Stanway C A, Gibbs J M, Kearsey S E, López M C, Baker H V
Department of Plant Sciences, University of Oxford, UK.
Mol Gen Genet. 1994 Apr;243(2):207-14. doi: 10.1007/BF00280318.
Transcription of the yeast phosphoglycerate kinase gene (PGK) is activated by an array of nuclear factors including the multifunctional protein RAP1. We have demonstrated that the transcriptional co-activator GAL11, which was identified as an auxiliary factor to GAL4 and which is believed to interact with the zinc finger of the trans-activator, positively influences the level of PGK transcription on both fermentable and non-fermentable carbon sources. This positive effect is only observed when the RAP1 site in the upstream activation sequence (UAS) is present, implying that GAL11 acts through RAP1. Expression of the RAP1 gene is not reduced in the gal11 background, and in vivo footprinting shows that GAL11 does not influence RAP1 DNA-binding activity. Therefore the effect of GAL11 on PGK transcription must be mediated at the PGK UAS, presumably as part of the activation complex. It has been proposed that RAP1 may act as a facilitator of GCR1 binding at the PGK UAS and therefore it is conceivable that the target for GAL11 may in fact be GCR1. A further implication of this study is that GAL11 can interact with proteins such as RAP1 or GCR1 that are apparently structurally dissimilar from GAL4 and other zinc finger DNA-binding proteins.
酵母磷酸甘油酸激酶基因(PGK)的转录由一系列核因子激活,包括多功能蛋白RAP1。我们已经证明,转录共激活因子GAL11,它被鉴定为GAL4的辅助因子,并且被认为与反式激活因子的锌指相互作用,在可发酵和不可发酵碳源上均对PGK转录水平产生正向影响。只有当上游激活序列(UAS)中的RAP1位点存在时,才会观察到这种正向效应,这意味着GAL11通过RAP1起作用。在gal11背景中,RAP1基因的表达没有降低,并且体内足迹分析表明GAL11不影响RAP1的DNA结合活性。因此,GAL11对PGK转录的影响必定是在PGK UAS处介导的,大概是作为激活复合物的一部分。有人提出,RAP1可能作为GCR1在PGK UAS处结合的促进因子,因此可以想象GAL11的靶标实际上可能是GCR1。这项研究的另一个含义是,GAL11可以与诸如RAP1或GCR1等蛋白质相互作用,这些蛋白质在结构上显然与GAL4和其他锌指DNA结合蛋白不同。
