,Phosphorylation of WHIRLY1 by CIPK14 Shifts Its Localization and Dual Functions in Arabidopsis

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Plastid-to-nucleus retrograde signaling is critical for normal growth and development in plants.The dualfunction and dual-located ssDNA binding protein WHIRLY1 (WHY1) has been proposed to coordinate the retrograde signaling from plastids to the nucleus.However,the regulatory mechanism goveing the functional switch of WHY1 for mediating plastid-to-nucleus retrograde signaling remains unknown.Here,we report that the Calcineurin B-Like-Interacting Protein Kinase14 (ClPK14) interacts with and phosphorylates WHY1 in Arabidopsis.Phosphorylation of WHY1 results in increased accumulation in the nucleus and enhanced binding with the promoter of WRKY53,which encodes a key transcription factor regulating leaf senescence in Arabidopsis.Transgenic plants overexpressing ClPK14 showed an increased nuclear isoform but decreased plastid isoform of WHY1,among which 95% of transgenic lines showed the staygreen phenotype and 5% of lines showed the variegated pale-green phenotype.Interestingly,the phenotypes of both types of transgenic plants could be recovered by overexpression of plastid-form WHY1.In contrast,knockdown of ClPK14 caused early senescence and even seedling-lethal phenotypes along with elevated expression of senescence-related genes such as WRKY53,SAG12,and NDHF but decreased expression of MER11,RAD50,and POR genes,which could be rescued by overexpression of ClPK14 but not by overexpressing plastid-form or nuclear-form WHY1;the stay-green plants overexpressing ClPK14 showed reduced expression of WRKY53,SAG12,NDHF,and large plastid rRNA.Consistently,the accumulation of nuclear-form WHY1 was significantly reduced in the CIPK14 knockdown lines,resulting in a low ratio of nuclear-/plastid-form WHY1.Taken together,our results demonstrate that CIPK14 regulates the phosphorylation and organellar distributions of WHY1 and pinpoint that ClPK14 may function as a cellular switch between leaf senescence and plastid development for coordinating the intercellular signaling in Arabidopsis.
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