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盘基网柄菌孢子囊中磷酸铵通过刺激渗透压感受器ACG促进孢子休眠。

Ammonium phosphate in sori of Dictyostelium discoideum promotes spore dormancy through stimulation of the osmosensor ACG.

作者信息

Cotter David A, Dunbar Andrew J, Buconjic Stanley D, Wheldrake John F

机构信息

Department of Biological Sciences, University of Windsor, 401 Sunset Avenue, Windsor, Ontario, Canada N9B 3P4.

School of Biological Sciences, The Flinders University of South Australia, Bedford Park, GPO Box 2100, Adelaide 5001, Australia.

出版信息

Microbiology (Reading). 1999 Aug;145 ( Pt 8):1891-1901. doi: 10.1099/13500872-145-8-1891.

Abstract

The sori of Dictyostelium discoideum (strains SG1, SG2, NC4 and V12) contained more than 100 mM ammonium phosphate. Glutamine synthetase (GS), which could remove ammonia from the sorus, was not present in 2-d-old dormant spores but enzyme activity returned to vegetative levels after spore germination. Based on mRNA blotting, the activity of this enzyme in germinating spores appeared to be transcriptionally controlled. At the same time that GS activity was increasing, ammonia was released from germinating spores. Exogenous ammonium ions at a concentration of 28 mM did not block germination nor modulate GS activity in nascent amoebae. It was concluded that the transcription and translation of GS is not environmentally regulated but is an integral part of the germination process, preparing nascent amoebae for vegetative growth. An exogenous concentration of 69 mM ammonium phosphate could maintain dormancy in spores of strains SG1 and SG2 for at least a week in the absence of any other inhibitory component from the sori. The inhibition was reversible at any time either by dilution or by washing the spores free of the ammonium ion. Spores of strain acg- were not inhibited by 100 mM ammonium phosphate. A model is presented in which GS in prespore cells serves as a sink for ammonia to allow the osmotically sensitive adenylyl cyclase aggregation protein (ACA) to activate protein kinase A (PKA) to induce fruiting-body formation. After fruiting-body formation is complete, the decline in GS and ACA activities in developing spores is offset by their replacement with the osmotically and ammonia-stimulated adenylyl cyclase osmosensor for germination (ACG). Ammonia and discadenine may act as separate signals to synergistically activate PKA by stimulating ACG activity while inhibiting cAMP phosphodiestrase activity in fully dormant spores.

摘要

盘基网柄菌(菌株SG1、SG2、NC4和V12)的孢子囊中含有超过100 mM的磷酸铵。谷氨酰胺合成酶(GS)可从孢子囊中去除氨,在2日龄的休眠孢子中不存在该酶,但孢子萌发后酶活性恢复到营养水平。基于mRNA印迹分析,该酶在萌发孢子中的活性似乎受转录调控。在GS活性增加的同时,氨从萌发的孢子中释放出来。浓度为28 mM的外源铵离子不会阻止萌发,也不会调节新生变形虫中的GS活性。得出的结论是,GS的转录和翻译不受环境调控,而是萌发过程的一个组成部分,为新生变形虫的营养生长做好准备。在没有孢子囊任何其他抑制成分的情况下,69 mM的外源磷酸铵浓度可使SG1和SG2菌株的孢子保持休眠至少一周。通过稀释或洗涤去除孢子中的铵离子,这种抑制在任何时候都是可逆的。acg-菌株的孢子不受100 mM磷酸铵的抑制。提出了一个模型,其中前孢子细胞中的GS作为氨的汇集点,使对渗透压敏感的腺苷酸环化酶聚集蛋白(ACA)激活蛋白激酶A(PKA)以诱导子实体形成。子实体形成完成后,发育中孢子中GS和ACA活性的下降被渗透压和氨刺激的腺苷酸环化酶萌发渗透传感器(ACG)所取代而抵消。氨和盘基网柄菌素可能作为单独的信号,通过刺激ACG活性同时抑制完全休眠孢子中的cAMP磷酸二酯酶活性来协同激活PKA。

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