Aronheim A, Zandi E, Hennemann H, Elledge S J, Karin M
Department of Pharmacology, Program in Biomedical Sciences, School of Medicine, University of California, San Diego, La Jolla 92093-0636, USA.
Mol Cell Biol. 1997 Jun;17(6):3094-102. doi: 10.1128/MCB.17.6.3094.
Transcription factor AP-1 transduces environmental signals to the transcriptional machinery. To ensure a quick response yet maintain tight control over AP-1 target genes, AP-1 activity is likely to be negatively regulated in nonstimulated cells. To identify proteins that interact with the Jun subunits of AP-1 and repress its activity, we developed a novel screen for detecting protein-protein interactions that is not based on a transcriptional readout. In this system, the mammalian guanyl nucleotide exchange factor (GEF) Sos is recruited to the Saccharomyces cerevisiae plasma membrane harboring a temperature-sensitive Ras GEF, Cdc25-2, allowing growth at the nonpermissive temperature. Using the Sos recruitment system, we identified new c-Jun-interacting proteins. One of these, JDP2, heterodimerizes with c-Jun in nonstimulated cells and represses AP-1-mediated activation.
转录因子AP-1将环境信号传导至转录机制。为确保快速响应并对AP-1靶基因保持严格控制,在未受刺激的细胞中,AP-1的活性可能受到负调控。为了鉴定与AP-1的Jun亚基相互作用并抑制其活性的蛋白质,我们开发了一种新型筛选方法来检测蛋白质-蛋白质相互作用,该方法不基于转录读数。在这个系统中,哺乳动物鸟苷酸交换因子(GEF)Sos被招募到含有温度敏感型Ras GEF(Cdc25-2)的酿酒酵母质膜上,从而使其在非允许温度下生长。利用Sos招募系统,我们鉴定出了新的与c-Jun相互作用的蛋白质。其中之一JDP2,在未受刺激的细胞中与c-Jun形成异源二聚体并抑制AP-1介导的激活。
