Author
Listed:
- Jiaxu Li
(The Pennsylvania State University, 208 Mueller Laboratory
Harvard Medical School)
- Toshinori Kinoshita
(Kyushu University)
- Sona Pandey
(The Pennsylvania State University, 208 Mueller Laboratory)
- Carl K.-Y. Ng
(The Pennsylvania State University, 208 Mueller Laboratory)
- Steven P. Gygi
(Harvard Medical School)
- Ken-ichiro Shimazaki
(Kyushu University)
- Sarah M. Assmann
(The Pennsylvania State University, 208 Mueller Laboratory)
Abstract
Protein kinases are involved in stress signalling in both plant and animal systems. The hormone abscisic acid mediates the responses of plants to stresses such as drought, salinity and cold. Abscisic-acid-activated protein kinase (AAPK)—found in guard cells, which control stomatal pores—has been shown to regulate plasma membrane ion channels1. Here we show that AAPK-interacting protein 1 (AKIP1), with sequence homology to heterogeneous nuclear RNA-binding protein A/B, is a substrate of AAPK. AAPK-dependent phosphorylation is required for the interaction of AKIP1 with messenger RNA that encodes dehydrin, a protein implicated in cell protection under stress conditions. AAPK and AKIP1 are present in the guard-cell nucleus, and in vivo treatment of such cells with abscisic acid enhances the partitioning of AKIP1 into subnuclear foci which are reminiscent of nuclear speckles. These results show that phosphorylation-regulated RNA target discrimination by heterogeneous nuclear RNA-binding proteins2 may be a general phenomenon in eukaryotes, and implicate a plant hormone in the regulation of protein dynamics during rapid subnuclear reorganization.
Suggested Citation
Jiaxu Li & Toshinori Kinoshita & Sona Pandey & Carl K.-Y. Ng & Steven P. Gygi & Ken-ichiro Shimazaki & Sarah M. Assmann, 2002.
"Modulation of an RNA-binding protein by abscisic-acid-activated protein kinase,"
Nature, Nature, vol. 418(6899), pages 793-797, August.
Handle:
RePEc:nat:nature:v:418:y:2002:i:6899:d:10.1038_nature00936
DOI: 10.1038/nature00936
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