提升BsPPS安定性應用於天然多酚磷酸化之研究

陳聖東; Sheng-Dong Chen

請用此 Handle URI 來引用此文件： http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/101685

完整後設資料紀錄

DC 欄位	值	語言
dc.contributor.advisor	蘇南維	zh_TW
dc.contributor.advisor	Nan-Wei Su	en
dc.contributor.author	陳聖東	zh_TW
dc.contributor.author	Sheng-Dong Chen	en
dc.date.accessioned	2026-02-26T16:42:15Z	-
dc.date.available	2026-02-27	-
dc.date.copyright	2026-02-26	-
dc.date.issued	2026	-
dc.date.submitted	2026-01-28	-
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dc.identifier.uri	http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/101685	-
dc.description.abstract	多酚類磷酸酯合成酶(Phenolic phosphate synthetase, BsPPS)為本實驗室先前鑑定出之新穎雙激酶，能以ATP作為磷酸供體進行多酚類化合物之磷酸酯化反應，其磷酸酯產物展現出顯著之水溶性與生物可利用率提升。BsPPS具廣泛之基質催化能力，涵蓋黃酮類、查耳酮、二苯乙烯類、薑黃素類、蒽醌類、香豆雌酚類以及香豆素類等近40種化合物，顯示其在天然物磷酸酯化合物開發上的高度潛力。本實驗室先前以BsPPS搭配ATP再生酵素ErPPK建立一套耦合雙酵素多酚類磷酸酯轉化系統，實際應用於木犀草素磷酸酯之合成。然而兩者最適催化溫度及安定性之差異使該系統受限於37°C下操作。有鑒於此，本研究嘗試透過定向演化(directed evolution)與理性設計(rational design)之蛋白質工程策略提升BsPPS之熱安定性，並降低熱安定性與催化活性取捨(trade-off)。期望獲得一株兼具良好熱安定性與催化活性之BsPPS突變株，進一步拓展該耦合雙酵素系統於高溫操作條件下之應用潛力，並提升整體磷酸酯化之效能。實驗第一部分我們首先針對定向演化之實務需求，以具螢光特性之umbelliferone (UMB)建立一套具高靈敏度與再現性之高通量活性篩選平台。實驗證實BsPPS可於UMB之7-OH位點進行單磷酸酯化，生成umbelliferone 7-O-phosphate (U7P)，其結構由LC-ESI-MS/MS與1H-31P HSQC NMR鑑定。由於磷酸酯化後U7P無法去質子化，而可藉由螢光減少量推估BsPPS磷酸酯化活性。實驗第二部分系統性評估最適UMB螢光量測條件，確立於pH 7.5、50% (v/v)甲醇環境下，以360/460 nm作為激發/放射波長進行螢光之量測。所建立之螢光定量方法於1~5 µM範圍內具良好線性(R² = 0.994)，且在同日間與異日間分析中皆展現良好準確度與精密度(CV < 10%)。基質效應測試亦顯示反應體系中ATP、Mg²⁺與DMSO等成分不會對螢光訊號造成干擾。實驗第三部分結合該平台，建構一套完整之BsPPS定向演化流程，涵蓋error-prone PCR隨機突變庫建立、96孔盤突變株重組蛋白表現、粗酵素液製備與突變株篩選。於低突變率條件下建立之突變庫大小約為2.82 × 10⁴ transformants，突變率為3.48 mutations/kb。透過優化lysozyme破菌條件，並評估孔間變異與流程重複性，確認該平台具良好之再現性，並已累計篩選3,360株突變株。	zh_TW
dc.description.abstract	Phenolic phosphate synthetase (BsPPS) is a novel dikinase previously identified by our lab that catalyzes the phosphorylation of polyphenolic compounds using ATP as the phosphate donor. The phosphorylated polyphenol exhibit significantly improved solubility and bioavailability. In addition, BsPPS displays broad substrate promiscuity, catalyzing the phosphorylation of flavonoids, chalcones, curcuminoids, anthraquinones, coumestans and coumarins up to 40 different polyphenolic compounds, highlighting its potential for the development of phosphate prodrugs derived from natural products. Previously, our lab established a coupled bienzymatic polyphenol phosphorylation system by combining BsPPS with an ATP regeneration enzyme, ErPPK, and successfully applied to the synthesis of luteolin phosphate. However, due to the distinct optimal catalytic temperatures and thermostability of BsPPS and ErPPK, the coupled system is currently restricted to operation at 37°C. To address this limitation, our study aimed to enhance the thermostability of BsPPS through directed evolution and rational design strategies, while minimizing the trade-off between stability and catalytic activity, in order to obtain a mutant with improved stability and retained enzymatic function. In the first part of this study, a high-throughput activity screening platform was established, using the fluorescent substrate umbelliferone (UMB). Experimental results demonstrated that BsPPS catalyzes the phosphorylation of UMB at the 7-OH position to form umbelliferone 7-O-phosphate (U7P), whose structure was confirmed by LC-ESI-MS/MS and 1H–31P HSQC NMR analyses. Phosphorylation at the 7-OH position suppresses deprotonation of UMB, resulting in a pronounced decrease in fluorescence intensity, which enables quantification of BsPPS activity based on fluorescence reduction. In the