完整後設資料紀錄
DC 欄位語言
dc.contributor.author范家瑛en_US
dc.contributor.authorChia-Ying Fanen_US
dc.contributor.author李耀坤en_US
dc.contributor.authorYaw-Kuen Lien_US
dc.date.accessioned2014-12-12T01:20:55Z-
dc.date.available2014-12-12T01:20:55Z-
dc.date.issued2007en_US
dc.identifier.urihttp://140.113.39.130/cdrfb3/record/nctu/#GT009577505en_US
dc.identifier.urihttp://hdl.handle.net/11536/40021-
dc.description.abstractCBP21是一種幾丁質結合蛋白(chitin binding protein),來自於沙雷氏菌Serratia marcescens(革蘭氏陰性桿菌),當將 S. marcescens 培養於以幾丁質為碳源的培養液中,CBP21將隨著其他幾丁質酵素的分泌,而同時被分泌出來。CBP21由197個胺基酸組成,其N-端27個胺基酸為訊息胜肽(signal peptide)。近年來,研究人員發現CBP21具有破壞聚乙醯胺基葡糖直鏈結構的作用,憑藉CBP21的幫助,幾丁質酵素可以更有效地水解聚乙醯胺基葡糖。而在先期試驗中知道CBP21在pH 8.0條件下能與幾丁質結合,而在pH<7條件下便可以洗脫。因此,應可將其建構成純化蛋白質的工具或作為實行酵素固定化之用。利用此特性,吾人應用分生剪接(PCR)技術,將CBP21基因及在其下游續接連接肽(linker)、蛋白酶切位點(protease cut site)及限制酵素多重切點(MCS)等DNA序列,建構於pRSET A表達載體上,再於限制酵素MCS位置分別嵌入數種糖類水解酵素之基因,並將之轉殖入大腸桿菌表現細胞BL21(DE3)中進行表現。利用自製幾丁質細粒管柱進行純化,已成功純化得純度90 % 以上且回收率達40 % 以上的CBP21融合的標的蛋白質。zh_TW
dc.description.abstractCBP21 is a chitin-binding protein from Serratia marcescens, a Gram-negative soil bacterium. When S. marcescens is grown in the presence of chitin as a carbon source, CBP21 (197 amino acids, including a 27-residue leader peptide) is one of the major proteins produced and secreted along with other chitinases. In recent years, researchers have found that the non-catalytic CBP21 can bind to the insoluble crystalline substrate and lead to structural change of substrate. Consequently, CBP21 can increase the substrate accessibility and strongly promote the hydrolysis of crystalline β-chitin by other chitinases. Previous study also showed that CBP21 can bind on chitin at a pH value around 8.0 and can be eluted in acid condition (pH < 7). This feature is potentially useful for establishing a system for protein purification and for serving as a tool in enzyme immobilization. Through the application of PCR amplification, a DNA fragment containing the CBP21 gene, a downstream peptide-linker and a genease cut site was obtained. The fragment was successfully inserted into the pRSET_A expression vector. Several genes of glycoside hydrolases, including chitosanase, chitinase, and laminaripentaose-producing β-1,3-glucanase (LPHase), were inserted into the multiple cloning site of the constructed plasmid and further transformed into the E. coli BL21 (DE3) for fusion-protein expression. The capability of this system was then evaluated using β-form chitin as matrix for affinity-column purification. Results showed that proteins with high purity (> 90% homogeneity for all cases) were easily obtained. The recovery yield was more than 40 percent.en_US
dc.language.isozh_TWen_US
dc.subject幾丁質結合蛋白zh_TW
dc.subject幾丁質zh_TW
dc.subjectChitin Binding Proteinen_US
dc.subjectChitinen_US
dc.title幾丁質結合蛋白的應用zh_TW
dc.titleThe Applications of Chitin Binding Proteinen_US
dc.typeThesisen_US
dc.contributor.department理學院應用科技學程zh_TW
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