Ginies Christian, Brillard Julien, Nguyen-The Christophe
UMR408 SQPOV, Sécurité et Qualité des Produits d'Origine Végétale, INRA, Université d'Avignon.
UMR408 SQPOV, Sécurité et Qualité des Produits d'Origine Végétale, INRA, Université d'Avignon; UMR1333 DGIMI, INRA, Université de Montpellier;
J Vis Exp. 2016 Dec 5(118):54960. doi: 10.3791/54960.
The Bacillus species contain branched chain and unsaturated fatty acids (FAs) with diverse positions of the methyl branch (iso or anteiso) and of the double bond. Changes in FA composition play a crucial role in the adaptation of bacteria to their environment. These modifications entail a change in the ratio of iso versus anteiso branched FAs, and in the proportion of unsaturated FAs relative to saturated FAs, with double bonds created at specific positions. Precise identification of the FA profile is necessary to understand the adaptation mechanisms of Bacillus species. Many of the FAs from Bacillus are not commercially available. The strategy proposed herein identifies FAs by combining information on the retention time (by calculation of the equivalent chain length (ECL)) with the mass spectra of three types of FA derivatives: fatty acid methyl esters (FAMEs), 4,4-dimethyl oxazoline derivatives (DMOX), and 3-pyridylcarbinyl ester (picolinyl). This method can identify the FAs without the need to purify the unknown FAs. Comparing chromatographic profiles of FAME prepared from Bacillus cereus with a commercial mixture of standards allows for the identification of straight-chain saturated FAs, the calculation of the ECL, and hypotheses on the identity of the other FAs. FAMEs of branched saturated FAs, iso or anteiso, display a constant negative shift in the ECL, compared to linear saturated FAs with the same number of carbons. FAMEs of unsaturated FAs can be detected by the mass of their molecular ions, and result in a positive shift in the ECL compared to the corresponding saturated FAs. The branching position of FAs and the double bond position of unsaturated FAs can be identified by the electron ionization mass spectra of picolinyl and DMOX derivatives, respectively. This approach identifies all the unknown saturated branched FAs, unsaturated straight-chain FAs and unsaturated branched FAs from the B. cereus extract.
芽孢杆菌属含有支链和不饱和脂肪酸(FAs),其甲基支链(异或反异)和双键位置各不相同。脂肪酸组成的变化在细菌适应环境中起着关键作用。这些修饰导致异支链脂肪酸与反异支链脂肪酸的比例以及不饱和脂肪酸相对于饱和脂肪酸的比例发生变化,同时在特定位置形成双键。精确鉴定脂肪酸谱对于理解芽孢杆菌属的适应机制至关重要。许多来自芽孢杆菌的脂肪酸没有商业供应。本文提出的策略通过将保留时间信息(通过计算等效链长(ECL))与三种脂肪酸衍生物的质谱相结合来鉴定脂肪酸:脂肪酸甲酯(FAMEs)、4,4-二甲基恶唑啉衍生物(DMOX)和3-吡啶基甲醇酯(吡啶基)。该方法无需纯化未知脂肪酸即可鉴定脂肪酸。将蜡样芽孢杆菌制备的FAME的色谱图与商业标准混合物进行比较,可鉴定直链饱和脂肪酸,计算ECL,并对其他脂肪酸的身份进行假设。与具有相同碳原子数的线性饱和脂肪酸相比,异或反异支链饱和脂肪酸的FAME在ECL上呈现恒定的负向偏移。不饱和脂肪酸的FAME可通过其分子离子的质量检测到,与相应的饱和脂肪酸相比,其ECL会出现正向偏移。脂肪酸的支链位置和不饱和脂肪酸的双键位置可分别通过吡啶基和DMOX衍生物的电子电离质谱来鉴定。这种方法可鉴定蜡样芽孢杆菌提取物中的所有未知饱和支链脂肪酸、不饱和直链脂肪酸和不饱和支链脂肪酸。