, which, together with the cell cycle arrest and apoptosis induction, might be orchestrated by p53 activation. Therefore, we postulate 6PGD as a novel therapeutic target to treat breast cancer.

Published

2021

7. β-Hydroxybutyrate Oxidation Promotes the Accumulation of Immunometabolites in Activated Microglia Cells

Author

Hector C. Keun, Nabil Hajji, Nelofer Syed, Adrian Benito, and Kevin O’Neill

Subjects

0301 basic medicine, Endocrinology, Diabetes and Metabolism, lcsh:QR1-502, microglia, 0601 Biochemistry and Cell Biology, Biochemistry, lcsh:Microbiology, Article, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, β-hydroxybutyrate, DHAP, medicine, metabolic reprogramming, Glycolysis, Molecular Biology, Dihydroxyacetone phosphate, Microglia, 1103 Clinical Sciences, metabolomics, Cell biology, Citric acid cycle, Cytosol, 030104 developmental biology, medicine.anatomical_structure, chemistry, stable-isotope tracing, NAD+ kinase, 0301 Analytical Chemistry, Flux (metabolism), 030217 neurology & neurosurgery

Abstract

Metabolic regulation of immune cells has arisen as a critical set of processes required for appropriate response to immunological signals. While our knowledge in this area has rapidly expanded in leukocytes, much less is known about the metabolic regulation of brain-resident microglia. In particular, the role of alternative nutrients to glucose remains poorly understood. Here, we use stable-isotope (13C) tracing strategies and metabolomics to characterize the oxidative metabolism of &beta, hydroxybutyrate (BHB) in human (HMC3) and murine (BV2) microglia cells and the interplay with glucose in resting and LPS-activated BV2 cells. We found that BHB is imported and oxidised in the TCA cycle in both cell lines with a subsequent increase in the cytosolic NADH:NAD+ ratio. In BV2 cells, stimulation with LPS upregulated the glycolytic flux, increased the cytosolic NADH:NAD+ ratio and promoted the accumulation of the glycolytic intermediate dihydroxyacetone phosphate (DHAP). The addition of BHB enhanced LPS-induced accumulation of DHAP and promoted glucose-derived lactate export. BHB also synergistically increased LPS-induced accumulation of succinate and other key immunometabolites, such as &alpha, ketoglutarate and fumarate generated by the TCA cycle. Finally, BHB upregulated the expression of a key pro-inflammatory (M1 polarisation) marker gene, NOS2, in BV2 cells activated with LPS. In conclusion, we identify BHB as a potentially immunomodulatory metabolic substrate for microglia that promotes metabolic reprogramming during pro-inflammatory response.

Published

2020

8. Tracing Nutrient Flux Following Monocarboxylate Transporter-1 Inhibition with AZD3965

Author

Adrian Benito, Eyal Gottlieb, Chris P. Barnes, Francesco Mauri, Kathrin Heinzmann, Gabriel N. Valbuena, Hector C. Keun, John Latigo, Maciej Kaliszczak, Laurence Carroll, Stephen M. Stribbling, Alice Beckley, Marta Braga, Gillian M. Mackay, Zachary T. Schug, Nicoleta Baxan, Eric O. Aboagye, and Cancer Research UK

Subjects

0301 basic medicine, Cancer Research, medicine.medical_specialty, diffuse large B-cell lymphoma, cancer metabolism, Nod, lcsh:RC254-282, Article, 03 medical and health sciences, 0302 clinical medicine, In vivo, Internal medicine, AZD3965, medicine, Glycolysis, 1112 Oncology and Carcinogenesis, positron emission tomography (PET), Fluorodeoxyglucose, lactate, biology, Chemistry, monocarboxylate transporter 1, Metabolism, glycolysis, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, metabolic flux, In vitro, Citric acid cycle, 030104 developmental biology, Endocrinology, Monocarboxylate transporter 1, Oncology, 030220 oncology & carcinogenesis, biology.protein, medicine.drug

