原发性乳腺癌短期抗雌激素治疗对雌激素受体mRNA和蛋白质表达以及雌激素调节基因的影响。
Effects of short-term antiestrogen treatment of primary breast cancer on estrogen receptor mRNA and protein expression and on estrogen-regulated genes.
作者信息
McClelland R A, Manning D L, Gee J M, Anderson E, Clarke R, Howell A, Dowsett M, Robertson J F, Blamey R W, Wakeling A E, Nicholson R I
机构信息
Tenovus Cancer Research Centre, Cardiff, UK.
出版信息
Breast Cancer Res Treat. 1996;41(1):31-41. doi: 10.1007/BF01807034.
Effects of the pure antiestrogen ICI182780 and tamoxifen on ER-protein, ER-mRNA, and estrogen-regulated mRNA expression were analysed using matched pretreatment core-cut biopsies and post-treatment mastectomy samples from 43 ER positive human breast cancers. Sixteen controls received either no preoperative treatment (n = 9) (7 days) or placebo (n = 7) (median 21 days) prior to primary surgery. Nineteen patients received ICI182780 6 mg/day (n = 10) or 18 mg/day (n = 9) for 7 days. Eight patients were given preoperative tamoxifen (4 x 40 mg-day 1, 20 mg/day thereafter, median 21 days). ER-protein expression was assessed on pre and post treatment samples by immunocytochemistry. ER, pS2, pLIV1, and actin-mRNA expression was determined by northern analysis on post-treatment samples only. ER-mRNA levels were similar to controls following ICI182780 or tamoxifen treatment. However ER-protein levels were significantly suppressed by ICI182780, particularly at the higher dosage (p = 0.0013). Tamoxifen had no significant effect on ER-protein levels. The ER-mRNA and ER-protein contents of control tumors were linearly related (Spearman r = 0.719, p = 0.006). A similar relationship between pretreatment protein and post ICI182780 treatment mRNA levels was observed (r = 0.652, p = 0.005). However, comparison of post ICI182780 treatment protein and mRNA results shows a loss of linearity through a reduction in protein without concurrent loss of mRNA (r = 0.28, p = 0.257). pS2 mRNA hybridization was lower in ICI182780 treated samples than controls (Mann-Whitney p = 0.035) but was unaffected by tamoxifen. pLIV1 mRNA hybridization was uninfluenced by either treatment. Short term exposure of breast tumors to ICI182780 appears to produce a greater inhibition of estrogen-induced transcriptional events than tamoxifen. These effects appear to occur without a concurrent reduction in ER mRNA levels.
使用43例雌激素受体(ER)阳性的人类乳腺癌患者治疗前的配对核心切割活检组织和治疗后的乳房切除术样本,分析了纯抗雌激素药物ICI182780和他莫昔芬对ER蛋白、ER信使核糖核酸(mRNA)以及雌激素调节的mRNA表达的影响。16例对照患者在初次手术前未接受任何术前治疗(n = 9)(7天)或接受安慰剂治疗(n = 7)(中位时间21天)。19例患者接受7天的ICI182780治疗,剂量为6毫克/天(n = 10)或18毫克/天(n = 9)。8例患者术前给予他莫昔芬(第1天4×40毫克,此后20毫克/天,中位时间21天)。通过免疫细胞化学对治疗前和治疗后的样本评估ER蛋白表达。仅通过对治疗后样本进行Northern印迹分析来测定ER、pS2、pLIV1和肌动蛋白mRNA的表达。ICI182780或他莫昔芬治疗后,ER mRNA水平与对照相似。然而,ICI182780可显著抑制ER蛋白水平,尤其是高剂量时(p = 0.0013)。他莫昔芬对ER蛋白水平无显著影响。对照肿瘤的ER mRNA和ER蛋白含量呈线性相关(斯皮尔曼相关系数r = 0.719,p = 0.006)。观察到治疗前蛋白水平与ICI182780治疗后mRNA水平之间存在类似关系(r = 0.652,p = 0.005)。然而,比较ICI182780治疗后的蛋白和mRNA结果显示,通过蛋白减少导致线性关系丧失,而mRNA没有同时减少(r = 0.28,p = 0.257)。在ICI182780治疗的样本中,pS2 mRNA杂交低于对照(曼-惠特尼检验p = 0.035),但不受他莫昔芬影响。pLIV1 mRNA杂交不受任何一种治疗的影响。与他莫昔芬相比,乳腺癌短期暴露于ICI182780似乎对雌激素诱导的转录事件产生更大的抑制作用。这些作用似乎在ER mRNA水平没有同时降低的情况下发生。
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