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A High-Throughput Fatty Acid Profiling Screen Reveals Novel Variations in Fatty Acid Biosynthesis in Chlamydomonas reinhardtii and Related Algae

机译:高通量脂肪酸分析屏幕揭示了莱茵衣藻和相关藻类中脂肪酸生物合成的新变化。

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摘要

Analysis of fatty acid methyl esters (FAMEs) by gas chromatography (GC) is a common technique for the quantitative and qualitative analysis of acyl lipids. Methods for FAME preparation are typically time-consuming and labor-intensive and require multiple transfers of reagents and products between reaction tubes and autosampler vials. In order to increase throughput and lower the time and materials costs required for FAME preparation prior to GC analysis, we have developed a method in which 10-to-20-mg samples of microbial biomass are transferred to standard GC autosampler vials, transesterified using an emulsion of methanolic trimethylsulfonium hydroxide and hexane, and analyzed directly by GC without further sample handling. This method gives results that are essentially identical to those obtained by the more labor- and material-intensive FAME preparation methods, such as transmethylation with methanolic HCl. We applied this method to the screening of laboratory and environmental isolates of the green alga Chlamydomonas for variations in fatty acid composition. This screening method facilitated two novel discoveries. First, we identified a common laboratory strain of C. reinhardtii, CC-620, completely lacking all ω-3 fatty acids normally found in this organism and showed that this strain contains an inactivating mutation in the CrFAD7 gene, encoding the sole ω-3 desaturase activity in this organism. Second, we showed that some species of Chlamydomonas make Δ6-unsaturated polyunsaturated fatty acids (PUFA) rather than the Δ5 species normally made by the previously characterized laboratory strains of Chlamydomonas, suggesting that there is species-specific variation in the regiospecificity and substrate selectivity of front-end desaturases in this algal genus.
机译:通过气相色谱法(GC)分析脂肪酸甲酯(FAME)是用于酰基脂质定量和定性分析的常用技术。 FAME的制备方法通常很耗时且费力,并且需要在反应管和自动进样器样品瓶之间多次转移试剂和产物。为了增加通量并降低在进行GC分析之前进行FAME制备所需的时间和材料成本,我们开发了一种方法,其中将10至20 mg的微生物生物量样品转移到标准GC自动进样器样品瓶中,使用甲醇三甲基hydroxide氢氧化物和己烷的乳液,无需进一步处理即可直接通过GC进行分析。此方法产生的结果与通过费时费力和材料密集的FAME制备方法(例如用甲醇HCl进行甲基转移)获得的结果基本相同。我们将这种方法应用于绿藻衣藻的实验室和环境分离物中脂肪酸组成变化的筛选。这种筛选方法促进了两个新颖的发现。首先,我们鉴定了一种普通的实验室莱茵衣藻CC-620,完全缺乏该生物体中正常存在的所有ω-3脂肪酸,并表明该菌株在CrFAD7基因中含有失活突变,编码唯一的ω-3该生物中的去饱和酶活性。其次,我们表明某些衣藻物种会产生Δ6-不饱和多不饱和脂肪酸(PUFA),而不是以前表征的衣藻实验室菌株通常产生的Δ5物种,这表明该物种的区域特异性和底物选择性存在特定物种的差异。藻类中的前端去饱和酶。

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