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首页> 外文期刊>V T T Publications Information Service >Isolation of the ace1 Gene Encoding a Cys_2-His_2 Transcription Factor Involved in Regulation of Activity of the Cellulase Promoter cbh1 of Trichoderma reesei
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Isolation of the ace1 Gene Encoding a Cys_2-His_2 Transcription Factor Involved in Regulation of Activity of the Cellulase Promoter cbh1 of Trichoderma reesei

机译:编码涉及里氏木霉纤维素酶启动子cbh1活性调节的Cys_2-His_2转录因子的ace1基因的分离。

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摘要

A genetic selection method was developed for the cloning of positive-acting transcriptional regulatory genes in Saccharomyces cerevisiae. The method was applied for the isolation of activators of Trichoderma reesei (Hypocrea jecorina) cellulase genes. Activator genes were isolated from a T. reesei expression cDNA library on the basis of the ability of their translation products to activate transcription from the full-length T. reesei cbh1 promoter coupled to the S. cerevisiae HIS3 gene and to support the growth of the yeast colonies in the absence of histidine. Among the clones obtained was the ace1 gene encoding a novel polypeptide, ACEI, that contains three zinc finger motifs of Cys_2-His_2 type. Possible ACEI homologues were found among expressed sequence tags of Aspergillus and Neurospora. The ability of ACEI to bind to the cbh1 promoter was further confirmed in the yeast one-hybrid system. In vitro binding and gel mobility shift assays revealed several binding sites for the ACEI protein in the cbh1 promoter. Disruption of the ace1 gene in T. reesei resulted in retarded growth of the fungus on a cellulose-containing medium, on which cel-lulases are normally highly expressed.
机译:开发了一种遗传选择方法,用于克隆酿酒酵母中的正性转录调控基因。该方法被用于分离里氏木霉(红霉菌)纤维素酶基因的激活剂。激活子基因是从里氏木霉表达cDNA文库中分离出来的,基于其翻译产物激活与里氏木霉HIS3基因偶联的全长里氏木霉cbh1启动子的转录并支持其生长的能力。没有组氨酸的酵母菌落。在获得的克隆中有ace1基因编码一种新型多肽ACEI,该多肽包含三个Cys_2-His_2类型的锌指基序。在曲霉和神经孢菌的表达序列标签中发现了可能的ACEI同源物。在酵母一杂交系统中进一步证实了ACEI与cbh1启动子结合的能力。体外结合和凝胶迁移率迁移分析揭示了cbh1启动子中ACEI蛋白的几个结合位点。里氏木霉中ace1基因的破坏导致真菌在含纤维素培养基上的生长受阻,该培养基通常高度表达纤维素。

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