Dual effect of vitamin D3 on breast cancer-associated fibroblasts

被引:4
作者
Labedz, Natalia [1 ,2 ]
Anisiewicz, Artur [1 ]
Stachowicz-Suhs, Martyna [1 ]
Banach, Joanna [1 ]
Klopotowska, Dagmara [1 ]
Maciejczyk, Adam [3 ,4 ]
Gazinska, Patrycja [2 ,5 ]
Piotrowska, Aleksandra [6 ]
Dziegiel, Piotr [6 ]
Matkowski, Rafal [3 ,4 ]
Wietrzyk, Joanna [1 ]
机构
[1] Hirszfeld Inst Immunol & Expt Therapy, Dept Expt Oncol, Weigla 12, PL-53114 Wroclaw, Poland
[2] Lukasiewicz Res Network, PORT Polish Ctr Technol Dev, Stablowicka 147, PL-54066 Wroclaw, Poland
[3] Wroclaw Med Univ, Dept Oncol, Pl Ludwika Hirszfelda 12, PL-53413 Wroclaw, Poland
[4] Lower Silesian Oncol Pulmonol & Hematol Ctr, Pl Ludwika Hirszfelda 12, PL-53413 Wroclaw, Poland
[5] Kings Coll London, Res Oncol, Div Canc Studies, London SE1 3SS, England
[6] Wroclaw Med Univ, Dept Human Morphol & Embryol, Div Histol & Embryol, Ul Chalubinskiego 6a, PL-50368 Wroclaw, Poland
关键词
Tumor microenvironment; Breast cancer; Fibroblasts; Vitamin D-3; Calcitriol; GROWTH-FACTOR-BETA; TISSUE INHIBITOR; TENASCIN-C; TUMOR STROMA; D-RECEPTOR; CELLS; OSTEOPONTIN; EXPRESSION; PATHWAY;
D O I
10.1186/s12885-024-11961-z
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
Background Cancer-associated fibroblasts (CAFs) play an important role in the tumor microenvironment. Despite the well-known in vitro antitumoral effect of vitamin D-3 (VD3), its impact on breast CAFs is almost unknown. In this study, we analyzed the ex vivo effects of calcitriol on CAFs isolated from breast cancer tissues. Methods CAFs were cultured with 1 and 10 nM calcitriol and their phenotype; gene expression, protein expression, and secretion were assessed. Calcitriol-treated CAFs-conditioned media (CM) were used to analyze the effect of CAFs on the migration and protein expression of MCF-7 and MDA-MB-231 cells. Results Tumor tissues from VD3-deficient patients exhibited lower levels of beta-catenin and TGF beta 1, along with higher levels of CYP24A1 compared to VD3-normal patients. In VD3-deficient patients, CAF infiltration was inversely associated with CYP24A1 levels and positively correlated with OPN levels. Calcitriol diminished CAFs' viability, but this effect was weaker in premenopausal and VD3-normal patients. Calcitriol reduced mRNA expression of CCL2, MMP9, TNC, and increased PDPN, SPP1, and TIMP1. It also decreased the secretion of CCL2, TNC, and the activity of MMP-2, while increasing cellular levels of TIMP1 in CAFs from all patient groups. In nonmetastatic and postmenopausal patients, PDPN surface expression increased, and CAFs CM from these groups decreased MCF-7 cell migration after ex vivo calcitriol treatment. In premenopausal and VD3-deficient patients, calcitriol reduced IDO1 expression in CAFs. Calcitriol-treated CAFs CM from these patients decreased OPN expression in MCF-7 and/or MDA-MB-231 cells. However, in premenopausal patients, calcitriol-treated CAFs CM also decreased E-cadherin expression in both cell lines. Conclusion The effects of calcitriol on breast CAFs, both at the gene and protein levels, are complex, reflecting the immunosuppressive or procancer properties of CAFs. The anticancer polarization of CAFs following ex vivo calcitriol treatment may result from decreased CCL2, TNC (gene and protein), MMP9, and MMP-2, while the opposite effect may result from increased PDPN, TIMP1 (gene and protein), and SPP1. Despite these multifaceted effects of calcitriol on molecule expression, CAFs' CMs from nonmetastatic and postmenopausal patients treated ex vivo with calcitriol decreased the migration of MCF-7 cells.
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页数:25
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