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Transcriptional activators Cat8 and Sip4 discriminate between sequence variants of the carbon source-responsive promoter element in the yeast Saccharomyces cerevisiae

机译:转录激活因子Cat8和Sip4区分了酿酒酵母中碳源响应性启动子元件的序列变体

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摘要

The structural genes for gluconeogenesis in the yeast Saccharomyces cerevisiae are activated by the carbon source-responsive element (CSRE) found in the respective upstream regions. Regulatory genes CAT8 and SIP4 both encode zinc-cluster proteins which can bind to CSRE motifs and activate target genes under conditions of glucose deprivation. In this work, we describe a functional analysis of sequence variants containing single mutations within the strongly activating CSRE ICL1 motif. While the sequence CCNNNNNNCCG was required as the minimal UAS for gene activation by both Cat8 and Sip4, the activators responded differently to sequence variations in the central part of the CSRE. Our results allowed us to derive a consensus sequence for efficient gene activation by Cat8 (YCCNYTNRKCCG), while a more specific motif is required for activation by Sip4 (TCCATTSRTCCGR). Although their zinc cluster domains are clearly related, Cat8 and Sip4 are not isofunctional. This conclusion is further supported by the finding that biosynthetic derepression of Cat8 in the presence of a nonfermentable carbon source precedes that of Sip4 by about 90 min.
机译:酵母酿酒酵母中糖异生的结构基因被相应上游区域中发现的碳源响应元件(CSRE)激活。调节基因CAT8和SIP4都编码锌簇蛋白,这些蛋白可以结合CSRE基序并在葡萄糖剥夺条件下激活靶基因。在这项工作中,我们描述了在强激活CSRE ICL1 母题中包含单个突变的序列变体的功能分析。虽然序列CCNNNNNNCCG是Cat8和Sip4激活基因所需的最小UAS,但激活剂对CSRE中央部分的序列变化的反应不同。我们的结果使我们能够得出一个由Cat8(YCCNYTNRKCCG)有效激活基因的共有序列,而由Sip4(TCCATTSRTCCGR)激活需要一个更具体的基序。尽管它们的锌簇结构域明显相关,但Cat8和Sip4不是同功能的。在不可发酵碳源存在下,Cat8的生物合成抑制作用比Sip4抑制作用约90分钟的发现进一步支持了这一结论。

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