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  1. NTU Theses and Dissertations Repository
  2. 醫學院
  3. 生物化學暨分子生物學科研究所
請用此 Handle URI 來引用此文件: http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/45924
完整後設資料紀錄
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dc.contributor.advisor周綠蘋
dc.contributor.authorSheng-Yeh Chouen
dc.contributor.author周聖燁zh_TW
dc.date.accessioned2021-06-15T04:48:59Z-
dc.date.available2013-09-09
dc.date.copyright2010-09-09
dc.date.issued2010
dc.date.submitted2010-08-02
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dc.identifier.urihttp://tdr.lib.ntu.edu.tw/jspui/handle/123456789/45924-
dc.description.abstract過去的研究中,幽門螺旋桿菌已被證實會造成胃部的發炎,並且與許多胃部的疾病(胃炎、胃潰瘍、十二指腸潰瘍、胃癌等)有高度的關連性,在本實驗室先前的研究中,發現了幽門螺旋桿菌新的致病因子 GroES 蛋白,幽門螺旋桿菌的 GroES 蛋白會使得人類周邊血液單核
細胞釋放前發炎細胞激素(proinflammatory cytokines),這個現象可能與胃癌的形成有關。然而,相較於幽門螺旋桿菌的 GroES 蛋白,大腸桿菌的 GroES 蛋白並不會造成周邊血液單核細胞產生前發炎細胞激素,在比對幽門螺旋桿菌與其他微生物的 GroES 蛋白序列後,發現幽門螺旋桿菌的 GroES 蛋白在羧基端有 28 個胺基酸片段的延伸。有鑑於此,我們想探討此一片段對於幽門螺旋桿菌的致病性是否扮演重要的角色。我們表現全長之幽門螺旋桿菌 GroES 蛋白(H. p GroES)、刪除羧基端 28 個胺基酸之 H. p ΔGroES(1-90)蛋白,以及大腸桿菌之 GroES蛋白(E. coli GroES),並以試管內(In vitro)以及活體中(In vivo)實驗方法來探討這些蛋白的功能。在試管內的方法中,將三種 GroES 蛋白分別處理細胞後發現,不論是在人類周邊血液單核球、MKN45 細胞或是 THP-1 細胞中,都可以發現全長之 H.p GroES 蛋白會引發這些細胞高量的前發炎細胞激素介白素-8(Interkeukin 8, IL-8)表現,反觀經 H. p ΔGroES(1-90)以及 E.coli GroES 處理的組別,其介白素-8 的表現較 H.p GroES 蛋白處理的組別低。在活體中的方法中,我們使用斑馬魚當做模式生物,分別將這些種蛋白處理斑馬魚後,以定量聚合酶連鎖反應(Q-PCR)檢測這些組別其前發炎細胞激素的 mRNA 表現,結果顯示 H. p GroES 蛋白處理的組別中,其前發炎細胞激素介白素-1、介白素-8 相較其他蛋白處理組別有高量表現。接著使用原位核酸雜交法(In Situ Hybridization)染色觀察不同組別的切片後更進一步發現,H. p GroES 蛋白處理的組別,其前發炎細胞激素介白素-1、介白素-8 與腫瘤壞死因子 α(Tumor necrosis factorα, TNFα)RNA 高量表現於斑馬魚之消化系統區域,而在其他蛋白處理組別並無發現這樣的情況。綜合以上,幽門螺旋桿菌羧基端的 28 個胺基酸對於 H. p GroES 蛋白誘發前發炎細胞激素釋放扮演著重要的角色,也暗示 H. p GroES 蛋白,可能使胃上皮細胞及免疫細胞引發持續性發炎的情況。
zh_TW
dc.description.abstractHelicobacter pylori has been proven to cause stomach inflammation and many gastric diseases are highly related with H. pylori. In our previous study, we discovered a new H. pylori virulence factor—GroES protein. H. pylori GroES protein induces the peripheral blood mononuclear cells (PBMCs) release proinflammatory cytokines may be related to the formation of gastric cancer. However, E. coli GroES protein does not result in this phenomenon. Compared H. pylori with other microorganisms’ GroES protein sequence, revealed that the H. pylori GroES have the carboxyl extension of 28 amino acid fragment, and this fragment is unique to H. pylori was not found in other organisms. In view of this, it is necessary to disscuss how this fragment playing an important role in the pathogenicity of H. pylori. Recombinant proteins of full length H. p GroES (H. p GroES), removing the carboxyl 28 amino acids of the H. p GroES (H. p ΔGroES(1-90)), and E. coli GroES were prepared, using in vitro and in vivo methods to study function of these proteins. In in vitro methods, human PBMCs, MKN45 cells and THP-1 cells, had treated with three types of GroES protein, found