Abstract

The monocarboxylate transporter 1 (MCT1) is a key element in tumor cell metabolism and inhibition of MCT1 with AZD3965 is undergoing clinical trials. We aimed to investigate nutrient fluxes associated with MCT1 inhibition by AZD3965 to identify possible biomarkers of drug action. We synthesized an 18F-labeled lactate analogue, [18F]-S-fluorolactate ([18F]-S-FL), that was used alongside [18F]fluorodeoxyglucose ([18F]FDG), and 13C-labeled glucose and lactate, to investigate the modulation of metabolism with AZD3965 in diffuse large B-cell lymphoma models in NOD/SCID mice. Comparative analysis of glucose and lactate-based probes showed a preference for glycolytic metabolism in vitro, whereas in vivo, both glucose and lactate were used as metabolic fuel. While intratumoral L-[1-13C]lactate and [18F]-S-FL were unchanged or lower at early (5 or 30 min) timepoints, these variables were higher compared to vehicle controls at 4 h following treatment with AZD3965, which indicates that inhibition of MCT1-mediated lactate import is reversed over time. Nonetheless, AZD3965 treatment impaired DLBCL tumor growth in mice. This was hypothesized to be a consequence of metabolic strain, as AZD3965 treatment showed a reduction in glycolytic intermediates and inhibition of the TCA cycle likely due to downregulated PDH activity. Glucose ([18F]FDG and D-[13C6]glucose) and lactate-based probes ([18F]-S-FL and L-[1-13C]lactate) can be successfully used as biomarkers for AZD3965 treatment.

Published

2020

9. Glucose-6-phosphate dehydrogenase and transketolase modulate breast cancer cell metabolic reprogramming and correlate with poor patient outcome

Author

Adrian Benito, Ibrahim H. Polat, Marta Cascante, Silvia Marin, Carlos J. Ciudad, and Véronique Noé

Subjects

0301 basic medicine, Cancer cells, pentose phosphate pathway, Oxidative phosphorylation, Pentose phosphate pathway, Transketolase, Biology, Metabolisme cel·lular, Càncer de mama, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Breast cancer, breast cancer, Glucose-6-phosphate dehydrogenase, Glycolysis, Tumors, chemistry.chemical_classification, Cell metabolism, 3. Good health, Metabolic pathway, 030104 developmental biology, Enzyme, Oncology, Biochemistry, chemistry, 030220 oncology & carcinogenesis, glucose-6-phosphate dehydrogenase, Cèl·lules canceroses, tumor metabolism, transketolase, Flux (metabolism), Research Paper

Abstract

The pentose phosphate pathway is a fundamental metabolic pathway that provides cells with ribose and NADPH required for anabolic reactions - synthesis of nucleotides and fatty acids - and maintenance of intracellular redox homeostasis. It plays a key role in tumor metabolic reprogramming and has been reported to be deregulated in different types of tumors. Herein, we silenced the most important enzymes of this pathway - glucose-6-phosphate dehydrogenase (G6PD) and transketolase (TKT) - in the human breast cancer cell line MCF7. We demonstrated that inhibition of G6PD, the oxidative branch-controlling enzyme, reduced proliferation, cell survival and increased oxidative stress. At the metabolic level, silencing of both enzymes reduced ribose synthesis. G6PD silencing in particular, augmented the glycolytic flux, reduced lipid synthesis and increased glutamine uptake, whereas silencing of TKT reduced the glycolytic flux. Importantly, we showed using breast cancer patient datasets that expression of both enzymes is positively correlated and that high expression levels of G6PD and TKT are associated with decreased overall and relapse-free survival. Altogether, our results suggest that this metabolic pathway could be subjected to therapeutic intervention to treat breast tumors and warrant further investigation.

