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研究生: 龔文玫
Wen-Mei Kung
論文名稱: 人類重組磷酸二酯酶第五型(PDE5)酵素於大腸桿菌之表現研究
An expression study of recombinant human phosphodiesterase V (PDE5) in Escherichia coli
指導教授: 許宗雄 博士
Dr. Tzong-Hsiung Hseu
口試委員:
學位類別: 碩士
Master
系所名稱: 生命科學暨醫學院 - 生物科技研究所
Biotechnology
論文出版年: 2005
畢業學年度: 93
語文別: 中文
論文頁數: 72
中文關鍵詞: 人類磷酸二酯酶第五型高效液相層析儀犀利士冷休克表現質體
外文關鍵詞: PDE5, HPLC, Tadalafil, cGMP, Cold-shock expression vector
相關次數: 點閱:2下載:0
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    • 磷酸二酯酶 cyclic nucleotide phosphodiesterases (PDEs) 是由一群酵素所組成的superfamily,可以降解細胞內的二級訊息傳遞物 cyclic AMP(cAMP) 及cyclic GMP(cGMP) 。其中專一性的cGMP-binding cGMP-specific phosphodiesterase (PDE5) 存在於許多組織細胞中,可以降解cGMP並且調節細胞內cGMP的含量,其中也包括了陰莖海綿體的平滑肌細胞。著名的威而剛 (Sildenafil; Viagra)與 犀利士(Tadalafil; Cialis)是兩個主要的PDE5抑制劑,藉由抑制PDE5的活性使cGMP在海綿體的平滑肌細胞內堆積,促使平滑肌的放鬆造成充血及勃起。
    本實驗是將人類PDE5基因,包含N端融合蛋白質Thioredoxin整段轉殖到一冷休克表現質體,即為pCold-PDE5A。此表現質體經由轉型作用到E.coli strain BL21(DE3)中,並且在15℃下加入1mM IPTG後誘導24小時可得到大量表現的可溶性蛋白質。接著利用Ni2+-IDA 親和性管柱做蛋白質純化。而存在於不可溶包涵體的蛋白質則是利用on-column chemical refolding方法純化。本實驗利用一種簡單的reverse-phase HPLC儀器測定人類重組PDE5活性。利用此方法可以在15分鐘內測定受質 (cGMP)和反應產物(GMP),其偵測反應產物GMP的靈敏度約在2x10-11 moles。經由實驗結果發現純化後的人類重組PDE5蛋白質其Km值在1.12- 1.27uM。Tadalafil (Cialis)可以有效的抑制人類重組PDE5蛋白質的活性,其IC50 約為 39nM,而Ki値約為3.7 nM。但是由不可溶包涵體 (inclusion bodies)所純化出來的重組蛋白質則是偵測不到酵素活性。本實驗也利用HPLC建立了一個可以偵測兩種PDE5抑制劑 Sildenafil 和Tadalafil的方法。分析五種商業藥品對於PDE5的活性發現皆具有很強的抑制作用,經由HPLC分析也證實了其中包含了Sildenafil 或Tadalafil兩種PDE5抑制劑之一。

    Cyclic nucleotide phosphodiesterases (PDEs) are a superfamily of enzymes that degrade the intracellular secondary messengers cyclic AMP (cAMP) and cyclic GMP (cGMP). The cGMP-binding cGMP-specific phosphodiesterase (PDE5) degrades cGMP and regulates the intracellular level of cGMP in many tissues including the smooth muscle of the corpus cavernosum. Sildenafi (Viagra) and Tadalafil (Cialis) are two specific PDE5 inhibitors, promote penile erection by blocking PDE5 activity, which causes cGMP accumulation in the corpus cavernosum and trigger smooth muscle relaxation and increases blood flow.
    In this study, a cDNA of thioredoxin- human PDE5 fusion protein was inserted into a cold-shock expression vector, pCold-PDE5A. This plasmid was transformed into E.coli strain BL21(DE3) and the recombinant protein was induced with 1mM IPTG at 15℃ for 24 hours. The soluble fraction of the fusion protein was purified by Ni2+-IDA affinity column. A simple method based on reverse-phase HPLC has been development for measuring the activity of recombinant human PDE5 protein. It allows quantization of product (GMP) and substrate (cGMP) in less than 15 min, and the sensitivity of detection is as low as 2x10-11 moles of GMP. The Km value of soluble human recombinant PDE5 protein is 1.12- 1.27 uM. Tadalafil (Cialis) potently inhibited the recombinant PDE5 protein with IC50 values of 39 nM, and the Ki value is 3.7 nM. The protein from inclusion bodies was also purified by on-column chemical refolding processes. However, the activity of recombinant Trx-PDE5 protein from inclusion bodies was not detected. We also established a method based on HPLC to detect two PDE5 inhibitors, Sildenafil and Tadalafil. Five different commercial drugs shown great inhibition of PDE5 activity were subjected to HPLC analysis, and it revealed that all of them contain either Sildenafil or Tadalafil.

