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研究生: 林芳瑜
Lin, Fang-Yu
論文名稱: 克雷白氏肺炎桿菌CG43全基因體解序、抗酸轉錄體分析與尿素酶基因群功能探討
Whole Genome Sequencing, Transcriptome Analysis of Acid Response, and Urease Gene Cluster Characterization of Klebsiella pneumoniae CG43
指導教授: 張晃猷
Chang, Hwan-You
口試委員: 賴怡琪
Lai, Yi-Chyi
高茂傑
Kao, Mou-Chieh
學位類別: 碩士
Master
系所名稱: 生命科學暨醫學院 - 分子醫學研究所
Institute of Molecular Medicine
論文出版年: 2013
畢業學年度: 101
語文別: 中文
論文頁數: 66
中文關鍵詞: 克雷白氏肺炎桿菌基因體定序轉錄體尿素酶
外文關鍵詞: Klebsiella pneumoniae, genome sequence, transcriptome, urease
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    • 克雷白氏肺炎桿菌屬腸道菌科,為一伺機性病原菌,感染宿主後會導致肺炎、泌尿道感染、腦膜炎、菌血症、敗血症等。在台灣,克雷白氏肺炎桿菌是主要造成糖尿病病人肝膿瘍的病原。引發肝膿瘍之克雷白氏肺炎桿菌其莢膜血清型大多數是屬於 K1 和 K2。克雷白氏肺炎桿菌 CG43 是從台灣分離自肝膿瘍病患,毒性較強的 K2 血清型菌株。本研究中將克雷白氏肺炎桿菌 CG43 基因體完整解序,其長度為 5,166,857 bp,與克雷白氏肺炎桿菌 NTUH-K2044 和 克雷白氏肺炎桿菌 MGH 78578 相似度分別為 93 % 及 94 %。克雷白氏肺炎桿菌 CG43 有 203 個不同於 MGH 78578 與 NTUH-K2044 的基因。對於腸內菌而言,抗酸能力是非常重要的,我們藉由轉錄體定序分析克雷白氏肺炎桿菌 CG43在酸性環境時基因表現的情況,結果顯示有 4.94 % 基因被誘導,18.34 % 基因被抑制表現超過 2 倍,主要分別為伴隨蛋白及麥芽糖操縱子相關之基因。此外,在克雷白氏肺炎桿菌 CG43 中存有兩套尿素酶基因組,與大多數克雷白氏肺炎桿菌只具有一套尿素酶基因組不同。尿素酶可以將尿素分解成二氧化碳和氨,提供氮源並中和酸性環境,幫助細菌生存於酸性環境。本研究建構三種尿素酶突變株 (ΔureA1、ΔureA2 與 ΔureA1 ΔureA2)。我們發現 ΔureA1 和 ΔureA1 ΔureA2在以尿素取代氯化銨的 M9 培養基中的生長的情形稍差。以 Christensen’s Urea Agar 測定尿素酶活性,結果顯示ΔureA1 和 ΔureA1 ΔureA2 幾乎無尿素酶活性。此外,在酸性環境下,野生株和三種突變株 (ΔureA1、ΔureA2 和 ΔureA1 ΔureA2) 有相似的生長曲線。根據這些結果我們推測尿素酶對於克雷白氏肺炎桿菌 CG43 在一般培養條件下之耐酸能力並非重要因子。本研究所完成之完整的克雷白氏肺炎桿菌 CG43 基因體序列可以提供我們更多資訊以進一步探討其致病因子。

    Klebsiella pneumoniae is an important opportunistic pathogen that causes various human diseases such as pneumonia, urinary tract infection, meningitis, bacteremia and septicemia. In Taiwan, K. pneumoniae is the predominant pathogen responsible for pyogenic liver abscess in diabetic patients and K1 and K2 serotypes account for the majority of the isolates. K. pneumoniae CG43 was originally isolated from a patient with pyogenic liver abscess in Taiwan. It is a highly virulent K2 serotype strain. In this study, the whole genome sequence of K. pneumoniae CG43 was determined and annotated. The genome is 5,166,857 bp in length. The similarity of the CG43 genome sequence with that of K. pneumoniae NTUH-K2044 and MGH 78578 are 93 % and 94 %, respectively. K. pneumoniae