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標題: | α-AMYLASE3在阿拉伯芥葉澱粉代謝中功能之研究 Study on roles of AtAMY3 in Arabidopsis leaf starch metabolism |
作者: | Pei-Ching Lo 羅珮菁 |
指導教授: | 王淑美(Shue-Mei Wang) |
共同指導教授: | 陳枝乾(Jychain Chen) |
關鍵字: | α-澱粉水解酶,葉澱粉,AMY3,sex4,AMY3的胺端, α-amylase,leaf starch,AMY3,sex4,N-terminus of AMY3, |
出版年 : | 2011 |
學位: | 碩士 |
摘要: | 葉澱粉在白天合成於葉綠體中,而在晚上降解以供應植物體所需的糖分。在阿拉伯芥中,AMY3是唯一位於葉綠體內的α-澱粉水解酶。AMY3的胺端有葉綠體導引訊息及與GWD1 (GLUCAN WATER DIKINASE)胺端相似的區段,而在羧端有α-澱粉水解酶活性區段。在一多澱粉突變株sex4 (starch excess 4)中,AMY3的蛋白質含量及酵素活性相較於野生型植株有減少的現象,然而在RNA含量上卻無差異,顯示SEX4透過後轉錄修飾調控AMY3蛋白質穩定度。為了解AMY3在葉澱粉代謝中所扮演的角色及其與SEX4之間的關係,分別構築具有葉綠體導引訊息和AMY3胺端或羧端區段與螢光蛋白(EYFP)序列結合的載體,使其於植物體中表現,並進一步分析轉殖株的蛋白質、澱粉及醣類含量。實驗結果顯示,AMY3N-EYFP與AMY3C-EYFP皆可透由葉綠體導引訊息進入葉綠體,但只有AMY3C-EYFP具水解澱粉的活性。內生性AMY3之蛋白質含量在P35S:AMY3C-EYFP/Col和P35S:AMY3C-EYFP/sex4轉殖株中較之在野生型植株中略微減少,而其在P35S:AMY3N-EYFP/Col和P35S:AMY3N-EYFP/sex4轉殖株中卻有上升的現象。此外在P35S:AMY3C-EYFP/- P35S:AMY3N-EYFP/-和 P35S:AMY3C-EYFP/- P35S:AMY3N-EYFP/- sex4/sex4轉殖株中,內生性AMY3及AMY3N-EYFP蛋白質含量有不同的變化。這些結果顯示AMY3的胺端會受到SEX4影響,而其羧端可能會參與在AMY3蛋白質的降解調控機制中。另一方面,在P35S:AMY3C-EYFP/Col和P35S:AMY3C-EYFP/sex4轉殖株中,有澱粉含量下降和葡萄糖含量上升的現象,然而在P35S:AMY3N-EYFP/Col和P35S:AMY3N-EYFP/sex4轉殖株中卻無此現象,顯示AMY3的羧端在植物體中確實會參與葉澱粉的降解,但其水解澱粉的活性會受本身蛋白質的胺端影響。綜上而言,本研究指出AMY3的胺端可能為SEX4穩定AMY3蛋白質的作用區段且參與其自身蛋白質水解澱粉活性的調控。 The Arabidopsis AMY3 gene encodes a plastidial α-amylase with protein features including the chloroplast targeting peptide (TP), GWD1 N-terminal like domain (CBD) and α-amylase (AAD) domains expanding from its N- to C-terminus. Previous studies show that the expression of AMY3 is posttranscriptionally attenuated in a starch-excess mutant, sex4 (starch excess 4). To investigate the role of AMY3 in leaf starch metabolism and to clarify if AMY3 is regulated by its protein features through a SEX4 dependent mechanism, I generated constructs of P35S:AMY3N-EYFP and P35S:AMY3C-EYFP which would express recombinant proteins TP-CBD-EYFP (AMY3N-EYFP) and TP-AAD-EYFP (AMY3C-EYFP) in plant cells, respectively. Interestingly, the chlorotic and reticulate leaves, dwarf, and late-flowering phenotypes were found only in P35S:AMY3C-EYFP/Col and P35S:AMY3C-EYFP/sex4 plants. The amount of endogenous AMY3 protein in P35S:AMY3C-EYFP/Col and P35S:AMY3C-EYFP/sex4 plants was slightly lower than that of wild-type plants, whereas that of P35S:AMY3N-EYFP/Col and P35S:AMY3N-EYFP/sex4 plants was higher. Moreover, there were different changes in protein contents of AMY3 and AMY3N-EYFP in P35S:AMY3C-EYFP/- P35S:AMY3N-EYFP/- and P35S:AMY3C-EYFP/- P35S:AMY3N-EYFP/- sex4/sex4 plants. These results suggest that the N-terminus of AMY3 is the domain subject to the action of SEX4 and the C-terminus of AMY3 may play a role in AMY3 protein turnover. Reduced starch contents and increased glucose contents in the P35S:AMY3C-EYFP/Col and P35S:AMY3C-EYFP/sex4 lines compared to those of wild-type plants indicate that the C-terminal AAD of AMY3 involves in leaf starch degradation and its activity is confined by the N-terminus of AMY3. I hypothesize that the N-terminal domain of AMY3 may regulate AMY3 function by confining the amylolytic activity of the C-terminal catalytic domain and is the targeted domain for SEX4 regulation. |
URI: | http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/23580 |
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顯示於系所單位: | 植物科學研究所 |
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