Abstract
The risk of cancer and associated mortality increases substantially in humans from the age of 65 years onwards1,2,3,4,5,6. Nonetheless, our understanding of the complex relationship between age and cancer is still in its infancy2,3,7,8. For decades, this link has largely been attributed to increased exposure time to mutagens in older individuals. However, this view does not account for the established role of diet, exercise and small molecules that target the pace of metabolic ageing9,10,11,12. Here we show that metabolic alterations that occur with age can produce a systemic environment that favours the progression and aggressiveness of tumours. Specifically, we show that methylmalonic acid (MMA), a by-product of propionate metabolism, is upregulated in the serum of older people and functions as a mediator of tumour progression. We traced this to the ability of MMA to induce SOX4 expression and consequently to elicit transcriptional reprogramming that can endow cancer cells with aggressive properties. Thus, the accumulation of MMA represents a link between ageing and cancer progression, suggesting that MMA is a promising therapeutic target for advanced carcinomas.
This is a preview of subscription content, access via your institution
Access options
Access Nature and 54 other Nature Portfolio journals
Get Nature+, our best-value online-access subscription
$29.99 / 30 days
cancel any time
Subscribe to this journal
Receive 51 print issues and online access
$199.00 per year
only $3.90 per issue
Buy this article
- Purchase on Springer Link
- Instant access to full article PDF
Prices may be subject to local taxes which are calculated during checkout
Similar content being viewed by others
Data availability
Information about the HS donors and the data from the metabolomics experiment can be found in Supplementary Table 1. RNA-seq data that support the findings of this study have been deposited in the Gene Expression Omnibus (under accession code GSE127001) and are presented in Supplementary Table 2. All raw data files, peak lists, and the sequence database for the proteomics analysis have been deposited in the MASSive repository (https://massive.ucsd.edu) under ID MSV000084974. Other data supporting the findings of this study are available from the corresponding authors upon reasonable request. Source data are provided with this paper.
Code availability
The quantification of invasion/migration assay images were carried out in an automated way on Fiji/ImageJ v1.52 using a custom macro script. This macro is a basic automation script and cannot be used as standalone code, but it is available from the corresponding authors upon reasonable request.
References
Wu, L. E., Gomes, A. P. & Sinclair, D. A. Geroncogenesis: metabolic changes during aging as a driver of tumorigenesis. Cancer Cell 25, 12–19 (2014).
Thigpen, T. et al. Age as a prognostic factor in ovarian carcinoma. The Gynecologic Oncology Group experience. Cancer 71 (Suppl), 606–614 (1993).
Deng, F. et al. Age is associated with prognosis in serous ovarian carcinoma. J. Ovarian Res. 10, 36 (2017).
Gloeckler Ries, L. A., Reichman, M. E., Lewis, D. R., Hankey, B. F. & Edwards, B. K. Cancer survival and incidence from the Surveillance, Epidemiology, and End Results (SEER) program. Oncologist 8, 541–552 (2003).
White, M. C. et al. Age and cancer risk: a potentially modifiable relationship. Am. J. Prev. Med. 46 (Suppl 1), S7–S15 (2014).
Balducci, L. & Ershler, W. B. Cancer and ageing: a nexus at several levels. Nat. Rev. Cancer 5, 655–662 (2005).
Serrano, M. & Blasco, M. A. Cancer and ageing: convergent and divergent mechanisms. Nat. Rev. Mol. Cell Biol. 8, 715–722 (2007).
Migkou, M. et al. Short progression-free survival predicts for poor overall survival in older patients with multiple myeloma treated upfront with novel agent-based therapy. Eur. J. Haematol. 87, 323–329 (2011).
Kasznicki, J., Sliwinska, A. & Drzewoski, J. Metformin in cancer prevention and therapy. Ann. Transl. Med. 2, 57 (2014).
Li, J., Kim, S. G. & Blenis, J. Rapamycin: one drug, many effects. Cell Metab. 19, 373–379 (2014).
De Lorenzo, M. S. et al. Caloric restriction reduces growth of mammary tumors and metastases. Carcinogenesis 32, 1381–1387 (2011).
Ligibel, J. Lifestyle factors in cancer survivorship. J. Clin. Oncol. 30, 3697–3704 (2012).
