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UAS1-B/CYC1两个半位点之间存在重叠的证据——Cyp1p(Hap1p)DNA结合的新模型。

Evidence of an overlap between the two half-sites of UAS1-B/CYC1--a new model for Cyp1p (Hap1p) DNA binding.

作者信息

Naït-Kaoudjt R, Guiard B, Gervais M

机构信息

Centre de Génétique Moléculaire, Laboratoire propre du Centre National de la Recherche Scientifique associé à l'Université Pierre et Marie Curie, Gif-sur-Yvette, France. nait

出版信息

Eur J Biochem. 1998 May 15;254(1):111-6. doi: 10.1046/j.1432-1327.1998.2540111.x.

Abstract

Cyp1p (Hap1p) is a yeast transcriptional regulator belonging to the zinc-cluster family. CGGNNNTANCGG was identified by PCR selection as the DNA sequence allowing its optimal binding. Nevertheless, this sequence is not a consensus sequence, the simultaneous presence of the two CGGs and the TA generally not being found in the known natural Cyp1p targets. In fact, our previous studies showed that the mechanism of Cyp1p DNA binding was target dependent. Data concerning the binding of Cyp1p to the UAS1-B/CYC1 are presented here. This target, containing the CGGGGTTTACGG sequence, was found to present the particular ability of stabilizing the binding of only one molecule of some monomeric Cyp1p fragments. This property was used to investigate the actual contribution of the TT and CGG sequences in the binding of Cyp1p. Our results indicate that each CGG belongs to a different half-site and, in contrast to a previous hypothesis, that the T nucleotide located four bases downstream from the left CGG is essential for the binding of one monomer to each half-site. The two half-sites of the UAS1-B/CYC1 thus overlap.

摘要

Cyp1p(Hap1p)是一种属于锌簇家族的酵母转录调节因子。通过PCR筛选鉴定出CGGNNNTANCGG为允许其最佳结合的DNA序列。然而,该序列并非共有序列,在已知的天然Cyp1p靶标中通常不会同时出现两个CGG和TA。事实上,我们之前的研究表明,Cyp1p与DNA结合的机制是依赖于靶标的。本文展示了关于Cyp1p与UAS1 - B/CYC1结合的数据。这个包含CGGGTTTACGG序列的靶标,被发现具有仅稳定某些单体Cyp1p片段的一个分子结合的特殊能力。这一特性被用于研究TT和CGG序列在Cyp1p结合中的实际作用。我们的结果表明,每个CGG属于不同的半位点,并且与之前的假设相反,位于左CGG下游四个碱基处的T核苷酸对于一个单体与每个半位点的结合至关重要。因此,UAS1 - B/CYC1的两个半位点相互重叠。

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