second part, the fluorescence measurement conditions for UMB were optimized. Optimal conditions were determined to be pH 7.5 in 50% (v/v) methanol, with excitation and emission wavelengths at 360 and 460 nm, respectively. The established fluorescence assay exhibited good linearity over a concentration range of 1–5 µM (R² = 0.994), as well as satisfactory accuracy and precision in both intra-day and inter-day analyses (CV < 10%). Matrix effect tests further confirmed that ATP, Mg²⁺, and DMSO present in the reaction system did not affect the fluorescence signal. In the third part, the screening platform was integrated to construct a directed evolution workflow for BsPPS, using error-prone PCR to generate the mutant library, recombinant protein expression in 96-well plates, crude enzyme preparation, and mutant screening. Under low mutation-rate conditions, a mutant library of approximately 2.82 × 10⁴ transformants was established, with an average mutation rate of 3.48 mutations/kb. Following optimization of cell lysis conditions and evaluation of variability and process reproducibility, the platform was confirmed to be robust and reliable, enabling the screening of a total of 3,360 mutants.	en
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dc.description.tableofcontents	謝辭 I 中文摘要 III Abstract V 目次 VII 圖次 X 表次 XII 縮寫表 XIII 第一章前言 1 第二章文獻回顧 2 第一節多酚類化合物 2 1.1 多酚類簡介 2 1.2 多酚類之生理活性 5 1.3 多酚類化合應用之限制 5 第二節磷酸化之應用 7 2.1 磷酸酯前驅藥物(Phosphate Prodrug) 7 2.2 類黃酮之微生物磷酸酯化 9 2.3 微生物磷酸酯化之限制 11 第三節多酚類磷酸酯合成酶 13 3.1 生化特性 13 3.2 催化機制 14 3.3 基質範圍(Substrate scope) 16 3.4 pH-stat ATP再生之耦合雙酵素系統生產平台 17 3.5 耦合雙酵素系統面臨之限制 18 第四節蛋白質熱安定性 20 4.1 熱安定性之重要性 20 4.2 影響熱安定性之分子本質 21 第五節蛋白質工程(protein engineering)策略 24 5.1 定向演化(Directed evolution) 24 第三章材料與方法 28 第一節實驗大綱 28 第二節實驗材料 29 1. 菌株 29 2. 培養基 29 3. 緩衝液 30 4. 多酚類基質 30 5. 試藥與溶劑 30 6. 分生試劑 31 7. 蛋白質實驗試劑 32 第三節實驗設備及儀器 33 第四節實驗方法 35 1. 篩選適用於快速測定BsPPS活性之基質 35 2. 以UMB螢光法建立高通量BsPPS活性快篩平台 40 3. 結合error-prone PCR與螢光高通量篩選之定向演化流程建構 43 第四章結果與討論 50 第一節篩選適用於高通量活性測定平台建立之基質 50 1.1 以BsPPS單磷酸酯化UMB能力測試 52 1.2 U1之結構鑑定 53 1.3 UMB及U7P螢光強度分析 57 1.4 UMB對BsPPS催化活性影響評估 57 第二節建立UMB螢光高通量BsPPS活性快篩平台 59 2.1 最適UMB螢光測量條件 59 2.2 最適激發波長及放射波長之選擇 61 2.3 UMB螢光－濃度檢量線之建立 61 2.4 螢光定量方法之確效試驗 62 2.5 基質效應測試 64 2.6 最適基質反應濃度 65 第三節結合error-prone PCR與螢光高通量篩選之定向演化流程建構 67 3.1 以error-prone PCR建立隨機突變庫 67 3.2 建立96孔盤重組蛋白表現及粗酵素液製備流程 69 3.3 粗酵素液中內源性蛋白之背景影響評估 70 3.4 Lysozyme最適破菌條件 71 3.5 高通量快篩流程孔間變異以及重複性之評估 72 3.6 BsPPS之error-prone PCR突變株篩選 73 第五章結論 75 第六章參考文獻 76 第七章附錄 83	-
dc.language.iso	zh_TW	-
dc.subject	多酚類磷酸酯合成酶	-
dc.subject	蛋白質工程	-
dc.subject	熱安定性	-
dc.subject	定向演化	-
dc.subject	高通量篩選	-
dc.subject	Phenolic phosphate synthetase	-
dc.subject	protein engineering	-
dc.subject	thermostability	-
dc.subject	directed evolution	-
dc.subject	high-throughput screening	-
dc.title	提升BsPPS安定性應用於天然多酚磷酸化之研究	zh_TW
dc.title	Enhancing the Stability of BsPPS for the Phosphorylation of Natural Polyphenols	en
dc.type	Thesis	-
dc.date.schoolyear	114-1	-
dc.description.degree	碩士	-
dc.contributor.oralexamcommittee	羅翊禎;方翠筠;林曉青;陳曄	zh_TW
dc.contributor.oralexamcommittee	Yi-Chen Lo;Tsuei-Yun Fang;Hsiao-Ching Lin;Yeh Chen	en
dc.subject.keyword	多酚類磷酸酯合成酶,蛋白質工程熱安定性定向演化高通量篩選	zh_TW
dc.subject.keyword	Phenolic phosphate synthetase,protein engineeringthermostabilitydirected evolutionhigh-throughput screening	en
dc.relation.page	87	-
dc.identifier.doi	10.6342/NTU202600283	-
dc.rights.note	未授權	-
dc.date.accepted	2026-01-29	-
dc.contributor.author-college	生物資源暨農學院	-
dc.contributor.author-dept	農業化學系	-
dc.date.embargo-lift	N/A	-
顯示於系所單位：	農業化學系

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