    中文摘要 ......................................................................................................................I 英文摘要 .................................................................................................................□II 第一章 前 言.........................................................................................................1 第二章 材料與方法 .................................................................................................6 2.1 藥品與材料…………………………………………………………………6 2.1.1一般化學藥品………………………………………………………..6 2.1.2 限制酶與實驗相關酵素…………………………………………….6 2.1.3 菌株及載體………………………………………………………….7 2.1.4蛋白質純化相關產品………………………………………………..7 2.2 實驗之儀器設備……………………………………………………………7 2.3 質體的來源與製備…………………………………………………………8 2.3.1 以氯化鈣法製備勝任細胞(competent cell preparation)………….8 2.3.2 人類磷酸二酯酶第五型(PDE5)基因來源………..............................8 2.3.3 聚合酶連鎖反應………………………………………………….....8 2.3.4 DNA洋菜膠電泳 (DNA agarose gel electrophoresis) ……………….9 2.3.5 聚合酶連鎖反應產物的純化……………………………………….9 2.3.6 DNA片段的磷酸化…………………………………………………10 2.3.7 載體DNA的製備…………………………………………………..10 2.3.8 載體DNA之回收與純化 (DNA recovery and purify)…………...…10 2.3.9 載體與DNA片段之接合 (DNA ligation) …………………………11 2.3.10 DNA轉型作用 (DNA transformation) …………………………….11 2.3.11小量質體DNA的抽取 (Mini-prep of plasmid DNA) ……….…….11 2.4親和性管柱的製備………………………………………………………....12 2.4.1樹脂的製備 ( Preparation of resin) …………………………..….…..12 2.4.2 親和性管柱分析試劑……………………………………………....12 2.4.3樹脂的再生 ( Regeneration of resin) ……………………………..…13 2.5 蛋白質的表現 (Protein expression) …………………………….…………...13 2.5.1小量蛋白質的誘導…………………………………….……………...13 2.5.2蛋白質聚丙醯胺膠體電泳 (SDS-PAGE) 之分析……………….…..14 2.5.3西方墨點法 (Western blot method) ……………..….…………..….....15 2.6 蛋白質的純化 (Protein purification) ……………………….……………….15 2.6.1蛋白質粗抽取液的製備(Preparation of protein clued extract) …….......15 2.6.2硫酸鎳金屬親和性管柱分析(Ni2+-affinity column chromatography)….16 2.6.3蛋白質的濃度定量………….………………………………………...16 2.6.4蛋白質的濃縮 ………….…………………………………………....17 2.6.5蛋白質的保存………….……………………………………………..17 2.7 On-Column Chemical Refolding of recombinant protein………….....……..…..17 2.8 PDE5酵素活性分析………….……………..……………………………….18 2.8.1酵素活性標準反應…….………………………………….…...……..18 2.8.2高效液相色層分析儀分析 (High Performance Liquid chromatography ; HPLC) ….……..…….…...18 2.8.3反應產物( GMP)的濃度定量………………………………………....18 2.8.4活性單位………………………………..…………………………......19 2.8.5 酵素動力學常數Km值的測定……………………………….……..19 2.8.6 Tadalafil (Cialis)對於酵素的抑制測定………...………………….…..19 2.8.7不同藥品對於酵素的抑制測定………...………………….………....20 2.9 HPLC分離PDE5抑制劑 Tadalafil 和 Sildenafil……..…………………....20第三章 實驗結果…………………………………….…………………….………21 3.1 重組質體的建構……………………………………………..…….……....21 3.1.1第一部份 (Thioredoxin-6HisTag) DNA片段的轉殖..…….……….....21 3.1.2第二部份 建構表現用的質體…………………..…….…………......22 3.2 蛋白質的表現與純化 ……..…….…………..............................................22 3.2.1人類重組磷酸二酯酶第五型(PDE5)的表現........................................22 3.2.2降低溫度增加可溶性蛋白質................................................................23 3.2.3比較不同溫度表現下蛋白質可溶性的情形........................................23 3.2.4利用西方墨點法觀察Trx-PDE5的表現 (Western blotting) .................24 3.2.5鎳離子親和性管柱 (Ni2+-IDA)純化可溶性重組蛋白質......................24 3.3 On-column chemical refolding of protein ........................................................25 3.4 酵素的活性測試及動力學分析..................................................................25 3.4.1反應產物( GMP)的標準曲線................................................................25 3.4.2 E coli BL21(DE3) 包含pColdIII質體的對照組實驗...........................26 3.4.3可溶性重組蛋白質Trx-PDE5酵素活性測定......................................26 3.4.4 On-column chemical refolding重組蛋白質的酵素活性測定................26 3.4.5 酵素動力學常數Km值與Vmax值....................................................27 3.5抑制劑與酵素的作用分析.............................................................................27 3.5.1 Tadalafil (Cialis) 對於Trx-PDE5酵素的抑制能力..............................27 3.5.2 酵素與抑制劑的Lineweaver-Burk plot ...............................................28 3.5.3 不同藥品對於Trx-PDE5酵素的抑制能力.........................................28 3.5.4 以HPLC分析藥品中PDE5抑制劑的存在.........................................29 第四章 討 論..........................................................................................................30 第五章 結 論..........................................................................................................37 圖 表............................................................................................................................38 參考文獻......................................................................................................................66

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