Characterization of LIM domain only 7(LMO7), a mitotic phosphoprotein

碩士 === 慈濟大學 === 分子生物及細胞生物研究所 === 95 === Human LMO7, a nuclear membrane protein, has been shown to function as a transcription factor that can control expression of Emery-Dreifuss muscular dystrophy (EDMD) related genes. In our yeast two-hybrid screening, human LMO7 was identified to interact with th...

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Main Authors: Chih-Yun Chang, 張智雲
Other Authors: none
Format: Others
Language:zh-TW
Online Access:http://ndltd.ncl.edu.tw/handle/17897176970140540274
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spelling ndltd-TW-095TCU050610032015-10-13T14:16:32Z http://ndltd.ncl.edu.tw/handle/17897176970140540274 Characterization of LIM domain only 7(LMO7), a mitotic phosphoprotein 在細胞有絲分裂期的磷酸化蛋白質LMO7之分析 Chih-Yun Chang 張智雲 碩士 慈濟大學 分子生物及細胞生物研究所 95 Human LMO7, a nuclear membrane protein, has been shown to function as a transcription factor that can control expression of Emery-Dreifuss muscular dystrophy (EDMD) related genes. In our yeast two-hybrid screening, human LMO7 was identified to interact with the spindle checkpoint protein hMad1. We have generated and purified rabbit anti-LMO7 antibodies for the analysis. By in vitro binding assay, bacterially expressed hMad1 recombinant protein could interact with the purified hLMO7bFL recombinant protein that was expressed in insect cells. By the coimmunoprecipitation assay, we found endogenous hLMO7 could interact with endogenous hMad1 in the HeLa cells. We found that LMO7 protein levels were cell cycle-regulated and relatively low in late mitosis and early G1. Although LMO7 protein level did not fluctuate from S to M phase, LMO7 was phosphorylated in M phase but not in S phase. We have confirmed that endogenous hLMO7 or recombinant hLMO7bFL protein could be phosphorylated by PKA, Aurora A, GSK-3α, and GSK-3β but not by Aurora B and CyclinB1/Cdc2 in the in vitro assay and its possible phosphorylated residues were identified by the AP MALDI/MS. We propose that LMO7 phosphorylation was related to mitosis progression. none 莊育梩 學位論文 ; thesis 59 zh-TW
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language zh-TW
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description 碩士 === 慈濟大學 === 分子生物及細胞生物研究所 === 95 === Human LMO7, a nuclear membrane protein, has been shown to function as a transcription factor that can control expression of Emery-Dreifuss muscular dystrophy (EDMD) related genes. In our yeast two-hybrid screening, human LMO7 was identified to interact with the spindle checkpoint protein hMad1. We have generated and purified rabbit anti-LMO7 antibodies for the analysis. By in vitro binding assay, bacterially expressed hMad1 recombinant protein could interact with the purified hLMO7bFL recombinant protein that was expressed in insect cells. By the coimmunoprecipitation assay, we found endogenous hLMO7 could interact with endogenous hMad1 in the HeLa cells. We found that LMO7 protein levels were cell cycle-regulated and relatively low in late mitosis and early G1. Although LMO7 protein level did not fluctuate from S to M phase, LMO7 was phosphorylated in M phase but not in S phase. We have confirmed that endogenous hLMO7 or recombinant hLMO7bFL protein could be phosphorylated by PKA, Aurora A, GSK-3α, and GSK-3β but not by Aurora B and CyclinB1/Cdc2 in the in vitro assay and its possible phosphorylated residues were identified by the AP MALDI/MS. We propose that LMO7 phosphorylation was related to mitosis progression.
author2 none
author_facet none
Chih-Yun Chang
張智雲
author Chih-Yun Chang
張智雲
spellingShingle Chih-Yun Chang
張智雲
Characterization of LIM domain only 7(LMO7), a mitotic phosphoprotein
author_sort Chih-Yun Chang
title Characterization of LIM domain only 7(LMO7), a mitotic phosphoprotein
title_short Characterization of LIM domain only 7(LMO7), a mitotic phosphoprotein
title_full Characterization of LIM domain only 7(LMO7), a mitotic phosphoprotein
title_fullStr Characterization of LIM domain only 7(LMO7), a mitotic phosphoprotein
title_full_unstemmed Characterization of LIM domain only 7(LMO7), a mitotic phosphoprotein
title_sort characterization of lim domain only 7(lmo7), a mitotic phosphoprotein
url http://ndltd.ncl.edu.tw/handle/17897176970140540274
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AT zhāngzhìyún zàixìbāoyǒusīfēnlièqīdelínsuānhuàdànbáizhìlmo7zhīfēnxī
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