淡江大學機構典藏:Item 987654321/51827
English  |  正體中文  |  简体中文  |  全文筆數/總筆數 : 64191/96979 (66%)
造訪人次 : 8221447      線上人數 : 7238
RC Version 7.0 © Powered By DSPACE, MIT. Enhanced by NTU Library & TKU Library IR team.
搜尋範圍 查詢小技巧:
  • 您可在西文檢索詞彙前後加上"雙引號",以獲取較精準的檢索結果
  • 若欲以作者姓名搜尋,建議至進階搜尋限定作者欄位,可獲得較完整資料
    •  進階搜尋


    請使用永久網址來引用或連結此文件: https://tkuir.lib.tku.edu.tw/dspace/handle/987654321/51827


    題名: 利用毛細管電泳探討dsDNA之異常電泳遷移行為
    其他題名: Study of anomalous electrophoretic migration of dsDNA by capillary electrophoresis
    作者: 許蘭婷;Hsu, Lan-ting
    貢獻者: 淡江大學化學學系碩士班
    吳俊弘;Wu, Chun-hung
    關鍵詞: 毛細管電泳;異常電泳遷移;雙股螺旋DNA;capillary electrophoresis;anomalous electrophoretic migration;dsDNA
    日期: 2010
    上傳時間: 2010-09-23 16:11:57 (UTC+8)
    摘要: 在本論文中我們開發了聚葡萄醣-毛細管電泳分析方法對dsDNA進行高解析分離,如此,我們可以偵測到DNA之間的微小電泳行為差異,進而探討dsDNA序列對其構型所造成的影響。
    根據文獻,DNA序列中含有A-track會使其構型產生彎曲,而導致DNA異常偏慢電泳遷移行為;而具有三重覆序列"CNG"的DNA因其構型較柔軟,會導致DNA異常偏快電泳遷移行為。我們計畫藉由此聚葡萄醣-毛細管電泳分析技術尋找其它可能導致DNA異常偏快電泳遷移的序列。
    我們以兩種限制酶(Hae III以及Alu I)分別對三種質體DNA(φx174、pBR322、pACPm)做切割(digest),所得六組DNA片段樣品兩兩混合成十三種組合樣品,再進行電泳分離實驗。將電泳結果以log(μ) (μ為DNA電泳遷移率)對log(1/bp) (bp為DNA鹼基對數目)作圖,依DNA大小分段進行線性廻歸而得到相關係數大於0.99以上的線性關係,電泳遷移行為與線性方程式吻合的DNA定義為正常電泳遷移DNA,電泳遷移率比其線性方程式預測值大者,定義為異常偏快電泳遷移DNA,若電泳遷移率比其線性方程式預測值較小者,則定義為異常偏慢電泳遷移DNA。我們在電泳緩衝溶液中添加不同濃度的溴化乙錠染料(EB),不同種類以及濃度的多價陽離子,或不同種類以及濃度的醣類,分析其對DNA異常遷移百分率的影響程度,探討DNA在不同環境下的構型改變,以及發現可能導致DNA異常電泳遷移行為的序列。根據本論文的實驗結果,我們歸納了幾種可能導致DNA異常偏快電泳行為的序列。
    In this thesis we have developed a Dextran-Capillary electrophoresis (Dextran-CE) based analytical method for the high resolution separation of dsDNA. In this way we are able to detect the minute difference in DNA electrophoretic migration behavior and furthermore to investigate the effect of DNA sequence on the DNA conformation.
    According to literatures, DNA sequence carrying A-tracks would result in bending conformation and cause anomalously slow electrophoretic migration behavior. On the other hand, DNA containing triplet repeat sequence “CNG” would have flexible conformation and thus shows anomalously rapid electrophoretic migration behavior. We plan to discover the other sequences which could lead to DNA anomalously rapid electrophoretic migration.
    Two restriction enzymes, Hae III and Alu I, were used to digest three plasmid DNAs, φx174, pBR322, and pACPm respectively, and every two of the subsequent six sets of restriction fragment samples were mixed to give 13 mixtures, which were then subjected to Dextran-CE separation experiments. The DNA base pair number (bp) and its corresponding measured electrophoretic mobility (μ) were plotted in the log(1/bp) versus log(μ) figure. Linear equations with correlation coefficients larger than 0.99 were obtained when we applied linear regression fittings to the data in different DNA size ranges. The DNA with electrophoretic mobility consisting with, larger than, or smaller than the linear prediction value was defined as normally, rapidly or slowly electrophoretic migrating DNA respectively. With the addition of different concentrations of ethidium bromide, various cations, or sacchrides into the CE run buffer and separation medium we were able to analyze their influences on the degree of DNA anomalous electrophoretic migration, to investigate the conformational change of DNA under different environments, and to discover the sequences which could induce the anomalous electrophoretic migration of DNA. According to the experimental results of the this thesis, we have inferred some DNA sequences which could possibly cause anomalous electrophoretic migration of DNA.
    顯示於類別:[化學學系暨研究所] 學位論文

    文件中的檔案:

    檔案 大小格式瀏覽次數
    index.html0KbHTML317檢視/開啟

    在機構典藏中所有的資料項目都受到原著作權保護.

    TAIR相關文章

    DSpace Software Copyright © 2002-2004  MIT &  Hewlett-Packard  /   Enhanced by   NTU Library & TKU Library IR teams. Copyright ©   - 回饋