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早期生长反应基因在人类前列腺癌中的表达

Expression of early growth response genes in human prostate cancer.

作者信息

Eid M A, Kumar M V, Iczkowski K A, Bostwick D G, Tindall D J

机构信息

Department of Urology, Mayo Clinic, Rochester, Minnesota 55905, USA.

出版信息

Cancer Res. 1998 Jun 1;58(11):2461-8.

PMID:9622090
Abstract

Early growth-response (EGR) genes are nuclear transcription factors that are implicated in regulating cell proliferation. Because these genes show divergent expression in various human tumors, we sought to determine their expression in nonmalignant and malignant prostate tissues. Total RNA extracted from prostate tissues was probed with EGR-1, EGR-2, and EGR-alpha cDNA for Northern blots and digoxigenin-labeled cRNA for in situ hybridization. Both Northern blot and in situ hybridization analyses demonstrated increased EGR-1, but not EGR-2 or EGR-alpha expression, in malignant prostate tissue as compared with weak expression in nonmalignant tissue. EGR-1 mRNA was quantified in 96 prostate specimens (86 adenocarcinomas representing different Gleason scores and 10 benign tissues showing no histological manifestation of benign prostatic hypertrophy) using in situ hybridization with an 35S-labeled cRNA probe. EGR-1 mRNA was expressed at significantly higher levels in cancer than in normal prostate (P < 0.001). In cancer with Gleason scores 8-10, the expression of EGR-1 was higher compared with those of lower Gleason scores (P < 0.005). Immunohistochemical staining showed predominately basal cell nuclear EGR-1 protein in prostatic acini. Nuclear staining was weak in nonmalignant tissues, more intense in moderately differentiated carcinoma, and most intense in poorly differentiated carcinoma. These results show that EGR-1 is overexpressed in prostate cancer and suggest a role for EGR-1 in prostate cancer growth.

摘要

早期生长反应(EGR)基因是参与调节细胞增殖的核转录因子。由于这些基因在各种人类肿瘤中表现出不同的表达,我们试图确定它们在非恶性和恶性前列腺组织中的表达情况。从前列腺组织中提取的总RNA用EGR-1、EGR-2和EGR-α cDNA进行Northern印迹杂交,并用地高辛标记的cRNA进行原位杂交。Northern印迹杂交和原位杂交分析均显示,与非恶性组织中的弱表达相比,恶性前列腺组织中EGR-1的表达增加,但EGR-2或EGR-α的表达未增加。使用35S标记的cRNA探针进行原位杂交,对96个前列腺标本(86个代表不同Gleason评分的腺癌和10个无良性前列腺增生组织学表现的良性组织)中的EGR-1 mRNA进行定量。EGR-1 mRNA在癌组织中的表达水平明显高于正常前列腺组织(P < 0.001)。在Gleason评分为8-10的癌组织中,EGR-1的表达高于Gleason评分较低的癌组织(P < 0.005)。免疫组织化学染色显示前列腺腺泡中主要为基底细胞核EGR-1蛋白。非恶性组织中的核染色较弱,中度分化癌中的核染色较强,低分化癌中的核染色最强。这些结果表明EGR-1在前列腺癌中过度表达,并提示EGR-1在前列腺癌生长中发挥作用。

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