CG43 has 203 open reading frames distinct from K. pneumoniae NTUH-K2044 and K. pneumoniae MGH 78578. Furthermore, because the ability of acid resistance is important for Enterobacteriaceae, we also performed transcriptome analysis of K. pneumoniae CG43 gene expression profile under acidic growth conditions. The data indicate that 4.94 % genes in CG43 genome were induced, while 18.34 % genes were repressed. Most of the up-regulated genes are associated with chaperone-related function and many of the down-regulated genes belong to maltose regulon. Besides, there are two urease gene clusters in K. pneumoniae CG43, different from most of K. pneumoniae that has only one urease gene cluster. Urease catalyzes the hydrolysis of the urea into carbon dioxide and ammonia. Besides providing nitrogen sources, the reaction can neutralize acidic environments, allowing pathogenic bacteria to survive the acidic conditions. Three types of urease mutant strains (ΔureA1, ΔureA2 and ΔureA1 ΔureA2) were constructed in CG43. Growth of ΔureA1 and ΔureA1 ΔureA2 double mutant was reduced in M9 minimal medium using urea as the sole nitrogen source. The two mutant strains lack urease activity as determined by Christensen’s Urea Agar. In addition, the growth of wild type and three urease mutant strains has no difference under acidic environment. The result suggests that urease is not a major factor contributing to acid tolerance of K. pneumoniae CG43 under normal cultural condition. To sum up, the complete CG43 genome sequence will provide critical information for future analysis of the virulence factors in the bacterium.

    中文摘要 I Abstract III 誌謝 V 縮寫字對照表 VII 目錄 VIII 表目錄 XI 圖目錄 XII 壹、 前言 1 貳、 材料與方法 6 2.1. 菌株、質體與生長環境 6 2.2. 染色體 DNA 萃取 6 2.3. 基因體定序、組裝、對應與填補 7 2.4. 基因體註解 7 2.5. 酸逆境處理 7 2.6. RNA萃取 8 2.7. 轉錄體 (transcriptome) 定序與分析 9 2.8. RNA 反轉錄反應 (reverse transcription) 9 2.9. 即時定量聚合酶連鎖反應 (real-time quantitative PCR) 10 2.10. 質體 DNA 萃取 10 2.11. 聚合酶連鎖反應 (Polymerase chain reaction,PCR) 11 2.12. 限制酵素處理 (digestion) 與接合作用 (ligation) 11 2.13. 製備勝任細胞 12 2.14. 熱休克轉型法 (heat shock transformation) 12 2.15. 構築 K. pneumoniae CG43 ureA1 與 ureA2 突變株 13 2.16. 細菌生長曲線測量 14 2.17. 尿素酶活性分析 14 2.18. 