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Possible dual regulatory circuits involving AtS6K1 in the regulation of plant cell cycle and growth

Authors
Shin, Yun-jeongKim, SunghanDu, HuiChoi, SoonyoungVerma, Desh Pal S.Cheon, Choong-Ill
Issue Date
May-2012
Publisher
KOREAN SOC MOLECULAR & CELLULAR BIOLOGY
Keywords
AtS6K1; auxin; phosphorylation; plant cell growth; TOR
Citation
MOLECULES AND CELLS, v.33, no.5, pp 487 - 496
Pages
10
Journal Title
MOLECULES AND CELLS
Volume
33
Number
5
Start Page
487
End Page
496
URI
https://scholarworks.sookmyung.ac.kr/handle/2020.sw.sookmyung/11922
DOI
10.1007/s10059-012-2275-4
ISSN
1016-8478
0219-1032
Abstract
The role of S6 Kinase 1 (AtS6K1), a downstream target of TOR kinase, in controlling plant growth and ribosome biogenesis was characterized after generating transgenic plants expressing AtS6K1 under auxin-inducible promoter. Down regulation of selected cell cycle regulatory genes upon auxin treatment was observed in the transgenic plants, confirming the negative regulatory role of AtS6K1 in the plant cell cycle progression reported earlier. Callus tissues established from these transgenic plants grew to larger cell masses with more number of enlarged cells than untransformed control, demonstrating functional implication of AtS6K1 in the control of plant cell size. The observed negative correlation between the expression of AtS6K1 and the cell cycle regulatory genes, however, was completely reversed in protoplasts generated from the transgenic plants expressing AtS6K1, suggesting a possible existence of dual regulatory mechanism of the plant cell cycle regulation mediated by AtS6K1. An alternative method of kinase assay, termed "substrate-mediated kinase pull down", was employed to examine the additional phosphorylation on other domains of AtS6K1 and verified the phosphorylation of both amino- and carboxy-terminal domains, which is a novel finding regarding the phosphorylation target sites on plant S6Ks by upstream regulatory kinases. In addition, this kinase assay under the stress conditions revealed the salt- and sugar-dependencies of AtS6K1 phosphorylations.
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