Targeting stromal components in the tumor microenvironment for cancer therapy
In the tumor microenvironment (TME), different cell components crosstalk with each other through various growth factors, cytokines, chemokines, and enzymes. They offered crucial survival signals for tumor cell proliferation and metastasis. Data presented in this thesis demonstrate approaches to target the stroma of the TME, which provided a novel paradigm for cancer therapy. It involves the conception of overcoming the resistance of conventional therapy, cut-out cancer cell energy support, and interrupting invasive assistance of cancer cells. We specifically focused on these two aspects: first, to resolve antiangiogenic drugs (AAD) resistance in those cancers with a lipid-rich environment or high FGF expression. In addition, to manipulate the brown adipose tissue (BAT) into mega BAT can be an approach in cancer therapy (Paper I-III). Second, we revealed the roles of stromal cells, including the cancerassociated fibroblasts (CAFs) and tumor-associated macrophages (TAMs), in pancreatic ductal adenocarcinoma (PDAC) (Paper IV); and the role of CAFs in the cancer hosts with disturbed circadian rhythm (CR) (Paper V).
In Paper I, we revealed the mechanism of AAD drug resistance in tumors surrounded by adipose tissue or lipid-rich environment, for example, colorectal cancer (CRC), PDAC and hepatocellular carcinoma (HCC) in the steatotic liver. Anti-VEGF-based AAD failed to reduce tumor size but triggered vessel regression in tumor tissues, leading to severe hypoxia in the TME. Hypoxia resulted in tumor metabolic reprogramming from glucose-based metabolism to free fatty acids (FFAs)-based metabolism. FFAs provided energy support to tumor cells, leading to accelerate tumor cell proliferation. Inhibition of FFA transporter reversed AAD resistance in anti-tumor effect. Our data suggested a therapeutic approach to reverse the AAD resistance in tumors with a lipid-rich environment.
Our previous study revealed the cold exposure and other β3-adrenorecptor stimuli induced the brown adipose tissue (BAT) activation by increasing the non-shivering thermogenesis (NST). The activated BAT decreased blood glucose and impeded glycolysis-based metabolism in cancer cells could suppress tumor growth. In Paper II, we addressed an approach to enlarge BAT into a mega-size BAT (megaBAT) in adult animals. In BAT, the differentiation of certain progenitor cells is controlled by the platelet-derived growth factor receptor α (PDGFRα). Using pharmacological approaches and genetic deletion, we downregulated the PDGFRα in BAT progenitor cells and promoted progenitor cells differentiation into functional brown adipocytes. We found a specific microRNA to target the PDGFRα signaling in vivo. The whole BAT tissue mass was markedly increased after PDGFRα inhibition owing to the increase of brown adipocyte numbers. We found that the obese mice with megaBAT under cold exposure showed improvement in blood glucose level, insulin tolerance, and blood lipid level. Histological analysis showed that the steatotic livers were markedly reversed in obese mice with megaBAT. The megaBAT could become a therapeutic approach to treat cancer and metabolic diseases.
We previously reported that fibroblast growth factor 2 (FGF-2) as one of the angiogenic factors contributed to tumor vessel remodeling by recruiting NG2 positive pericytes onto tumor vessels through the PDGFRβ signaling. Therefore, monotherapy with anti-VEGF or anti-PDGFR had become resistant in tumors with high FGF-2 expression. So far, there are no potent anti-FGF drugs available. In Paper III, we found combination therapy with anti-VEGF and anti- PDGFRβ showed superior anti-tumor effects in high FGF-2 tumors. Anti-PDGFRβ treatment suppressed pericyte recruitment, and anti-VEGF precisely targeted tumor vessels. With this study, we provided a new paradigm for resolving AAD resistance by targeting FGF-2 off-target signaling, VEGF and PDGF in cancer therapy.
In Paper IV, we identified the CAFs-TAMs crosstalk through the IL-33-ST2-CXCL3-CXCR2 axis in PDAC and triggered cancer cell metastasis. Mouse and human PDAC samples under unbiased genomic-wide profiling analysis and genetic and pharmacological gain/loss-offunction experiments demonstrated a high level of IL-33 expression. IL-33 bound to its receptor ST2 on the TAMs and induced TAMs infiltration. Transcriptomic analysis identified IL-33-ST2 induced high CXCL3 expression, which was produced by TMAs. CXCL3 bound to its receptors CXCR2 on CAFs induced CAFs-myoCAF transition and cell proliferation. CAFs transited to myoCAFs had a high expression of collagen III, which induced the formation of tumor cells and myofibroblast clusters. Tumor cells increased metastasis under this tumormyofibroblasts clusters. Pharmacological targeting of this pathway would provide a potential therapeutic strategy for treating PDAC.
