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离线固相萃取样品制备后植物细胞中核苷酸糖的定量高效液相色谱-质谱分析。

Quantitative HPLC-MS analysis of nucleotide sugars in plant cells following off-line SPE sample preparation.

作者信息

Behmüller Robert, Forstenlehner Ines C, Tenhaken Raimund, Huber Christian G

机构信息

Department of Molecular Biology, Division of Chemistry and Bioanalytics, University of Salzburg, Hellbrunner Straße 34, 5020, Salzburg, Austria.

出版信息

Anal Bioanal Chem. 2014 May;406(13):3229-37. doi: 10.1007/s00216-014-7746-3. Epub 2014 Mar 18.

Abstract

An analytical workflow was developed for the absolute quantification of uridine diphosphate (UDP)-sugars in plant material in order to compare their metabolism both in wild-type Arabidopsis thaliana and mutated plants (ugd2,3) possessing genetic alterations within the UDP-glucose dehydrogenase genes involved in UDP-sugar metabolism. UDP-sugars were extracted from fresh plant material by chloroform-methanol-water extraction and further purified by solid-phase extraction with a porous graphitic carbon adsorbent with extraction efficiencies between 80 ± 5 % and 90 ± 5 %. Quantitative determination of the UDP-sugars was accomplished through HPLC separation with a porous graphitic carbon column (Hypercarb(TM)) which was interfaced to electrospray ionization Orbitrap mass spectrometry. The problem of instable retention times due to redox processes on the stationary phase were circumvented by grounding of the column effluent and incorporation of a column regeneration procedure using acetonitrile-water containing 0.10 % trifluoroacetic acid. The method was calibrated using external calibration and UDP as internal standard. Calibration functions were approximated by first- or second-order regression analysis for concentrations spanning three orders of magnitude. Upon injecting sample volumes of 2.65 μL, the limits of detection for the UDP-sugars were in the 70 nmol L(-1) range. Six different UDP-sugars, including UDP-glucose, UDP-galactose, UDP-arabinose, UDP-xylose, UDP-glucuronic acid, and UDP-galacturonic acid were found in concentrations of 0.4 to 38 μg/g plant material. Data evaluation by analysis of variance (ANOVA) revealed statistically significant differences in UDP-sugar concentrations between wild-type and mutant plants, which were found to conclusively mirror the impaired metabolic pathways in the mutant plants.

摘要

为了比较野生型拟南芥和在参与尿苷二磷酸(UDP)-糖代谢的UDP-葡萄糖脱氢酶基因内具有基因改变的突变植物(ugd2,3)中UDP-糖的代谢情况,开发了一种用于绝对定量植物材料中UDP-糖的分析工作流程。UDP-糖通过氯仿-甲醇-水萃取从新鲜植物材料中提取,并进一步用多孔石墨化碳吸附剂进行固相萃取纯化,萃取效率在80±5%至90±5%之间。UDP-糖的定量测定通过使用多孔石墨化碳柱(Hypercarb(TM))的高效液相色谱分离来完成,该柱与电喷雾电离轨道阱质谱联用。通过将柱流出物接地并采用含0.10%三氟乙酸的乙腈-水进行柱再生程序,解决了固定相上氧化还原过程导致的保留时间不稳定问题。该方法使用外标法并以UDP作为内标进行校准。对于跨越三个数量级的浓度,校准函数通过一阶或二阶回归分析进行近似。进样体积为2.65 μL时,UDP-糖的检测限在70 nmol L(-1)范围内。在植物材料中发现了六种不同的UDP-糖,包括UDP-葡萄糖、UDP-半乳糖、UDP-阿拉伯糖、UDP-木糖、UDP-葡萄糖醛酸和UDP-半乳糖醛酸,浓度为0.4至38 μg/g。通过方差分析(ANOVA)进行数据评估,结果显示野生型和突变型植物中UDP-糖浓度存在统计学上的显著差异,这些差异最终反映了突变型植物中受损的代谢途径。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9e5c/3992224/1236ce3bd4a5/216_2014_7746_Figa_HTML.jpg

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