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  1. NTU Theses and Dissertations Repository
  2. 醫學院
  3. 生物化學暨分子生物學科研究所
請用此 Handle URI 來引用此文件: http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/44006
標題: Tyrosine磷酸化修飾對ROCKI活性調控之探討
Regulation of ROCKI by tyrosine phosphorylation
作者: Jheng-Guang Jhong
鍾政光
指導教授: 張智芬(Zee-Fen, Chang)
關鍵字: RhoA,ROCKI,c-Src,
出版年 : 2009
學位: 碩士
摘要: RhoA-regulated cell contractility plays important roles in variety of cellular
processes. Rho-associated coiled–coil kinase (ROCK) is one of the downstream
effectors of RhoA signaling and generates cell contraction force by promoting myosin
light chain (MLC) phosphorylation. Two isoforms of ROCK, ROCKI and ROCKII,
have been characterized. Previously, our laboratory has demonstrated that
RhoA-dependent ROCKII activation is negatively regulated by tyrosine
phosphorylation of ROCKII, which is controlled by c-Src and Shp2. In this study, I
investigated whether ROCKI activation is also regulated by tyrosine phosphorylation.
First, I detected tyrosine phosphorylation of ROCKI in HEK293T cells after
treatment with pervanadate, a phosphatase inhibitor, and this phosphorylation event
requires Src kinase. By expressing of dominant active SrcY527F and performing in
vitro assay with c-Src kinase, I demonstrated that c-Src phosphorylates ROCKI in
vivo and in vitro. Furthermore, I generated several deletion and YF substitution
mutants of flag-ROCKI, and found that Tyr913 residue is one of Src-mediated
phosphorylation sites of ROCKI. However, expression of flag-ROCKI(Y913F) had
little effect on nocodazole-stimulated RhoA-mediated MLC phosphorylation in
NIH3T3 cells, indicating that phosphorylation of Tyr913 may not participate in
negative regulation of ROCKI.
In summary, I may conclude that in addition to Tyr913, ROCKI has another
tyrosine phosphorylation sites, and the tyrosine phosphorylation on regulating ROCKI
activity should be investigated further.
URI: http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/44006
全文授權: 有償授權
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