鼠李糖脂生物表面活性剂促进铜绿假单胞菌降解十六烷。

G S Shreve, S Inguva, S Gunnam
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引用次数: 0

摘要

利用铜绿假单胞菌产生和不产生鼠李糖脂生物表面活性剂的突变体,研究细胞相关生物表面活性剂对细胞与碳氢-水界面结合和碳氢吸收的影响。铜绿假单胞菌不产生鼠李糖脂的突变体65E12在没有外源添加表面活性剂的情况下,不能在以十六烷为碳源的最小培养基中生长。突变体PG201::rhlR在缺乏外源表面活性剂的情况下生长非常缓慢。这两个突变体都缺乏控制鼠李糖脂合成激活的正调控基因。65E12是一种双突变体,也缺乏脂多糖合成。然而,当少量纯化鼠李糖脂或合成阴离子表面活性剂烷基苯磺酸盐(ABS)添加到培养物中时,十六烷上的生长可以得到不同程度的恢复。鼠李糖脂生物表面活性剂在将烃类溶解到水相中方面的效果是合成阴离子表面活性剂ABS的9倍左右。描述了鼠李糖脂和ABS胶束的物理特性,通过激光散射来解释鼠李糖脂在溶解十六烷方面更有效的原因。在鼠李糖脂或合成ABS表面活性剂存在和不存在的情况下,研究了野生型和突变型菌株对碳氢化合物-水界面的细胞附着和细胞聚集。观察到的十六烷降解率的差异是根据乳化十六烷浓度、细胞表面疏水性和细胞在培养中的定位来解释的。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Rhamnolipid biosurfactant enhancement of hexadecane biodegradation by Pseudomonas aeruginosa.

Mutants of Pseudomonas aeruginosa that produce and do not produce rhamnolipid biosurfactant are used to investigate the influence of cell-associated biosurfactant on cellular association with the hydrocarbon-water interface and on hydrocarbon uptake. Rhamnolipid-nonproducing mutant 65E12 of P. aeruginosa is unable to grow in minimal media containing hexadecane as a carbon source in the absence of exogenously added surfactant. Mutant PG201::rhlR grows very slowly in the absence of exogenously added surfactants. Both mutants are deficient in the positive regulatory gene controlling the activation of rhamnolipid synthesis. 65E12 is a double mutant that is also deficient in lipopolysaccharide synthesis. However, growth on hexadecane may be restored to varying degrees when small amounts of purified rhamnolipids or the synthetic anionic surfactant alkyl benzene sulfonate (ABS) is added to the cultures. Rhamnolipid biosurfactant is shown to be approximately 9 times more effective than the structurally similar synthetic anionic surfactant ABS in solubilizing hydrocarbon into the aqueous phase. Physical characteristics of the rhamnolipid and ABS micelles as determined by laser light scattering are described to explain the greater effectiveness of the rhamnolipid in solubilizing hexadecane. The cellular attachment to hydrocarbon-water interfaces and cellular aggregation of the wild-type and mutant strains are examined in the presence and absence of rhamnolipid or synthetic ABS surfactants. Differences in observed hexadecane degradation rates are explained on the basis of emulsified hexadecane concentration, cell surface hydrophobicity, and cellular localization in the culture.

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