Li Xin, Qi Xiaoping, Zhou Lingyin, Catera Deborah, Rote Neal S, Potashkin Judith, Abdul-Karim Fadi W, Gorodeski George I
Department of Reproductive Biology, CASE Case Western Reserve University, Cleveland, OH 44106, USA.
Gynecol Oncol. 2007 Jul;106(1):233-43. doi: 10.1016/j.ygyno.2007.03.032. Epub 2007 May 4.
To understand the potential role of P2X(7) as biomarker of endometrial cancer, and the molecular mechanisms by which cancerous epithelial cells maintain low expression of P2X(7).
Feasibility clinical experimental study. Normal (28), simple or complex hyperplasia (7), complex hyperplasia with atypia (6) and cancer endometrial discarded tissues (40) were obtained from a total of 81 women, ages 25-75. Endpoint for P2X(7) protein was average pixel signal density of tissue immunoreactivity with anti-P2X(7) antibody. Endpoint for P2X(7) mRNA was one-step quantitative Real-Time PCR. Experiments in-vitro included normal (hEVEC) and cancerous cervical epithelial cells (HeLa) transfected with reporter plasmid containing luciferase-3' untranslated region (3'UTR)-P2X(7) cDNA, using as endpoint steady-state luciferase mRNA levels.
Levels of P2X(7) protein and mRNA were significantly lower in vivo, in tissues of complex hyperplasia with atypia or endometrial adenocarcinoma, than in tissues of normal endometrium, simple hyperplasia or complex hyperplasia tissues (sensitivity and specificity of 89-100%, p<0.0001-0.01). Steady-state levels of luciferase mRNA increased over a 6 h incubation period in hEVEC cells transfected with the 3'UTR-P2X(7)-luciferase vector, but decreased in HeLa cells transfected with the reporter plasmid.
Tissue levels of P2X(7) protein and mRNA can differentiate effectively and accurately between normal and benign hyperplastic endometrial tissues from pre-cancerous and cancer tissues. Cancerous epithelial cells degrade P2X(7) mRNA by activation of instability domains located at the 3'UTR of the P2X(7).
了解P2X(7)作为子宫内膜癌生物标志物的潜在作用,以及癌上皮细胞维持P2X(7)低表达的分子机制。
可行性临床实验研究。从总共81名年龄在25 - 75岁的女性中获取正常组织(28例)、单纯或复杂性增生组织(7例)、非典型复杂性增生组织(6例)和子宫内膜癌废弃组织(40例)。P2X(7)蛋白的终点指标是组织与抗P2X(7)抗体免疫反应的平均像素信号密度。P2X(7) mRNA的终点指标是一步定量实时PCR。体外实验包括用含有荧光素酶-3'非翻译区(3'UTR)-P2X(7) cDNA的报告质粒转染的正常宫颈上皮细胞(hEVEC)和癌性宫颈上皮细胞(HeLa),以荧光素酶mRNA稳态水平作为终点指标。
在体内,非典型复杂性增生或子宫内膜腺癌组织中P2X(7)蛋白和mRNA水平显著低于正常子宫内膜、单纯增生或复杂性增生组织(敏感性和特异性为89 - 100%,p<0.0001 - 0.01)。在转染了3'UTR - P2X(7) - 荧光素酶载体的hEVEC细胞中,荧光素酶mRNA稳态水平在6小时孵育期内升高,但在转染了报告质粒的HeLa细胞中降低。
P2X(7)蛋白和mRNA的组织水平能够有效且准确地区分正常和良性增生的子宫内膜组织与癌前及癌组织。癌上皮细胞通过激活位于P2X(7) 3'UTR的不稳定结构域来降解P2X(7) mRNA。