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植物13C代谢通量分析中的特定区室标记信息

Compartment-specific labeling information in 13C metabolic flux analysis of plants.

作者信息

Allen Doug K, Shachar-Hill Yair, Ohlrogge John B

机构信息

Department of Plant Biology, Michigan State University, East Lansing, MI 48824, USA.

出版信息

Phytochemistry. 2007 Aug-Sep;68(16-18):2197-210. doi: 10.1016/j.phytochem.2007.04.010. Epub 2007 May 25.

DOI:10.1016/j.phytochem.2007.04.010
PMID:17532016
Abstract

Metabolic engineering of plants has great potential for the low cost production of chemical feedstocks and novel compounds, but to take full advantage of this potential a better understanding of plant central carbon metabolism is needed. Flux studies define the cellular phenotype of living systems and can facilitate rational metabolic engineering. However the measurements usually made in these analyses are often not sufficient to reliably determine many fluxes that are distributed between different subcellular compartments of eukaryotic cells. We have begun to address this shortcoming by increasing the number and quality of measurements that provide (13)C labeling information from specific compartments within the plant cell. The analysis of fatty acid groups, cell wall components, protein glycans, and starch, using both gas chromatography/mass spectrometry and nuclear magnetic resonance spectroscopy are presented here. Fatty acid labeling determinations are sometimes highly convoluted. Derivatization to butyl amides reduces the errors in isotopomer resolution and quantification, resulting in better determination of fluxes into seed lipid reserves, including both plastidic and cytosolic reactions. While cell walls can account for a third or more of biomass in many seeds, no quantitative cell wall labeling measurements have been reported for plant flux analysis. Hydrolyzing cell wall and derivatizing sugars to the alditol acetates, provides novel labeling information and thereby can improve identification of flux through upper glycolytic intermediates of the cytosol. These strategies improve the quantification of key carbon fluxes in the compartmentalized flux network of plant cells.

摘要

植物的代谢工程在低成本生产化学原料和新型化合物方面具有巨大潜力,但要充分利用这一潜力,需要更好地理解植物中心碳代谢。通量研究定义了生命系统的细胞表型,并有助于合理的代谢工程。然而,这些分析中通常进行的测量往往不足以可靠地确定真核细胞不同亚细胞区室之间分布的许多通量。我们已开始通过增加测量的数量和质量来解决这一缺点,这些测量提供来自植物细胞内特定区室的(13)C标记信息。本文介绍了使用气相色谱/质谱和核磁共振光谱对脂肪酸基团、细胞壁成分、蛋白质聚糖和淀粉的分析。脂肪酸标记测定有时非常复杂。衍生化为丁酰胺可减少同位素异构体分辨率和定量中的误差,从而更好地确定进入种子脂质储备的通量,包括质体和胞质反应。虽然在许多种子中,细胞壁可占生物量的三分之一或更多,但尚未有关于植物通量分析的定量细胞壁标记测量报告。水解细胞壁并将糖衍生化为糖醇乙酸酯,可提供新的标记信息,从而有助于识别通过胞质溶胶上部糖酵解中间体的通量。这些策略改进了植物细胞区室化通量网络中关键碳通量的定量。

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