通过竞争性聚合酶链反应检测乳腺癌中真核翻译起始因子4E(eIF4E)基因扩增
Detection of eIF4E gene amplification in breast cancer by competitive PCR.
作者信息
Sorrells D L, Black D R, Meschonat C, Rhoads R, De Benedetti A, Gao M, Williams B J, Li B D
机构信息
Department of Surgery, Louisiana State University Medical Center, Shreveport 71130, USA.
出版信息
Ann Surg Oncol. 1998 Apr-May;5(3):232-7. doi: 10.1007/BF02303778.
BACKGROUND
Initiation factor eIF4E binds to mRNA as the initial step for protein translation. Overexpression of the eIF4E oncoprotein has been found in breast cancer but not in benign breast tissue. The objective of this study is to determine if eIF4E oncoprotein overexpression is associated with eIF4E gene amplification in breast cancer using Western blots and competitive polymerase chain reaction (PCR).
METHODS
Unknown concentrations of DNA extracted from breast specimens were amplified by PCR using a set of primers spanning intron 2/exon 3 of the eIF4E gene. In the same PCR tube, an internal control consisting of a known concentration of an eIF4E DNA template with 20-base pair (bp) deletion was used as the competitive reference standard (CRS) for competitive PCR. Gel electrophoresis of the PCR products was performed and the bands quantified by densitometry. eIF4E gene amplification was then determined relative to a nonamplified gene (gastrin). Using an anti-eIF4E rabbit antibody, Western blots were performed on benign and malignant breast specimens. Quantification was accomplished by developing blots with a color assay using nitro blue tetrazolium (NBT) and 5-bromo-4-chloro-3-indolyl phosphate (BCIP), scanned and analyzed by densitometry.
RESULTS
Twenty-two breast specimens (14 cancer, 8 control) from patients were examined for eIF4E gene amplification and oncoprotein expression. In all fourteen specimens from stage I-III breast cancer patients, eIF4E overexpression was detected at 3- to 30-fold ( 16.71 +/- 7.83) elevations. Similarly, all 14 specimens demonstrated eIF4E gene amplification by competitive PCR (3.69 +/- 1.27). In the eight benign breast specimens examined, all were negative for eIF4E overexpression and gene amplification.
CONCLUSIONS
Overexpression of eIF4E was associated with eIF4E gene amplification in breast cancer specimens. No overexpression or gene amplification was detected in benign breast tissues. eIF4E gene amplification may be one mechanism for eIF4E oncoprotein overexpression.
背景
起始因子eIF4E与mRNA结合是蛋白质翻译的起始步骤。已发现在乳腺癌中eIF4E癌蛋白过表达,而在良性乳腺组织中未发现。本研究的目的是使用蛋白质印迹法和竞争性聚合酶链反应(PCR)来确定乳腺癌中eIF4E癌蛋白过表达是否与eIF4E基因扩增有关。
方法
使用一组跨越eIF4E基因内含子2/外显子3的引物,通过PCR扩增从乳腺标本中提取的未知浓度的DNA。在同一PCR管中,将由已知浓度的具有20个碱基对(bp)缺失的eIF4E DNA模板组成的内部对照用作竞争性PCR的竞争性参考标准(CRS)。对PCR产物进行凝胶电泳,并通过光密度测定法定量条带。然后相对于未扩增基因(胃泌素)确定eIF4E基因扩增。使用抗eIF4E兔抗体,对良性和恶性乳腺标本进行蛋白质印迹分析。通过使用硝基蓝四唑(NBT)和5-溴-4-氯-3-吲哚磷酸(BCIP)的显色测定法对印迹进行显影、扫描并通过光密度测定法进行分析来完成定量。
结果
对22例患者的乳腺标本(14例癌症标本,8例对照标本)进行了eIF4E基因扩增和癌蛋白表达检测。在所有来自I-III期乳腺癌患者的14个标本中,检测到eIF4E过表达,升高了3至30倍(16.71±7.83)。同样,所有14个标本通过竞争性PCR显示eIF4E基因扩增(3.69±1.27)。在检测的8个良性乳腺标本中,所有标本的eIF4E过表达和基因扩增均为阴性。
结论
乳腺癌标本中eIF4E过表达与eIF4E基因扩增有关。在良性乳腺组织中未检测到过表达或基因扩增。eIF4E基因扩增可能是eIF4E癌蛋白过表达的一种机制。
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