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海洋产脂肪酶细菌对脂质降解的测定:脂肪酶活性测定的批判性评估

Determination of lipid degradation by marine lipase-producing bacteria: critical evaluation of lipase activity assays.

作者信息

Duflos Marie, Goutx Madeleine, Van Wambeke France

机构信息

Laboratoire de Microbiologie, Géochimie et Ecologie Marines, Centre d'Océanologie de Marseille, CNRS UMR 6117, Université de la Méditerranée, Campus de Luminy, 13288 Marseille Cedex 09, France.

出版信息

Lipids. 2009 Dec;44(12):1113-24. doi: 10.1007/s11745-009-3358-7. Epub 2009 Oct 23.

Abstract

With the aim of obtaining a better understanding of lipids-lipases interactions in bacterioplankton communities in oceans, we used different methods for measuring lipase activities in pure cultures of the marine strain Alteromonas macleodii. The decay of tripalmitate added to cultures was followed chemically over time. In an enzymatic approach, lipase activities were measured using the fluorogenic lipid analogs MUF-palmitate and ELF-palmitate. When hydrolyzed by lipase, the non-fluorescent substrates release MUF and ELF Alcohol (ELFA) which are fluorescent. As shown by spectrofluorometry, ELF-palmitate was an efficient competitor for MUF-palmitate. However, the activities reached using these two fluorogenic substrates were different, but still much higher than the tripalmitate hydrolysis rate, measured chemically. MUF- and ELF-palmitate would not be hydrolyzed by lipase sensu stricto (defined as triacylglycerol acylesterase E.C. 3.1.1.3) but rather reflects lipolytic activities in a broad sense. ELFA is also water-insoluble and theoretically precipitates in the external membrane of bacteria causing its hydrolysis, which would allow microscopic identification of active cells. By epifluorescence microscopy, the accumulation of ELFA fluorescence over time was detected (as large, diffuse halos), but no precipitates were clearly associated with bacteria on slide preparations, neither for pure cultures of Alteromonas macleodii nor for natural samples from the Bay of Marseille, France. Among possible biases, those related to the hydrophobic/hydrophilic conditions required for precipitation are discussed.

摘要

为了更好地理解海洋浮游细菌群落中脂质与脂肪酶的相互作用,我们采用了不同方法来测量海洋菌株麦克劳德氏交替单胞菌纯培养物中的脂肪酶活性。随着时间推移,通过化学方法追踪添加到培养物中的三棕榈酸酯的降解情况。在酶法中,使用荧光脂质类似物MUF-棕榈酸酯和ELF-棕榈酸酯测量脂肪酶活性。当被脂肪酶水解时,非荧光底物会释放出具有荧光的MUF和ELF醇(ELFA)。荧光分光光度法显示,ELF-棕榈酸酯是MUF-棕榈酸酯的有效竞争物。然而,使用这两种荧光底物测得的活性不同,但仍远高于化学测量的三棕榈酸酯水解速率。MUF-和ELF-棕榈酸酯不会被狭义的脂肪酶(定义为三酰甘油酰基酯酶E.C. 3.1.1.3)水解,而是在广义上反映脂解活性。ELFA也不溶于水,理论上会在细菌外膜中沉淀并导致其水解,这将有助于通过显微镜鉴定活性细胞。通过落射荧光显微镜,检测到ELFA荧光随时间的积累(呈现为大的、弥散的光晕),但在载玻片制备上,无论是麦克劳德氏交替单胞菌的纯培养物还是来自法国马赛湾的自然样本,都没有明显的沉淀物与细菌相关联。在可能的偏差中,讨论了与沉淀所需的疏水/亲水条件相关的偏差。

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