Ye, X. & Weinberg, R. A. Epithelial–mesenchymal plasticity: a central regulator of cancer progression. Trends Cell Biol. 25, 675–686 (2015).
Wu, Y. & Zhou, B. P. Inflammation: a driving force speeds cancer metastasis. Cell Cycle 8, 3267–3273 (2009).
Ferrucci, L. & Fabbri, E. Inflammageing: chronic inflammation in ageing, cardiovascular disease, and frailty. Nat. Rev. Cardiol. 15, 505–522 (2018).
Zhu, Y., Carvey, P. M. & Ling, Z. Age-related changes in glutathione and glutathione-related enzymes in rat brain. Brain Res. 1090, 35–44 (2006).
Tong, J. et al. Do glutathione levels decline in aging human brain? Free Radic. Biol. Med. 93, 110–117 (2016).
Madeo, F., Carmona-Gutierrez, D., Kepp, O. & Kroemer, G. Spermidine delays aging in humans. Aging (Albany NY) 10, 2209–2211 (2018).
Meynial-Denis, D. Glutamine metabolism in advanced age. Nutr. Rev. 74, 225–236 (2016).
Chandler, R. J. & Venditti, C. P. Genetic and genomic systems to study methylmalonic acidemia. Mol. Genet. Metab. 86, 34–43 (2005).
Riekeberg, E. & Powers, R. New frontiers in metabolomics: from measurement to insight. F1000 Res. 6, 1148 (2017).
Baik, H. W. & Russell, R. M. Vitamin B12 deficiency in the elderly. Annu. Rev. Nutr. 19, 357–377 (1999).
Zhang, J. et al. SOX4 induces epithelial-mesenchymal transition and contributes to breast cancer progression. Cancer Res. 72, 4597–4608 (2012).
Wang, L. et al. SOX4 is associated with poor prognosis in prostate cancer and promotes epithelial-mesenchymal transition in vitro. Prostate Cancer Prostatic Dis. 16, 301–307 (2013).
Yang, M. et al. Estrogen induces androgen-repressed SOX4 expression to promote progression of prostate cancer cells. Prostate 75, 1363–1375 (2015).
Liao, Y. L. et al. Identification of SOX4 target genes using phylogenetic footprinting-based prediction from expression microarrays suggests that overexpression of SOX4 potentiates metastasis in hepatocellular carcinoma. Oncogene 27, 5578–5589 (2008).
Lourenço, A. R. & Coffer, P. J. SOX4: joining the master regulators of epithelial-to-mesenchymal transition? Trends Cancer 3, 571–582 (2017).
Vervoort, S. J. et al. Global transcriptional analysis identifies a novel role for SOX4 in tumor-induced angiogenesis. eLife 7, e27706 (2018).
Wong, C. C., Qian, Y. & Yu, J. Interplay between epigenetics and metabolism in oncogenesis: mechanisms and therapeutic approaches. Oncogene 36, 3359–3374 (2017).
Vervoort, S. J., van Boxtel, R. & Coffer, P. J. The role of SRY-related HMG box transcription factor 4 (SOX4) in tumorigenesis and metastasis: friend or foe? Oncogene 32, 3397–3409 (2013).
Debnath, J., Muthuswamy, S. K. & Brugge, J. S. Morphogenesis and oncogenesis of MCF-10A mammary epithelial acini grown in three-dimensional basement membrane cultures. Methods 30, 256–268 (2003).
Minn, A. J. et al. Genes that mediate breast cancer metastasis to lung. Nature 436, 518–524 (2005).
Yuan, M., Breitkopf, S. B., Yang, X. & Asara, J. M. A positive/negative ion-switching, targeted mass spectrometry-based metabolomics platform for bodily fluids, cells, and fresh and fixed tissue. Nat. Protoc. 7, 872–881 (2012).
Rappsilber, J., Ishihama, Y. & Mann, M. Stop and go extraction tips for matrix-assisted laser desorption/ionization, nanoelectrospray, and LC/MS sample pretreatment in proteomics. Anal. Chem. 75, 663–670 (2003).
Erickson, B. K. et al. Active instrument engagement combined with a real-time database search for improved performance of sample multiplexing workflows. J. Proteome Res. 18, 1299–1306 (2019).
Eng, J. K., McCormack, A. L. & Yates, J. R. An approach to correlate tandem mass spectral data of peptides with amino acid sequences in a protein database. J. Am. Soc. Mass Spectrom. 5, 976–989 (1994).