Paper V we presented the link between CR disruption and tumor metastasis. We explored CR disruption by using a genetic model of Bmal1 gene knockout (KO) mice. Various types of tumors in Bmal1 KO mice presented high growth speed with an elevated expression of myofibroblast markers. Unbiased genomic-wide profiling using the stromal vascular fraction (SVF) from the tumors of Bmal1 KO mice demonstrated a downregulated expression of the plasminogen activator inhibitor (PAI-1) gene. The BMAL1 protein directly regulated PAI-1 gene transcription. Lacking BMAL1 resulted in low PAI-1 expression, which continuously removed the inhibition of downstream proteins, including tissue plasmin activator (tPA) and urokinase (uPA). The tPA and uPA accumulation transformed plasminogen into plasmin, which converted the latent TGF-β into active form. The active TGF-β contributed to the CAFs transition into myofibroblasts, which induced tumor tissue mass expansion and increased metastasis. Inhibition of TGF-β in tumors with CR disruption or maintenance of CR homeostasis could be a therapeutic approach to tumor therapy.
Collectively, the works in this thesis uncover important roles of stromal cellular components in the TME, which lay the ground for the development of novel pharmaceutical approaches in cancer therapy.
List of scientific papers
I. H. Iwamoto, M. Abe, Y. Yang, D. Cui, T. Seki, M. Nakamura, K. Hosaka, S. Lim, J. Wu, X. He, X. Sun, Y. Lu, Q. Zhou, W. Shi, T. Torimura, G. Nie, Q. Li and Y. Cao (2018). Cancer Lipid Metabolism Confers Antiangiogenic Drug Resistance. Cell Metabolism. 28 (1): 104-117, e105.
https://doi.org/10.1016/j.cmet.2018.05.005
II. Q. Du*, J. Wu*, C. Fischer, T. Seki, X. Jing, J. Gao, X. He, K. Hosaka, L. Tong, A. Yasue, M. Miyake, M. Sobajima, S. Oyadomari, X. Sun, Y. Yang, Q. Zhou, M. Ge, W. Tao, S. Yao and Y. Cao (2022). Generation of mega brown adipose tissue in adults by controlling brown adipocyte differentiation in vivo. Proceedings of the National Academy of Sciences. 119 (40): e2203307119. *Equal contribution.
https://doi.org/10.1073/pnas.2203307119
III. K. Hosaka, Y. Yang, T. Seki, Q. Du, X. Jing, X. He, J. Wu, Y. Zhang, H. Morikawa, M. Nakamura, M. Scherzer, X. Sun, Y. Xu, T. Cheng, X. Li, X. Liu, Q. Li, Y. Liu, A. Hong, Y. Chen and Y. Cao (2020). Therapeutic paradigm of dual targeting VEGF and PDGF for effectively treating FGF-2 off-target tumors. Nature Communications. 11 (1):3704.
https://doi.org/10.1038/s41467-020-17525-6
IV. X. Sun, X. He, Y. Zhang, K. Hosaka, P. Andersson, J. Wu, J. Wu, X. Jing, Q. Du, X. Hui, B. Ding, Z. Guo, A. Hong, X. Liu, Y. Wang, Q. Ji, R. Beyaert, Y. Yang, Q. Li and Y. Cao (2021). Inflammatory cell-derived CXCL3 promotes pancreatic cancer metastasis through a novel myofibroblasthijacked cancer escape mechanism. Gut. (2021).
https://doi.org/10.1136/gutjnl-2020-322744
V. J. Wu*, X. Jing*, Q. Du, X. Sun, J. Gao, X. He, K. Hosaka, C. Zhao, W. Tao, G. A. FtzGerald, Y. Yang, L. Jensen and Y. Cao. Disruption of circadian rhythm promotes cancer metastasis through the BMAL1-PAI-1-TGF-β-myoCAF signaling mechanism. *Equal contribution. [Manuscript]
History
Defence date
2023-01-13Department
- Department of Microbiology, Tumor and Cell Biology
Publisher/Institution
Karolinska InstitutetMain supervisor
Cao, YihaiCo-supervisors
Hosaka, KayokoPublication year
2022Thesis type
- Doctoral thesis
ISBN
978-91-8016-899-1Number of supporting papers
5Language
- eng