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原位³¹P核磁共振用于观察碱化后恒化器培养的酿酒酵母中多聚磷酸盐和分解代谢物的反应。

In situ 31P nuclear magnetic resonance for observation of polyphosphate and catabolite responses of chemostat-cultivated Saccharomyces cerevisiae after alkalinization.

作者信息

Castro C D, Meehan A J, Koretsky A P, Domach M M

机构信息

Department of Chemical Engineering, Carnegie Mellon University, Pittsburgh, Pennsylvania 15213, USA.

出版信息

Appl Environ Microbiol. 1995 Dec;61(12):4448-53. doi: 10.1128/aem.61.12.4448-4453.1995.

Abstract

The proposed pH buffering and phosphagenic functions of polyphosphate were investigated by subjecting chemostat-cultivated Saccharomyces cerevisiae to alkalinization (NaOH addition) and anaerobiosis. The subsequent changes in intracellular phosphate-containing species were observed in situ by nuclear magnetic resonance (NMR) spectroscopy by using the NMR cultivator we developed. For the alkalinization experiments, changes in catabolite secretion were also measured in parallel experiments. Additionally, a range of potential neutralization capacity was investigated: a dilute culture and concentrated cultures with low or high polyphosphate content. The concentrated cultures displayed increased cytosolic pH and rapid polyphosphate degradation to small chains. The pH changes and extent of polyphosphate degradation depended inversely on initial polyphosphate content. The dilute culture restored extracellular pH rapidly and secreted acetate. The concentrated culture with low polyphosphate reserves also secreted acetate. In contrast to the alkalinization-induced polyphosphate dynamics, anaerobiosis resulted in the complete hydrolysis of polyphosphate to P(i), as opposed to small chains, and reduced cytosolic pH. The results and calculations suggest that the bulk of NMR-observable polyphosphate (vacuolar) degradation to short polymers conceivably contributes to neutralizing added alkalinity. In other circumstances, such as anaerobiosis, degradation serves other functions, such as phosphorylation potential regulation.

摘要

通过对恒化器培养的酿酒酵母进行碱化处理(添加氢氧化钠)和厌氧处理,研究了多聚磷酸盐的pH缓冲和磷酸原功能。利用我们开发的核磁共振培养器,通过核磁共振光谱原位观察了随后细胞内含磷物质的变化。对于碱化实验,在平行实验中还测量了分解代谢物分泌的变化。此外,还研究了一系列潜在的中和能力:稀释培养物以及低聚磷酸盐含量或高聚磷酸盐含量的浓缩培养物。浓缩培养物显示出胞质pH值升高,多聚磷酸盐迅速降解为短链。pH值变化和多聚磷酸盐降解程度与初始多聚磷酸盐含量成反比。稀释培养物能迅速恢复细胞外pH值并分泌乙酸盐。低聚磷酸盐储备的浓缩培养物也分泌乙酸盐。与碱化诱导的多聚磷酸盐动态变化相反,厌氧处理导致多聚磷酸盐完全水解为无机磷酸盐(P(i)),而不是短链,并降低了胞质pH值。结果和计算表明,核磁共振可观察到的大部分多聚磷酸盐(液泡)降解为短聚合物,可能有助于中和添加的碱度。在其他情况下,如厌氧处理,降解发挥其他功能,如调节磷酸化电位。

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