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Production of Rhamnolipids by Pseudomonas chlororaphis , a Nonpathogenic Bacterium. Nereus W. Gunther IV , Alberto Nuñez, William Fett and Daniel K.Y. Solaiman Applied And Environmental Microbiology 71 (2005) 2288-2293 報告學生:陳佳. Rhamnolipids. 生物介面活性劑 清潔除污性能
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Production of Rhamnolipids by Pseudomonas chlororaphis, a Nonpathogenic Bacterium Nereus W. Gunther IV , Alberto Nuñez, William Fett and Daniel K.Y. Solaiman Applied And Environmental Microbiology 71 (2005) 2288-2293 報告學生:陳佳
Rhamnolipids • 生物介面活性劑 • 清潔除污性能 • Pseudomonas aeruginosa、 Pseudomonas putida 皆具有致病力 (Anaissie, 1987、Macfarlane, 1991)
實驗流程 33株菌株接種至液態培養基 Minaeral salt-CTAB-methylene blue agar method觀察有無產生rhamnolipids 增加產量,以DCAT 11 tensiometer測量其表面張力 純化rhamnolipids TLC及HPLC/MS分析rhamnolipid種類 比較三菌株之rhamnolipid
菌株 • P. aeruginosa strains PG201, PG201-RhlA::Tn5, and NRRL B-800 • P. fluorescens strains ATCC 17397, ATCC 17824, ATCC 17577, and ATCC 17816 • P. chlororaphis strains ATCC 17812, NRRL B-14869, NRRL B-30761, and ATCC 9446 • P. putida strains ATCC 17527, W4P396, ATCC 17391, and ATCC 12633 • P. marginalis strains ATCC 10844 and HT041B • P. tolaasii strains ATCC 33618, ATCC 14340, C8, and C9 • P. syringae strain Cit7 • P. flavescens strain B62 • P. oleovorans strains NRRL B-778, NRRL B-14682, and NRRL B-14683 • P. resinovorans strain NRRL B-2649 • P. stutzeri strain ATCC 17588 • P. corrugata strains 388, ATCC 29756, and VC1-VC7 • Ralstonia eutropha strain • R. solanacearum strain
Kay’s minimal medium • Kay’s minimal medium(液態):0.3% NH4H2PO4, 0.2% K2HPO4, 0.2% glucose, 0.5mg/liter FeSO4, 0.1%MgSO4 • 培養條件:37℃,250 rpm
實驗流程 33株菌株接種至液態培養基 Minaeral salt-CTAB-methylene blue agar method觀察有無產生rhamnolipids 增加產量,以DCAT 11 tensiometer測量其表面張力 純化rhamnolipids TLC及HPLC/MS分析rhamnolipid種類 比較三菌株之rhamnolipid
Mineral salt-CTAB-methylene blue agar plate method • Mineral salts medium 添加 200μg/ml cetyltrimethylammonium bromide, 5 μg/ml methylene blue, and 1.5% agar • Mineral salts medium:per liter, 0.7g KH2PO4, 0.9g Na2HPO4,2g NaNO3, 0.4g MgSO4˙7H2O, 0.1g CaCl2‧2H2O, 2 ml of trace elements (per liter, 2g FeSO4 ,1.5g MnSO4‧H2O, 0.6g (NH4)6Mo7O24‧4H2O • 30 ℃下培養24~48小時 • 移至4℃下培養數天
glass pipette(10-ml )加熱 • 接種10-μl菌液
結果 • 陽離子介面活性劑及甲基藍與rhamnolipids結合呈藍紫色 • P. chlororaphis strain NRRL B-30761,30 ℃下呈現弱的正反應 • P. chlororaphis strain NRRL B-30761於4℃下仍呈正反應
實驗流程 33株菌株接種至液態培養基 Minaeral salt-CTAB-methylene blue agar method觀察有無產生rhamnolipids 增加產量,以DCAT 11 tensiometer測量其表面張力 純化rhamnolipids TLC及HPLC/MS分析rhamnolipid種類 比較三菌株之rhamnolipid
‧培養基表面積與體積比越大,產量 越高 ‧培養120小時,有最大產量 ‧23℃時,有最大產量
實驗流程 33株菌株接種至液態培養基 Minaeral salt-CTAB-methylene blue agar method觀察有無產生rhamnolipids 增加產量,以DCAT 11 tensiometer測量其表面張力 純化rhamnolipids TLC及HPLC/MS分析rhamnolipid種類 TLC及HPLC/MS分析rhamnolipid種類 比較三菌株之rhamnolipid
結果 • 將P. chlororaphis strain NRRL B-30761與市面販賣P.aeruginosa純化過的rhamnolipids做比較 • 不同分子的極性不相同 • TLC:P. chlororaphis的確具有rhamnolipids • HPLC: P. chlororaphis分泌的rhamnolipids無觀測到di-rhamnolipids
實驗流程 33株菌株接種至液態培養基 Minaeral salt-CTAB-methylene blue agar method觀察有無產生rhamnolipids 增加產量,以DCAT 11 tensiometer測量其表面張力 純化rhamnolipids TLC及HPLC/MS分析rhamnolipid種類 比較三菌株之rhamnolipid
結論 • 工業上以P. chlororaphis生產rhamnolipids可消除致病菌株產生毒性的問題 • 以glucose為碳源並改變萃取方式後P. chlororaphis最大rhamnolipids產量可達1 g/liter和P. aeruginosa利用glucose為碳源產量差不多(1.0至1.6 g/liter) • 靜置培養可節省能源