Published

2017

10. Ketogenic diet and metabolic regulation of brain microglia

Author

Hector C. Keun, Nelofer Syed, Adrian Benito, Kevin O’Neill, and Nabil Hajji

Subjects

Cancer Research, medicine.medical_specialty, Microglia, medicine.medical_treatment, Metabolism, Biology, Phenotype, Abstracts, Endocrinology, medicine.anatomical_structure, Immune system, Oncology, Metabolic regulation, Tumor progression, Internal medicine, medicine, Ketone bodies, Neurology (clinical), Ketogenic diet

Abstract

Ketogenic diet (KD) has been proposed as a coadjuvant therapy in the treatment of brain tumours. Reduction of blood glucose and increase in ketone bodies concentration are amongst the most important changes induced by KD in patients. Preliminary data collected in our lab indicates that KD induces substantial changes in the immune system in mice bearing brain tumours. Microglia are brain-resident immune cells that account for around 30% of the tumour mass and play a major role in controlling tumour progression by adopting a protumour (M2 polarisation) or antitumour (M1 polarisation) phenotype. We are interested in understating the molecular and metabolic determinants of microglia polarisation and how these can be modulated by the metabolic microenvironment and KD. We report some initial findings that indicate microglia adapt to changes in the metabolic microenvironment and that nutrient availability can modulate microglia activation and polarisation. We believe that the study of microglia metabolism and nutritional interventions like KD can provide new knowledge about the regulation of the brain immune system and unveil novel routes for brain cancer treatment.

Published

2019

11. MIDcor, an R-program for deciphering mass interferences in mass spectra of metabolites enriched in stable isotopes

Author

Adrian Benito, Silvia Marin, Ibrahim H. Polat, Esther Aguilar, Vitaly A. Selivanov, Anibal Miranda, Marta Cascante, Paul W. N. Lee, Anusha Jayaraman, Josep J. Centelles, Universitat de Barcelona, Department of Biochemistry and Molecular Biology [Barcelona, Spain], Universitat de Barcelona (UB), Associated Unit to Consejo Superior de Investigaciones Científicas - CSIC [Barcelona, Spain], University of Barcelona-Institute of Biomedicine - IBUB [Barcelona, Spain], Department of Pediatrics [Torrance, CA, USA], University of California [Los Angeles] (UCLA), University of California (UC)-University of California (UC)- Los Angeles Biomedical Research Institute (LA BioMed), The Spanish Government and the European Union FEDER funds (SAF2014-56059-R), ICREA Academia prize (MC) and AGAUR (2014SGR1017)., European Project: 654241,H2020,H2020-EINFRA-2014-2,PhenoMeNal(2015), European Project: 312941,EC:FP7:INFRA,FP7-INFRASTRUCTURES-2012-1,COSMOS(2012), European Project: 264780,EC:FP7:PEOPLE,FP7-PEOPLE-2010-ITN,METAFLUX(2010), BMC, BMC, PhenoMeNal: A comprehensive and standardised e-infrastructure for analysing medical metabolic phenotype data - PhenoMeNal - - H20202015-09-01 - 2018-08-31 - 654241 - VALID, Developing an efficient e-infrastructure, standards and data-flow for metabolomics and its interface to biomedical and life science e-infrastructures in Europe and world-wide - COSMOS - - EC:FP7:INFRA2012-10-01 - 2015-09-30 - 312941 - VALID, and Metabolic Flux Analysis and Cancer - METAFLUX - - EC:FP7:PEOPLE2010-11-01 - 2014-10-31 - 264780 - VALID