酸性環境下的生長曲線 15 參、 結果 16 3.1. K. pneumoniae CG43 基因體之特徵 16 3.2. 比較 K. pneumoniae CG43、K. pneumoniae MGH 78578 和 K. pneumoniae NTUH-K2044 所擁有基因之差異 16 3.3. 分析K. pneumoniae CG43 (K2) 之莢膜基因組組成並與 K. pneumoniae NTHU-K2044 (K1) 比較 17 3.4. K. pneumoniae CG43 纖毛基因組 17 3.5. 預測K. pneumoniae CG43 第六型分泌系統之基因組示意圖 18 3.6. 預測K. pneumoniae CG43 的酸適應島嶼基因組 19 3.7. K. pneumoniae CG43 在酸性環境下其基因表達情況 20 3.8. K. pneumoniae CG43 的兩套尿素酶基因組之第一個被轉錄基因,在經過酸處理後的表現量 21 3.9. 比對 K. pneumoniae 中 UreA 之相似度 21 3.10. 建構 ureA 基因缺損突變株 (ΔureA1、ΔureA2 與 ΔureA1 ΔureA2) 22 3.11. K. pneumoniae CG43 野生株 (WT) 與突變株 (ΔureA1、ΔureA2 與ΔureA1ΔureA2 之生長曲線與菌落型態 22 3.12. K. pneumoniae CG43 野生株 (WT) 與突變株 (ΔureA1、ΔureA2 與ΔureA1 ΔureA2) 尿素酶活性分析 23 3.13. K. pneumoniae CG43 野生株 (WT) 與突變株 (ΔureA1、ΔureA2 與ΔureA1 ΔureA2) 在酸性環境下的生長曲線 24 3.14. K. pneumoniae CG43 野生株 (WT) 與突變株 (ΔureA1、ΔureA2 與ΔureA1ΔureA2) 培養於有無添加尿素的 pH 4.4 LB 培養液,六小時後環境酸鹼值變化 24 肆、 討論 26 伍、 參考文獻 30 表目錄 表一、菌株與質體 40 表二、引子序列表 41 表三、比較K. pneumonia CG43、K. pneumoniae NTUH-K2044 和 K. pneumoniae MGH 78578 基因體特徵 42 表四、K. pneumoniae CG43、K. pneumoniae NTUH-K2044 和 K. pneumoniae MGH 78578 纖毛基因組的比較 43 表五、在轉錄體定序中,細菌生長於 pH 7與 pH 3 表現量相差兩倍的基因數量 44 表六、K. pneumoniae CG43 在 pH 3 環境中被誘導表現量最高的前 50 名基因 45 表七、K. pneumoniae CG43 在 pH 3 環境中被抑制表現量最高的前 50 名基因 47 表八、細菌在 pH 4.4 LB 培養 6 小時後上清液的 pH 值 50 圖目錄 圖一、K. pneumoniae CG43 基因體之圓形示意圖 51 圖二、K. pneumoniae CG43、K. pneumoniae NTUH-K2044 和 K. pneumoniae MGH 78578 所擁有基因之差異 52 圖三、比較 K. pneumoniae NTHU-K2044 (K1) 及 CG43 (K2) 之莢膜基因組組成 53 圖四、K. pneumoniae CG43 纖毛基因組示意圖 54 圖五、K. pneumoniae CG43 中所預測第六型分泌系統之基因組示意圖 55 圖六、K. pneumoniae CG43 染色體上預測的酸適應島嶼基因組 56 圖七、K. pneumoniae CG43 兩套尿素酶基因組之第一個被轉錄之基因,在經過酸處理後的表現量 57 圖八、比對K. pneumoniae CG43、K. pneumoniae K2044 和 K. pneumoniae MGH 78578中 UreA 之相似度 58 圖九、建構K. pneumoniae CG43 ΔureA (ureA1 與 ureA2) 突變株流程圖 59 圖十、利用聚合酶連鎖反應確認 K. pneumoniae CG43 ΔureA1、ΔureA2 與 ΔureA1 ΔureA2突變株 60 圖十一、K. pneumoniae CG43 野生株 (WT) 與突變株 (ΔureA1、ΔureA2 與ΔureA1 ΔureA2) 之生長曲線 62 圖十二、K. pneumoniae CG43 野生株 (WT) 與突變株 (ΔureA1、ΔureA2 與ΔureA1 ΔureA2) 在不同培養基的菌落型態 64 圖十三、檢測 K. pneumoniae CG43野生株 (WT) 與突變株 (ΔureA1、ΔureA2 與ΔureA1 ΔureA2) 的尿素酶活性 65 圖十四、比較 K. pneumoniae CG43野生株 (WT) 與突變株 (ΔureA1、ΔureA2 與 ΔureA1 ΔureA2) 在酸性條件的生長情形 66

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