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使用改良的代表性差异分析鉴定ErbB3刺激基因。

Identification of ErbB3-stimulated genes using modified representational difference analysis.

作者信息

Edman C F, Prigent S A, Schipper A, Feramisco J R

机构信息

Cancer Center, University of California, San Diego School of Medicine, La Jolla, CA 92093-0684, U.S.A.

出版信息

Biochem J. 1997 Apr 1;323 ( Pt 1)(Pt 1):113-8. doi: 10.1042/bj3230113.

Abstract

The epidermal growth factor receptor (EGFR) family of tyrosine kinases is involved in the growth of normal and tumour cells. The specific contribution of each of the four family members to these processes remains unclear. In the present study we have used a PCR-based subtractive approach to identify differences in messages induced in response to activation of ErbB3 and EGFR. The approach described is a modification of the representational difference analysis technique adapted for analysis of cDNA, which we have modified to permit identification of differential gene expression using as little as 20 microg of total RNA as the starting material. The mRNA obtained from EGF-stimulated NIH-3T3 cells expressing chimaeric EGFR-ErbB3 receptors provided the tester amplicons (small PCR-amplified fragments) which were subtracted against driver amplicons derived from unstimulated NIH-3T3 cells expressing the EGFR-ErbB3 chimaera or EGF-stimulated NIH-3T3 cells overexpressing the EGFR. A total of 22 different clones were isolated, 90% of which showed increased expression in the tester amplicons. Six of these, corresponding to known DNA sequences, were selected for further Northern blot analysis against total RNA prepared from the starting cell lines. Of these, the gene encoding the protein dlk (or a closely related protein, Pref-1) was identified as being regulated by ErbB3 but not by the EGFR. Other genes appeared to be elevated by both ErbB3 and EGFR, including those encoding c-jun, Ret finger protein (RFP), neuroleukin and amyloid protein precursor. One gene product, TIS11, was identified as being regulated by EGFR but not by ErbB3.

摘要

酪氨酸激酶的表皮生长因子受体(EGFR)家族参与正常细胞和肿瘤细胞的生长。该家族四个成员对这些过程的具体作用仍不清楚。在本研究中,我们采用基于PCR的消减方法来鉴定因ErbB3和EGFR激活而诱导产生的信息差异。所描述的方法是对适用于cDNA分析的代表性差异分析技术的一种改进,我们对其进行了修改,以便能够使用低至20微克的总RNA作为起始材料来鉴定差异基因表达。从表达嵌合EGFR-ErbB3受体的EGF刺激的NIH-3T3细胞中获得的mRNA提供了测试扩增子(小的PCR扩增片段),将其与来自表达EGFR-ErbB3嵌合体的未刺激NIH-3T3细胞或过表达EGFR的EGF刺激的NIH-3T3细胞产生的驱动扩增子进行消减。总共分离出22个不同的克隆,其中90%在测试扩增子中显示表达增加。选择其中六个与已知DNA序列对应的克隆,针对从起始细胞系制备的总RNA进行进一步的Northern印迹分析。其中,编码蛋白dlk(或密切相关蛋白Pref-1)的基因被鉴定为由ErbB3而非EGFR调节。其他基因似乎在ErbB3和EGFR的作用下均上调,包括那些编码c-jun、Ret指蛋白(RFP)、神经白细胞素和淀粉样蛋白前体的基因。一种基因产物TIS11被鉴定为由EGFR而非ErbB3调节。

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