Elias, J. E. & Gygi, S. P. Target-decoy search strategy for increased confidence in large-scale protein identifications by mass spectrometry. Nat. Methods 4, 207–214 (2007).
Huttlin, E. L. et al. A tissue-specific atlas of mouse protein phosphorylation and expression. Cell 143, 1174–1189 (2010).
Shin, S., Dimitri, C. A., Yoon, S. O., Dowdle, W. & Blenis, J. ERK2 but not ERK1 induces epithelial-to-mesenchymal transformation via DEF motif-dependent signaling events. Mol. Cell 38, 114–127 (2010).
Blighe, K. EnhancedVolcano: publication-ready volcano plots with enhanced colouring and labeling. R Package Version 1.0.1 (2019).
Reich, M. et al. GenePattern 2.0. Nat. Genet. 38, 500–501 (2006).
Dennis, G., Jr et al. DAVID: Database for annotation, visualization, and integrated discovery. Genome Biol. 4, 3 (2003).
Shen, L. & Sinai, M. GeneOverlap: Test and visualize gene overlaps. R Package Version 1.18.0 (2018).
Oskarsson, T. et al. Breast cancer cells produce tenascin C as a metastatic niche component to colonize the lungs. Nat. Med. 17, 867–874 (2011).
Goyenechea, E. et al. Expression of proinflammatory factors in renal cortex induced by methylmalonic acid. Ren. Fail. 34, 885–891 (2012).
van Gorsel, M., Elia, I. & Fendt, S.-M. in Metabolic Signaling: Methods and Protocols Methods in Molecular Biology (eds Lundt, Sophia & Fendt, S.-M.) chapter 4 (Humana, 2018).
Elia, I. et al. Proline metabolism supports metastasis formation and could be inhibited to selectively target metastasizing cancer cells. Nat. Commun. 8, 15267 (2017).
Lorendeau, D. et al. Dual loss of succinate dehydrogenase (SDH) and complex I activity is necessary to recapitulate the metabolic phenotype of SDH mutant tumors. Metab. Eng. 43 (Pt. B), 187–197 (2017).
Fernandez, C. A., Des Rosiers, C., Previs, S. F., David, F. & Brunengraber, H. Correction of 13C mass isotopomer distributions for natural stable isotope abundance. J. Mass Spectrom. 31, 255–262 (1996).
Acknowledgements
We thank members of the Blenis and Cantley laboratories for input; P. Coffer for the list of SOX4 targets; R. Pritchard for experimental assistance. A.P.G. is supported by a Susan G. Komen Postdoctoral Fellowship and a Pathway to Independence Award from NCI (K99CA218686). T.S. is supported by the NIH F31 pre-doctoral fellowship F31CA220750. J.F.-G. is supported by an FWO fellowship. C.K. was supported by a Medical Scientist Training Program grant from the NIGM/NIH T32GM007739 to the Weill Cornell/Rockefeller/Sloan Kettering Tri-Institutional MD-PhD Program. This research was supported by NIH grant R01CA46595 to J.B. S.-M.F. is funded by the European Research Council under the ERC Consolidator Grant Agreement number 711486 – MetaRegulation, FWO research grants and projects, and KU Leuven Methusalem Co-funding.
Author information
Authors and Affiliations
Contributions
A.P.G. conceived the project. A.P.G. and D.I. performed all the molecular biology experiments, the EMT-related experiments and the invasion and migration experiments, prepared the RNA for RNA-seq experiments and assisted on all other experiments. A.P.M. quantified the migration and invasion experiments. T.S. evaluated the stemness markers. V.L., J.E.E. and D.B. performed the mouse experiments. A.R. performed the drug resistance assays, prepared the metabolites for metabolomic analysis, produced the viral particles and assisted in multiple other experiments. J.H. generated the constructs and the cell lines. C.K. and J.E.E. performed the assessment of histone post-translational modifications. D.B. and M.P. measured the concentration of MMA and analysed the data. A.A. and N.D. performed and analysed the results of the proteomic analysis of HS samples. T.S., E.M., I.E. and J.F.-G. assisted with the metabolomics experiments and helped with the metabolite treatments. J.A. performed the metabolomic analysis in HS. A.P.G., J.A., L.C.C., R.d.C., N.D., S.-M.F. and J.B. supervised the project. A.P.G., D.I., J.F.-G., M.P., D.B., T.S., V.L., J.E.E., and N.D. analysed the data. The manuscript was written by A.P.G. and edited by J.B., D.I., V.L., T.S., J.F.-G., I.E., D.B. and S.-M.F. All authors discussed the results and approved the manuscript.
