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Soy Isoflavones Exert Differential Effects on Androgen Responsive Genes in LNCaP Human Prostate Cancer Cells

机译:大豆异黄酮对LNCaP人前列腺癌细胞中雄激素反应基因有差异作用

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摘要

The high consumption of soy isoflavones in Asian diets has been correlated to a lower incidence of clinically important cases of prostate cancer. This study characterized the effects of a soy-derived isoflavone concentrate (ISF) on growth and gene expression profiles in the LNCaP, an androgen-sensitive human prostate cancer cell line. ISF caused a dose-dependent decrease in viability (P<0.05) and DNA synthesis (P<0.01), as well as an accumulation of cells in G2/M, and G0/G1 phases of the cell cycle compared with controls. Using Affymetrix oligonucleotide DNA microarrays (U133A), we determined that ISF upregulated 80 genes and downregulated 33 genes (P<0.05) involving androgen-regulated genes and pathways controlling cell cycle, metabolism, and intracellular trafficking. Changes in the expression of the genes of interest, identified by microarrays, were validated by Western immunoblot, Northern blot, and luciferase reporter assays. Prostate-specific antigen, homeobox protein NKX3, and cyclin B mRNA were significantly reduced, whereas mRNA was significantly upregulated for p21CIP1, a major cell cycle inhibitory protein, and fatty acid and cholesterol synthesis pathway genes. ISF also significantly increased cyclin-dependent kinase inhibitor p27KIP1 and FOXO3A/FKHRL1, a forkhead transcription factor. A differential pattern of androgen-regulated genes was apparent with genes involved in prostate cancer progression being downregulated by ISF, whereas metabolism genes were upregulated. In summary, we found that ISF inhibits the growth of LNCaP cells through the modulation of cell cycle progression and the differential expression of androgen-regulated genes. Thus, ISF treatment serves to identify new therapeutic targets designed to prevent proliferation of malignant prostate cells.
机译:亚洲饮食中大豆异黄酮的高消耗与临床上重要的前列腺癌病例的发生率较低相关。这项研究表征了大豆异黄酮浓缩物(ISF)对LNCaP(一种对雄激素敏感的人前列腺癌细胞系)中生长和基因表达谱的影响。与对照组相比,ISF导致活力(P <0.05)和DNA合成(P <0.01)以及细胞周期的G2 / M和G0 / G1期的细胞蓄积性呈剂量依赖性降低。使用Affymetrix寡核苷酸DNA微阵列(U133A),我们确定ISF上调了80个基因,下调了33个基因(P <0.05),涉及雄激素调节基因和控制细胞周期,代谢和细胞内运输的途径。通过Western免疫印迹,Northern印迹和荧光素酶报告基因检测法验证了通过微阵列鉴定的目的基因表达的变化。前列腺特异性抗原,同源盒蛋白NKX3和细胞周期蛋白B mRNA显着降低,而p21 CIP1 ,一种主要的细胞周期抑制蛋白以及脂肪酸和胆固醇合成途径基因的mRNA显着上调。 ISF还显着增加了细胞周期蛋白依赖性激酶抑制剂p27 KIP1 和前叉转录因子FOXO3A / FKHRL1。雄激素调节基因的差异模式很明显,与前列腺癌进展有关的基因被ISF下调,而代谢基因被上调。总之,我们发现ISF通过调节细胞周期进程和雄激素调节基因的差异表达来抑制LNCaP细胞的生长。因此,ISF治疗可用于确定旨在预防恶性前列腺细胞增殖的新治疗靶标。

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