Department of Pharmaceutical Sciences, University of Maryland School of Pharmacy, Baltimore, MD 21201, USA.
Department of Pharmacy, Health and Nutritional Sciences, University of Calabria, Ed. Polifunzionale, I-87036 Arcavacata di Rende, CS, Italy.
Cells. 2022 Feb 24;11(5):792. doi: 10.3390/cells11050792.
Vitamin A is an essential diet-derived nutrient that has biological activity affected through an active metabolite, all-trans retinoic acid (atRA). Retinol-binding protein type 1 (RBP1) is an intracellular chaperone that binds retinol and retinal with high affinity, protects retinoids from non-specific oxidation, and delivers retinoids to specific enzymes to facilitate biosynthesis of RA. RBP1 expression is reduced in many of the most prevalent cancers, including breast cancer. Here, we sought to understand the relationship between RBP1 expression and atRA biosynthesis in mammary epithelial cells, as well as RBP1 expression and atRA levels in human mammary tissue. We additionally aimed to investigate the impact of RBP1 expression and atRA on the microenvironment as well as the potential for therapeutic restoration of RBP1 expression and endogenous atRA production. Using human mammary ductal carcinoma samples and a series of mammary epithelial cell lines representing different stages of tumorigenesis, we investigated the relationship between RBP1 expression as determined by QPCR and atRA via direct liquid chromatography-multistage-tandem mass spectrometry-based quantification. The functional effect of RBP1 expression and atRA in epithelial cells was investigated via the expression of direct atRA targets using QPCR, proliferation using Ki-67 staining, and collagen deposition via picrosirius red staining. We also investigated the atRA content of stromal cells co-cultured with normal and tumorigenic epithelial cells. Results show that RBP1 and atRA are reduced in mammary tumor tissue and tumorigenic epithelial cell lines. Knock down of RBP1 expression using shRNA or overexpression of RBP1 supported a direct relationship between RBP1 expression with atRA. Increases in cellular atRA were able to activate atRA direct targets, inhibit proliferation and inhibit collagen deposition in epithelial cell lines. Conditions encountered in tumor microenvironments, including low glucose and hypoxia, were able to reduce RBP1 expression and atRA. Treatment with either RARα agonist AM580 or demethylating agent Decitabine were able to increase RBP1 expression and atRA. Cellular content of neighboring fibroblasts correlated with the RA producing capacity of epithelial cells in co-culture. This work establishes a direct relationship between RBP1 expression and atRA, which is maintained when RBP1 expression is restored therapeutically. The results demonstrate diseases with reduced RBP1 could potentially benefit from therapeutics that restore RBP1 expression and endogenous atRA.
维生素 A 是一种必需的膳食来源营养素,其生物活性受到活性代谢物全反式视黄酸 (atRA) 的影响。视黄醇结合蛋白 1(RBP1)是一种细胞内伴侣蛋白,能与视黄醇和视黄醛高亲和力结合,保护类视黄醇免受非特异性氧化,并将类视黄醇递送给特定的酶,以促进 RA 的生物合成。RBP1 的表达在许多最常见的癌症中都降低了,包括乳腺癌。在这里,我们试图了解 RBP1 表达与乳腺上皮细胞中 atRA 生物合成之间的关系,以及 RBP1 表达与人类乳腺组织中 atRA 水平之间的关系。我们还旨在研究 RBP1 表达和 atRA 对微环境的影响,以及恢复 RBP1 表达和内源性 atRA 产生的治疗潜力。使用人乳腺导管癌样本和一系列代表不同肿瘤发生阶段的乳腺上皮细胞系,我们通过直接液相色谱-多级串联质谱法基于定量检测来研究 RBP1 表达(由 QPCR 确定)与 atRA 之间的关系。通过 QPCR 检测直接 atRA 靶基因的表达、Ki-67 染色检测增殖以及 picrosirius 红染色检测胶原蛋白沉积,研究了 RBP1 表达和 atRA 在上皮细胞中的功能作用。我们还研究了与正常和致瘤上皮细胞共培养的基质细胞中的 atRA 含量。结果表明,RBP1 和 atRA 在乳腺肿瘤组织和致瘤上皮细胞系中减少。使用 shRNA 敲低 RBP1 表达或过表达 RBP1 支持 RBP1 表达与 atRA 之间的直接关系。细胞内 atRA 的增加能够激活 atRA 直接靶基因,抑制上皮细胞系的增殖和胶原蛋白沉积。肿瘤微环境中遇到的条件,包括低糖和缺氧,能够降低 RBP1 表达和 atRA。用 RARα 激动剂 AM580 或去甲基化剂地西他滨治疗能够增加 RBP1 表达和 atRA。与上皮细胞共培养的邻近成纤维细胞的细胞内含量与 RA 产生能力相关。这项工作建立了 RBP1 表达与 atRA 之间的直接关系,当 RBP1 表达通过治疗恢复时,这种关系得以维持。结果表明,表达降低的疾病可能受益于恢复 RBP1 表达和内源性 atRA 的治疗。
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