Corresponding authors
Ethics declarations
Competing interests
L.C.C. owns equity in, receives compensation from, and serves on the Board of Directors and Scientific Advisory Board of Agios Pharmaceuticals and Petra Pharma Corporation. No potential competing interests were disclosed by the other authors.
Additional information
Peer review information Nature thanks Xiang H.-F. Zhang and the other, anonymous, reviewer(s) for their contribution to the peer review of this work.
Publisher’s note Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
Extended data figures and tables
Extended Data Fig. 1 Serum of old donors induces a mesenchymal-like phenotype in non-small cell lung cancer cells.
Morphology of A549 cells cultured for 4 days with HS (n = 15 biologically independent samples per HS donor group, first batch of donors). Scale bar = 100 μm; red label indicates outlier donors.
Extended Data Fig. 2 Serum of old donors induces an epithelial-to-mesenchymal transition phenotype in non-small cell lung cancer cells.
Morphology of A549 cells cultured for 4 days with HS (n = 15 biologically independent samples per HS donor group, second batch of donors). Scale bar = 100 μm; red label indicates outlier donors.
Extended Data Fig. 3 Serum of old donors induces a mesenchymal-like phenotype in triple negative breast cancer cells.
Morphology of HCC1806 cells cultured for 4 days with HS (n = 15 biologically independent samples per HS donor group, second batch of donors). Scale bar = 100 μm; red label indicates outlier donors.
Extended Data Fig. 4 Serum of old donors induces aggressive properties in cancer cells and displays a distinct metabolic profile.
a, b, Immunoblots of A549 (total of n = 30 biologically independent samples per HS donor group, see Fig. 1b) (a) and HCC1806 (n = 15 biologically independent samples per HS donor group) (b) cells cultured for 4 days with HS c, Resistance to paclitaxel in A549 cells cultured for 4 days with HS (n = 15 biologically independent samples per HS donor group, two-way ANOVA). d, Volcano plot summarizing the proteomics analysis of all 60 human serum samples used in this study. e, List of all metabolites that are increased at a statistically significant level in the sera of old donors (n = 11 biologically independent HS donors, two-sided t-test). f, Immunoblots of A549 cells treated with 5 mM of each metabolite for 10 days; representative images (n = 4 independent experiments; QA: quinolinate, PEP: phosphoenolpyruvate, MMA: methylmalonic acid) g, Concentrations of MMA in 10 outlier human sera (serum from 5 young and 5 old donors, each bar represents the concentration of a single donor) h, i, Concentrations of vitamin B12 in all HS samples (n = 30 biologically independent samples per HS donor group, two sided t-test) (h) and 10 outlier human sera (serum from 5 young and 5 old donors, each bar represents the concentration of a single donor) (i). For (c, h) data are presented as mean ± SEM. For gel source data, see Supplementary Fig. 2.
Extended Data Fig. 5 Methylmalonic acid promotes epithelial-to-mesenchymal transition and metastatic-like properties.
a, b, Immunoblots of MCF-10A (a) and HCC1806 (b) cells treated with MMA for 10 days (n = 4 independent experiments). c, d, Immunoblots of MCF-10A (c), A549 and HCC1806 (d) cells treated with 5 mM of the indicated acids for 10 days (n = 4 independent experiments). e-h, Resistance to carboplatin and paclitaxel in A549 (e, f) and HCC1806 (g, h) cells treated with 5 mM MMA for 10 days (n = 4 independent experiments, two-way ANOVA). i. Transwell migration assay of A549 cells treated with 5 mM MMA for 10 days (n = 4 independent experiments, two-sided t-test). j, k, Stemness evaluated by the increase in the CD44 marker in MCF-10A cells treated with MMA for 10 days (j) and by the increase in the CD44 marker and the decrease in CD24 marker in A549 cells treated with 5 mM MMA for 10 days (k) (n = 4 independent experiments, two-sided t-test). l, Immunoblots of MDA-MB-231-luciferase cells treated with 5 mM MMA for 5 days (n = 4 independent experiments). For (e-k) data are presented as mean ± SEM; (a-d, l) are representative images. For gel source data, see Supplementary Fig. 2.
