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灰盖鬼伞(Coprinus cinereus)子实体形成过程中表达的半乳糖凝集素编码基因cgl2的启动子分析

Promoter analysis of cgl2, a galectin encoding gene transcribed during fruiting body formation in Coprinopsis cinerea (Coprinus cinereus).

作者信息

Bertossa Rinaldo C, Kües Ursula, Aebi Markus, Künzler Markus

机构信息

Institute of Microbiology, ETH Zürich, Wolfgang-Pauli-Strasse 10, 8093 Zürich, Switzerland.

出版信息

Fungal Genet Biol. 2004 Dec;41(12):1120-31. doi: 10.1016/j.fgb.2004.09.001.

Abstract

In the homobasidiomycete Coprinopsis cinerea, expression of the two fruiting body-specific galectins, CGL1 and CGL2, is controlled by nutrients, light and darkness and the A mating type genes. In this study, we analyzed the promoter of the cgl2 gene by measuring transcript levels by quantitative real-time PCR and show that regulation of CGL2 expression occurs at the transcriptional level. A minimal promoter sufficient to confer regulated expression of a heterologous reporter gene and comprising 627 base pairs from the start codon was defined. On the minimal promoter we identified a 120 bp sequence mediating induction of the cgl2 gene in constant darkness. Along with direct repeats (TGGAAG/TGGAAG/GGAA), the sequence contains a CRE consensus site (cAMP-responsive element, TGCGTCA) suggesting the involvement of cAMP signaling in cgl2 activation. No specific elements responsible for light repression and mating type regulation were found in the promoter.

摘要

在同担子菌灰盖鬼伞中,两种子实体特异性半乳糖凝集素CGL1和CGL2的表达受营养物质、光照和黑暗以及A交配型基因的控制。在本研究中,我们通过定量实时PCR测量转录水平来分析cgl2基因的启动子,并表明CGL2表达的调控发生在转录水平。定义了一个足以赋予异源报告基因调控表达的最小启动子,其包含起始密码子上游627个碱基对。在最小启动子上,我们鉴定出一个120 bp的序列,该序列介导在持续黑暗中cgl2基因的诱导。该序列与直接重复序列(TGGAAG/TGGAAG/GGAA)一起包含一个CRE共有位点(cAMP反应元件,TGCGTCA),表明cAMP信号传导参与cgl2的激活。在启动子中未发现负责光抑制和交配型调控的特定元件。

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