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使用高效阴离子交换色谱-脉冲安培检测法对包被链球菌中的细胞内糖磷酸酯和糖核苷酸进行定量分析。

Quantitative analysis of intracellular sugar phosphates and sugar nucleotides in encapsulated streptococci using HPAEC-PAD.

作者信息

Marcellin Esteban, Nielsen Lars K, Abeydeera Peter, Krömer Jens O

机构信息

Australian Institute for Bioengineering and Nanotechnology, University of Queensland, Brisbane, QLD, Australia.

出版信息

Biotechnol J. 2009 Jan;4(1):58-63. doi: 10.1002/biot.200800197.

Abstract

Metabolomics is a powerful tool for the study of biological systems. Besides analytical techniques, cell harvest and extraction are critical steps, especially when studying encapsulated streptococci. We have compared four different harvesting techniques for biomass from liquid culture of the hyaluronic acid (HA)-producing bacterium Streptococcus zooepidemicus. The best method for cell separation was quick (2 min) centrifugation, which allowed efficient medium removal and enabled quantification of the broadest range of sugar metabolites. Unlike observations for other microbes, changes in metabolite pools due to a delay of extraction by the centrifugation were not observed, so metabolite levels accurately reflected the metabolome at the point of cell harvest. A hypothesis is that the capsule itself isolates the cells from the surroundings and still supports it with nutrients during the harvest. Quantification of sugar phosphates and nucleotide sugars was performed using high-performance anion exchange chromatography combined with pulsed amperometric detection, achieving limits of quantification of 2.5 pmol for sugar phosphates and 5 pmol on column for nucleotide sugars. Intracellular pool sizes for intermediates of the HA pathway under production conditions ranged from 0.2 to 0.5 micromol/g cell dry weight.

摘要

代谢组学是研究生物系统的强大工具。除分析技术外,细胞收获和提取是关键步骤,尤其在研究包膜链球菌时。我们比较了四种从产透明质酸(HA)的兽疫链球菌液体培养物中收获生物质的不同技术。最佳的细胞分离方法是快速(2分钟)离心,这种方法能有效去除培养基,并能对最广泛的糖类代谢物进行定量。与其他微生物的观察结果不同,未观察到因离心提取延迟导致代谢物池的变化,因此代谢物水平准确反映了细胞收获时的代谢组。一种假设是,在收获过程中,荚膜本身将细胞与周围环境隔离开来,同时仍为细胞提供营养支持。使用高效阴离子交换色谱结合脉冲安培检测对糖磷酸盐和核苷酸糖进行定量,糖磷酸盐的定量限为2.5皮摩尔,核苷酸糖在柱上的定量限为5皮摩尔。在生产条件下,HA途径中间体的细胞内池大小范围为0.2至0.5微摩尔/克细胞干重。

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