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盘基网柄菌前柄细胞诱导因子DIF-1指导一种bZIP转录因子的磷酸化。

The Dictyostelium prestalk inducer DIF-1 directs phosphorylation of a bZIP transcription factor.

作者信息

Yamada Yoko, Kubohara Yuzuru, Kikuchi Haruhisa, Oshima Yoshiteru, Wang Hong-Yu, Ross Susan, Williams Jeffrey G

机构信息

College of Life Sciences, Welcome Trust Biocentre, University of Dundee, UK.

出版信息

Int J Dev Biol. 2013;57(5):375-81. doi: 10.1387/ijdb.130046jw.

DOI:10.1387/ijdb.130046jw
PMID:23873369
Abstract

DIF-1, a chlorinated hexaphenone produced by developing Dictyostelium cells, induces prestalk differentiation. DimB is a bZIP transcription factor that accumulates in the nucleus upon exposure to DIF-1, where it directly activates transcription of DIF-responsive genes. The signaling steps upstream of DimB and downstream of DIF-1 are entirely unknown. Analysis by mass spectrometry shows that incubation with DIF-1 rapidly stimulates phosphorylation at several sites in DimB. We characterize the most highly responsive site, S590, which is located very close to the C terminus. A point mutation in this site, S590A, does not inhibit DimB nuclear accumulation in response to DIF. However, this seems likely to reflect functional redundancy with other sites; because a panel of chemical variants on the structure of DIF-1 show a correlation between their potencies as inducers of DimB nuclear accumulation and their potencies as inducers of phosphorylation at S590. Furthermore, the S590A mutant is fully active in mutant rescue of a dimB null strain, arguing against an alternative role in transcriptional activation of target genes. We conclude that i) DIF-1 directs phosphorylation at S590, ii) although it is not essential for nuclear accumulation in response to DIF-1 correlative evidence, based upon a panel of DIF-1 related molecules, suggests that this modification may play a redundant role in the process. iii) We also present evidence that the kinase activity, which phosphorylates S590, is non-nuclear and that this signalling pathway is, in part at least, independent of the DIF-regulated STATc activation pathway.

摘要

DIF-1是发育中的盘基网柄菌细胞产生的一种氯化六苯酮,可诱导前柄细胞分化。DimB是一种bZIP转录因子,在暴露于DIF-1后会在细胞核中积累,在细胞核中它直接激活DIF反应基因的转录。DimB上游和DIF-1下游的信号传导步骤完全未知。质谱分析表明,与DIF-1孵育会迅速刺激DimB多个位点的磷酸化。我们鉴定了反应最强烈的位点S590,它位于非常靠近C末端的位置。该位点的点突变S590A并不抑制DimB对DIF的核积累反应。然而,这可能反映了与其他位点的功能冗余;因为一组DIF-1结构的化学变体显示,它们作为DimB核积累诱导剂的效力与其作为S590磷酸化诱导剂的效力之间存在相关性。此外,S590A突变体在dimB缺失菌株的突变体拯救中完全活跃,这与它在靶基因转录激活中的另一种作用相矛盾。我们得出以下结论:i)DIF-1指导S590的磷酸化;ii)尽管它对于响应DIF-1的核积累不是必需的,但基于一组与DIF-1相关的分子的相关证据表明,这种修饰可能在该过程中起冗余作用;iii)我们还提供证据表明,使S590磷酸化的激酶活性是非核的,并且这条信号通路至少部分独立于DIF调节的STATc激活通路。

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引用本文的文献

1
The Dictyostelium prestalk inducer differentiation-inducing factor-1 (DIF-1) triggers unexpectedly complex global phosphorylation changes.盘基网柄菌前柄细胞诱导物分化诱导因子-1(DIF-1)引发了意想不到的复杂全局磷酸化变化。
Mol Biol Cell. 2015 Feb 15;26(4):805-20. doi: 10.1091/mbc.E14-08-1319. Epub 2014 Dec 17.