Subjects

0301 basic medicine, Metabolite, [SDV]Life Sciences [q-bio], Bioinformatics, 01 natural sciences, Biochemistry, chemistry.chemical_compound, User-Computer Interface, Isotopes, Structural Biology, Cromatografia de gasos, Carbon Isotopes, Gas chromatography, Isotope, R-program, Stable isotope ratio, Methodology Article, Applied Mathematics, Metabolisme, Computer Science Applications, [SDV] Life Sciences [q-bio], Isotope Labeling, Metabolome, Isòtops, Gas chromatography/mass spectrometry, Cèl·lules, Cells, Mass spectrometry, Gas Chromatography-Mass Spectrometry, Isotopic effect, Cell Line, 03 medical and health sciences, TRACER, Correction of peaks overlapping, Humans, Derivatization, Computational analysis, Molecular Biology, Internet, Chromatography, 010401 analytical chemistry, 0104 chemical sciences, Culture Media, Espectrometria de masses, 030104 developmental biology, Metabolism, chemistry, Mass spectrum, Gas chromatography–mass spectrometry, 13C labeling of metabolites

Abstract

Background: Tracing stable isotopes, such as 13C using various mass spectrometry (MS) methods provides a valuable information necessary for the study of biochemical processes in cells. However, extracting such information requires special care, such as a correction for naturally occurring isotopes, or overlapping mass spectra of various components of the cell culture medium. Developing a method for a correction of overlapping peaks is the primary objective of this study.Results: Our computer program-MIDcor (free at https://github.com/seliv55/mid_correct) written in the R programming language, corrects the raw MS spectra both for the naturally occurring isotopes and for the overlapping of peaks corresponding to various substances. To this end, the mass spectra of unlabeled metabolites measured in two media are necessary: in a minimal medium containing only derivatized metabolites and chemicals for derivatization, and in a complete cell incubated medium. The MIDcor program calculates the difference (D) between the theoretical and experimentally measured spectra of metabolites containing only the naturally occurring isotopes. The result of comparison of D in the two media determines a way of deciphering the true spectra. (1) If D in the complete medium is greater than that in the minimal medium in at least one peak, then unchanged D is subtracted from the raw spectra of the labeled metabolite. (2) If D does not depend on the medium, then the spectrum probably overlaps with a derivatized fragment of the same metabolite, and D is modified proportionally to the metabolite labeling. The program automatically reaches a decision regarding the way of correction. For some metabolites/fragments in the case (2) D was found to decrease when the tested substance was 13C labeled, and this isotopic effect also can be corrected automatically, if the user provides a measured spectrum of the substance in which the 13C labeling is known a priori.Conclusion: Using the developed program improves the reliability of stable isotope tracer data analysis.

Published

2017

12. Metabolic network adaptations in cancer as targets for novel therapies.

Author

Marta Cascante, Adrian Benito, Miriam Zanuy, Pedro Vizán, Silvia Marín, and Pedro de atauri

Subjects

*CANCER treatment, *METABOLITES, *ENZYMES, *STABLE isotopes, *PENTOSE phosphate pathway, *CELL transformation

Abstract

Metabolite concentrations and fluxes are the system variables that characterize metabolism. The systematic study of metabolite profiles is known as metabolomics; however, knowledge of the complete set of metabolites may not be enough to predict distinct phenotypes. A complete understanding of metabolic processes requires detailed knowledge of enzyme-controlled intracellular fluxes. These can be estimated through quantitative measurements of metabolites at different times or by analysing the stable isotope patterns obtained after incubation with labelled substrates. We have identified distinct intracellular fluxes associated with metabolic adaptations accompanying cancer. The maintenance of an imbalance between fluxes for the oxidative and non-oxidative PPP (pentose phosphate pathway) has been shown to be critical for angiogenesis and cancer cell survival. Mouse NIH 3T3 cells transformed by different mutated K-ras oncogenes have differential routing of glucose to anaerobic glycolysis, the PPP and the Krebs cycle. These results indicate that knowledge of metabolic fingerprints associated with an altered genetic profile could be exploited in the rational design of new therapies. We conclude that the understanding of the multifactorial nature of metabolic adaptations in cancer may open new ways to develop novel multi-hit antitumoral therapies. [ABSTRACT FROM AUTHOR]

Published

2010