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翼状螺旋转录因子CPCR1参与产黄青霉中β-内酰胺生物合成的调控。

Winged helix transcription factor CPCR1 is involved in regulation of beta-lactam biosynthesis in the fungus Acremonium chrysogenum.

作者信息

Schmitt Esther K, Bunse Astrid, Janus Danielle, Hoff Birgit, Friedlin Ernst, Kürnsteiner Hubert, Kück Ulrich

机构信息

Lehrstuhl für Allgemeine und Molekulare Botanik, Ruhr-Universität Bochum, D-44780 Bochum, Germany.

出版信息

Eukaryot Cell. 2004 Feb;3(1):121-34. doi: 10.1128/EC.3.1.121-134.2004.

Abstract

Winged helix transcription factors, including members of the forkhead and the RFX subclasses, are characteristic for the eukaryotic domains in animals and fungi but seem to be missing in plants. In this study, in vitro and in vivo approaches were used to determine the functional role of the RFX transcription factor CPCR1 from the filamentous fungus Acremonium chrysogenum in cephalosporin C biosynthesis. Gel retardation analyses were applied to identify new binding sites of the transcription factor in an intergenic promoter region of cephalosporin C biosynthesis genes. Here, we illustrate that CPCR1 recognizes and binds at least two sequences in the intergenic region between the pcbAB and pcbC genes. The in vivo relevance of the two sequences for gene activation was demonstrated by using pcbC promoter-lacZ fusions in A. chrysogenum. The deletion of both CPCR1 binding sites resulted in an extensive reduction of reporter gene activity in transgenic strains (to 12% of the activity level of the control). Furthermore, Acremonium transformants with multiple copies of the cpcR1 gene and knockout strains support the idea of CPCR1 being a regulator of cephalosporin C biosynthesis gene expression. Significant differences in pcbC gene transcript levels were obtained with the knockout transformants. More-than-twofold increases in the pcbC transcript level at 24 and 36 h of cultivation were followed by a reduction to approximately 80% from 48 to 96 h in the knockout strain. The overall levels of the production of cephalosporin C were identical in transformed and nontransformed strains; however, the knockout strains showed a striking reduction in the level of the biosynthesis of intermediate penicillin N to less than 20% of that of the recipient strain. We were able to show that the complementation of the cpcR1 gene in the knockout strains reverses pcbC transcript and penicillin N amounts to levels comparable to those in the control. These results clearly indicate the involvement of CPCR1 in the regulation of cephalosporin C biosynthesis. However, the complexity of the data points to a well-controlled or even functional redundant network of transcription factors, with CPCR1 being only one player within this process.

摘要

翼状螺旋转录因子,包括叉头亚类和RFX亚类的成员,是动物和真菌真核结构域的特征,但在植物中似乎不存在。在本研究中,采用体外和体内方法来确定丝状真菌产黄青霉中RFX转录因子CPCR1在头孢菌素C生物合成中的功能作用。凝胶阻滞分析用于鉴定转录因子在头孢菌素C生物合成基因的基因间启动子区域中的新结合位点。在此,我们表明CPCR1识别并结合pcbAB和pcbC基因之间基因间区域中的至少两个序列。通过在产黄青霉中使用pcbC启动子-lacZ融合体,证明了这两个序列在体内对基因激活的相关性。两个CPCR1结合位点的缺失导致转基因菌株中报告基因活性大幅降低(降至对照活性水平的12%)。此外,具有多个cpcR1基因拷贝的产黄青霉转化体和敲除菌株支持CPCR1是头孢菌素C生物合成基因表达调节因子的观点。敲除转化体的pcbC基因转录水平存在显著差异。在培养24和36小时时,敲除菌株中pcbC转录水平增加了两倍多,随后在48至96小时时降至约80%。转化菌株和未转化菌株中头孢菌素C的总体产量相同;然而,敲除菌株中中间产物青霉素N的生物合成水平显著降低,降至受体菌株的不到20%。我们能够证明敲除菌株中cpcR1基因的互补使pcbC转录本和青霉素N的量恢复到与对照相当的水平。这些结果清楚地表明CPCR1参与了头孢菌素C生物合成的调节。然而,数据的复杂性表明转录因子存在一个控制良好甚至功能冗余的网络,CPCR1只是这个过程中的一个参与者。

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