that H. p GroES will lead to high levels of proinflammatory cytokine IL-8. In the cantrast, H. p ΔGroES(1-90) and E. coli GroES treatment groups had lower ability to induce IL-8 secretion in these cells. In in vivo approach, zebrafish were used as a model organism, dealing with these kinds of proteins in zebrafish. Using Q-PCR to analyze these groups of their mRNA expression showed that IL-1, IL-8 had high levels in H. p GroES treatment groups compared to control and other treatment groups. Performing In situ Hybridization to stain different groups of biopsy also discovered IL-1, IL-8 and TNF-α had higher RNA expression level at the digestive tract in zebrafish treated by H. p GroES. This phenomenon cannot be found in other treatment group. In summary, H. pylori Carboxyl 28 amino acids plays a key part in H. p GroES to induce the release of proinflammatory cytokines, and these results also suggested that H. pylori GroES protein may promote the gastric epithelial cells and immune cells inflammatory response.en
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dc.description.tableofcontents摘要 III
Abstract IV
縮寫 V
第一章 導論 10
第一節 幽門螺旋桿菌 10
1.1 幽門螺旋桿菌的形態與特徵 10
1.2 幽門螺旋桿菌之流行病學 10
1.3 幽門螺旋桿菌所造成之宿主反應 11
1.4 幽門螺旋桿菌的致病因子(virulence factors) 15
第二節 斑馬魚動物模型 20
2.1 斑馬魚的形態與特徵 20
2.2 以斑馬魚做為模式生物進行疾病研究 20
2.3 以斑馬魚做為模式生物進行免疫學研究 20
第三節 研究動機 21
第二章 材料與方法 22
第一節 材料 22
1.1 試藥 22
1.2 試劑組 24
1.3 各式溶液 25
1.4 重要儀器 30
1.4 重要耗材 31
第二節 實驗方法 32
2.1 幽門螺旋桿菌重組蛋白GroES(1-118)及ΔGroES(1-90)的表現與純化 32
2.2大腸桿菌重組蛋白GroES(1-90)的表現與純化 33
2.3 十二烷基磺酸鈉-聚丙醯胺凝膠電泳法(SDS-PAGE) 34
2.4 幽門螺旋桿菌GroES(1-118)與ΔGroES(1-90)及大腸桿菌重組蛋白GroES(1-90)處理細胞 35
2.5 酵素連結免疫吸附分析(Enzyme-Linked Immunosorbent Assay, ELISA) 37
2.6 以斑馬魚(Zebrafish)構築活體中GroES刺激免疫反應模型 38
2.7 使用原位核酸雜交染色法鑑定GroES蛋白處理斑馬魚(Zebrafish)後之免疫反應 42
第三章 結果 49
第一節 活體外實驗(In vitro experiment) 49
1.1幽門螺旋桿菌GroES蛋白與大腸桿菌GroES蛋白之表現與純化 49
1.2重組蛋白之內毒素測試 49
1.3幽門螺旋桿菌GroES蛋白誘導周邊血液單核球釋放前發炎細胞激素介白素-8 50
1.4幽門螺旋桿菌GroES蛋白誘導THP-1細胞釋放前發炎細胞激素介白素-8 50
1.5幽門螺旋桿菌GroES蛋白誘導MKN45細胞釋放前發炎細胞激素介白素-8 51
第二節 活體內實驗(In vivo experiment)-I 52
2.1以定量聚合酶鏈鎖技術證明幽門螺旋桿菌GroES蛋白誘導斑馬魚表現前發炎細胞激素基因 52
第三節 活體內實驗(In vivo experiment)-II 55
3.1質體構築與目標基因RNA探針製備 55
3.2以原位核酸雜交染色證明幽門螺旋桿菌GroES蛋白誘導斑馬魚消化道表現前發炎細胞激素基因 56
第四章 討論 58
第一節 幽門螺旋桿菌GroES蛋白誘導細胞釋放前發炎細胞激素介白素-8 59
第二節 幽門螺旋桿菌GroES蛋白誘導斑馬魚消化道前發炎細胞激素基因表現 61
第五章 結語 63
第六章 參考文獻 64
附圖與附表 71
附錄 85
dc.language.isozh-TW
dc.title幽門螺旋桿菌 GroES 蛋白在試管中及活體內誘發前發炎細胞
激素釋放
zh_TW
dc.titleHelicobacter pylori GroES induces proinflammatory responses
in vitro and in vivo
en
dc.typeThesis
dc.date.schoolyear98-2
dc.description.degree碩士
dc.contributor.oralexamcommittee張百恩,繆希椿,胡忠怡
dc.subject.keyword幽門螺旋桿菌,GroES,前發炎細胞激素,模式生物斑馬魚,zh_TW
dc.subject.keywordHelicobacter pylori,GroES,proinflammatory cytokines,Model organism Zebrafish,en
dc.relation.page88
dc.rights.note有償授權
dc.date.accepted2010-08-03
dc.contributor.author-college醫學院zh_TW
dc.contributor.author-dept生物化學暨分子生物學研究所zh_TW
顯示於系所單位:生物化學暨分子生物學科研究所

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