Extended Data Fig. 6 Methylmalonic acid delivery is regulated by lipidic structures (LSs) in the sera of old donors.
a, b, Intracellular MMA concentrations in A549 cells cultured with HS for 4 h (n = 6 biologically independent samples per HS donor group, two-sided t-test) (a) and with 5 mM MMA for indicated time periods (n = 6 independent experiments, two-sided t-test) (b). c, d, Immunoblots of MCF-10A (c), A549 and HCC1806 (d) cells treated with various concentrations (5–0.001 mM) of dimethyl methylmalonic acid for 10 days (n = 4 independent experiments). e, Immunoblots of A549 cells cultured for 4 days with young and old untreated HS, or old HS that was passed through size exclusion columns or delipidated (n = 6 biologically independent samples per HS donor group). f, MMA concentrations in the human serum used in (e) (n = 6 biologically independent samples per HS donor group, two-sided t-test). g-i, Immunoblots of A549 cells treated with complexes of lipofectamine (LA) with indicated amounts of MMA (n = 3 independent experiments) (g) and with LSs isolated from FBS that were complexed with indicated amounts of MMA (n = 4 independent experiments) (h), or of MCF10A treated with LSs isolated from FBS that were complexed with indicated amounts of MMA (n = 4 independent experiments) (i). j, Intracellular MMA concentrations in A549 cells cultured with MMA-loaded FBS lipidic structures (LSs) for 4 h (n = 6 independent experiments, two-sided t-test). k, Immunoblots of A549 cells treated with LSs isolated from young/old HS, and MMA-loaded LSs isolated from young HS (10 μM MMA) (n = 6 biologically independent samples per HS donor group). l, MMA concentrations in serum from old donors after depletion of LSs compared to control HS (n = 6 biologically independent samples per HS donor group, two-sided t-test). m, Immunoblots of A549 cells treated for 4 days with HS from old donors after depletion of LSs or from control donors (n = 6 biologically independent samples per HS donor group). For (a, b, f, j, l) data are presented as mean ± SEM; (c, d, e, h, i, k, m) are representative images. For gel source data, see Supplementary Fig. 2.
Extended Data Fig. 7 Methylmalonic acid induces tumour progression through regulation of pro-aggressive and poor prognosis genes.
a-c, End-point serum MMA concentrations (n = 8 mice per group, two-sided t-test) (a), bioluminescence intensity of the primary tumours (n = 9 mice on vehicle group and n = 10 on Low and High MMA group, two-sided t-test) (b), and metastases (n = 10 mice per group) (c) in mice that were xenografted with MDA-MB-231-luciferase cells and treated with MMA in their drinking water. d-f, Summary of RNA-seq analysis in A549 cells treated with 5 mM MMA for 10 days: a heatmap representation of hierarchical clustering of the top 100 changed mRNAs (d), functional annotation clustering analysis of the >1.5-fold changed mRNAs detected by RNA-seq analysis in A549 cells treated with 5 mM MMA for 10 days (e), and a volcano plot representation of the complete curated data set (the statistically significantly (FDR ≤ 0.05) altered mRNAs that are changed more than 1.5-fold are displayed in red) (f) (n = 3 independent experiments). g, h, mRNA levels of pro-aggressive cell intrinsic factors (g) and secreted factors (h) evaluated by qPCR in A549 cells treated with 5 mM MMA for 10 days (n = 4 independent experiments, two-sided t-test). i, mRNA levels of transcription factors evaluated by qPCR in A549 cells treated with 5 mM MMA for 3 days (n = 3 independent experiments, two-sided t-test). j, k, Immunoblots of MCF-10A and HCC1806 cells treated with MMA for 10 days (j) and of MDA-MB-231-luciferase cells treated with 5 mM MMA for 5 days (k) (n = 4 independent experiments) l, Immunoblots of HCC1806 and MD-MBA-231-luciferase cells cultured with HS for 4 days (n = 6 biologically independent samples per HS donor group) m, Venn diagram showing the overlap of altered mRNAs between A549 cells treated with MMA for 10 days and the genes altered by SOX4 induction28 (Fisher’s exact test). For (a-c, g-i) data are presented as mean ± SEM; (j, k) are representative images. For gel source data, see Supplementary Fig. 2.
