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http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/75911| Title: | 純化及鑑定負向調節AGP基因表現的轉錄因數 Purification And Characterization Of A Negative Transcription Factor For α 1-Acid Glycoprotein Gene Expression |
| Authors: | Wen-Hai Tsai 蔡文海 |
| Publication Year : | 1992 |
| Degree: | 碩士 |
| Abstract: | 近幾年來本實驗室研究老鼠肝臟的α l-Acid Glycoprotein ( AGP )基因表現之調控機制,此基因啟動子 ( promoter )的鹼基序列 -180/+10 之間,包括五個主要序列,分別為A,B,C,D及E。同時也鑑定出幾 個轉錄因數,其中之一AGP/EBP可以結合到A,C,D,E四個序列,加強AGP基因的表現,而另一方面B序列經 特異位置突變( site-directed mutagenesis )及功能性分析 ( functional assays )已確定其為一負向序 列( negative element )。 本篇論文主要就是應用傳統的生物化學方法,將肝臟細胞的核萃取液通過離子交換層析管柱及DNA親和性層 析管柱,藉以純化和B序列相結合,且具有負向調節效果的轉錄因數AGP/NTF。此因數對熱大致穩定,經 south–western blot的分析,發現至少有六個多勝?,其中分子量45一66kDa之間,具有主要結合B序列的活性。 α 1-acid glycoprotein (AGP) is an acute-responsive, 1iver-specific gene. Its expression is regulated by both positive and negative trans-acting factors. At least five cis-e1ements have been identified within the 180 bp region of AGP promoter. Four of these sites, A, C, D and E are recognized by AGP/EBP or AGP/EBP-like factors in liver nuclear extracts. Site-directed mutagenesis and trasfection analysis indicate that A, C, D and E regions are positive regulatory elements enhancing the expression of AGP gene while B motif is a negative regu1atory element repressing the expression of AGP gene. We have purified several proteins that bind to the B region in the AGP gene promoter. These proteins were purified from rat liver nuclear extracts by chromatography on heparin-agarose and oligonucleotide affinity columns. Analysis of purified protein fractions by southwestern blot reveals more than six polypeptides having binding activity to B motif. The purified protein from each fraction was recovered from SDS-PAGE, and those of the molecular size ranging from 45 to 66 kDa were demonstrated to have major binding activity toward B region of the AGP promoter. |
| URI: | http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/75911 |
| Fulltext Rights: | 未授權 |
| Appears in Collections: | 生化科學研究所 |
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