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酵母氮代谢物阻遏由不同于谷氨酰胺和谷氨酸储备的信号维持。

Yeast nitrogen catabolite repression is sustained by signals distinct from glutamine and glutamate reservoirs.

作者信息

Fayyad-Kazan Mohammad, Feller A, Bodo E, Boeckstaens M, Marini A M, Dubois E, Georis I

机构信息

Institut de Recherches Microbiologiques J.-M. Wiame, 1070, Brussels, Belgium.

Laboratoire de Biologie du Transport Membranaire, Institut de Biologie et de Médecine Moléculaires, Université Libre de Bruxelles, 6041, Gosselies, Belgium.

出版信息

Mol Microbiol. 2016 Jan;99(2):360-79. doi: 10.1111/mmi.13236. Epub 2015 Nov 13.

DOI:10.1111/mmi.13236
PMID:26419331
Abstract

Nitrogen catabolite repression (NCR) is a wide transcriptional regulation program enabling baker's yeast to downregulate genes involved in the utilization of poor nitrogen sources when preferred ones are available. Nowadays, glutamine and glutamate, the major nitrogen donors for biosyntheses, are assumed to be key metabolic signals regulating NCR. NCR is controlled by the conserved TORC1 complex, which integrates nitrogen signals among others to regulate cell growth. However, accumulating evidence indicate that the TORC1-mediated control of NCR is only partial, arguing for the existence of supplementary regulatory processes to be discovered. In this work, we developed a genetic screen to search for new players involved in NCR signaling. Our data reveal that the NADP-glutamate dehydrogenase activity of Gdh1 negatively regulates NCR-sensitive gene transcription. By determining the total, cytoplasmic and vacuolar pools of amino acids, we show that there is no positive correlation between glutamine/glutamate reservoirs and the extent of NCR. While our data indicate that glutamine could serve as initial trigger of NCR, they show that it is not a sufficient signal to sustain repression and point to the existence of yet unknown signals. Providing additional evidence uncoupling TORC1 activity and NCR, our work revisits the dogmas underlying NCR regulation.

摘要

氮分解代谢物阻遏(NCR)是一种广泛的转录调控程序,使面包酵母能够在有优质氮源时下调参与利用劣质氮源的基因。如今,谷氨酰胺和谷氨酸作为生物合成的主要氮供体,被认为是调节NCR的关键代谢信号。NCR由保守的TORC1复合体控制,该复合体整合多种信号包括氮信号来调节细胞生长。然而,越来越多的证据表明,TORC1介导的NCR控制只是部分的,这表明存在有待发现的补充调控过程。在这项工作中,我们开发了一种遗传筛选方法来寻找参与NCR信号传导的新因子。我们的数据表明,Gdh1的NADP - 谷氨酸脱氢酶活性负向调节NCR敏感基因的转录。通过测定氨基酸的总量、细胞质和液泡池中的氨基酸量,我们发现谷氨酰胺/谷氨酸储备与NCR程度之间没有正相关。虽然我们的数据表明谷氨酰胺可以作为NCR的初始触发因素,但它们表明谷氨酰胺不是维持阻遏的充分信号,并指出存在未知信号。我们的工作提供了更多将TORC1活性与NCR解偶联的证据,重新审视了NCR调控背后的教条。

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