Extended Data Fig. 8 SOX4 mediates methylmalonic acid-induced pro-aggressive transcriptional reprogramming.
a-d, mRNA levels of fibronectin (FN) (a), IL32 (b), N-cadherin (CDH2) (c) and TGFB1I1 (d) evaluated by qPCR in A549 cells with SOX4 knockdown and treated with 5 mM MMA for 10 days (n = 4 independent experiments, two-sided t-test). e, f, Immunoblots (e) and transwell migration/invasion assays (f) of MDA-MB-231-luciferase cells with SOX4 knockdown and treated with 5 mM MMA for 5 days (n = 4 independent experiments, two-sided t-test). g, Immunoblots of MDA-MB-231-luciferase cells with SOX4 knockdown and treated with HS for 5 days (n = 6 biologically independent samples per HS donor group) h, i, Resistance to carboplatin and paclitaxel in A549 cells with SOX4 knockdown and treated with 5 mM MMA for 10 days (h) and in MDA-MB-231-luciferase cells with SOX4 knockdown and treated with 5 mM MMA for 5 days (i) (n = 4 independent experiments, two-way ANOVA). For (a-d, f, h, i) data are presented as mean ± SEM; (e, g) are representative images. For gel source data, see Supplementary Fig. 2.
Extended Data Fig. 9 Methylmalonic acid induces SOX4 through activation of TGFβ signalling.
a, b, Immunoblots for histone marks in A549 (a) and MCF-10A (b) cells treated with 5 mM MMA for 1 or 3 days (n = 4 independent experiments). c, TGFB2 mRNA levels determined by qPCR in A549 cells treated with 5 mM MMA for 3 days (n = 4 independent experiments, two-sided t-test). d, e, Immuno-blots of A549 cells treated with 5 mM MMA for the indicated time points (d) or with 5 mM MMA in the presence of TGFBR inhibitor for 5 days (e) (n = 4 independent experiments). f, Age-induced accumulation of circulatory MMA induces SOX4 expression through the TGFβ pathway and elicits a transcriptional reprogramming that supports aggressiveness, promoting tumour progression and metastasis formation; This illustration was created using the Smart Servier Medical Art library (https://smart.servier.com/), which is licensed under a Creative Commons Attribution 3.0 Unported License. For (c) data are presented as mean ± SEM; (a, b, d, e) are representative images. For gel source data, see Supplementary Fig. 2.
Supplementary information
Supplementary Information
This file contains Supplementary Table 3, which provides the primer sequences for qPCR analyses, Supplementary Fig. 1, which provides the representative gating strategy for the FACS analyses and Supplementary Fig. 2, which provide the Western source images for all figures.
Supplementary Table
Supplementary Table 1: This file contains information about the human serum donors and the metabolomics analyses on the human serum.
Supplementary Table
Supplementary Table 2: This file contains information about the differentially changed genes in the 3-day and 10-day RNA-seq data, GO-term analysis of the 10-day RNA-seq data, the overlap of our RNA-seq data and the published Sox4 RNA-seq data, and the DAVID analysis of this overlap.
Rights and permissions
About this article
Cite this article
Gomes, A.P., Ilter, D., Low, V. et al. Age-induced accumulation of methylmalonic acid promotes tumour progression. Nature 585, 283–287 (2020). https://doi.org/10.1038/s41586-020-2630-0
Received:
Accepted:
Published:
Issue Date:
DOI: https://doi.org/10.1038/s41586-020-2630-0
This article is cited by
-
An aging-related immune landscape in the hematopoietic immune system
Immunity & Ageing (2024)
-
Metabolic heterogeneity in cancer
Nature Metabolism (2024)
-
1H-NMR metabolomics analysis identifies hypoxanthine as a novel metastasis-associated metabolite in breast cancer
Scientific Reports (2024)
-
Single-cell transcriptomics enable the characterization of local extension in retinoblastoma
Communications Biology (2024)
-
The association between methylmalonic acid, a biomarker of mitochondrial dysfunction, and risk of prostate cancer
International Urology and Nephrology (2024)
Comments
By submitting a comment you agree to abide by our Terms and Community Guidelines. If you find something abusive or that does not comply with our terms or guidelines please flag it as inappropriate.