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葡萄酒(酿酒葡萄美乐)中RGII亚结构域的恢复及精细结构变异性

Recovery and fine structure variability of RGII sub-domains in wine (Vitis vinifera Merlot).

作者信息

Buffetto F, Ropartz D, Zhang X J, Gilbert H J, Guillon F, Ralet M-C

机构信息

INRA, UR1268 Biopolymères Interactions Assemblages, 44300 Nantes, France.

Institute for Cell and Molecular Biosciences Medical School, Newcastle University, Framlington Place, UK.

出版信息

Ann Bot. 2014 Oct;114(6):1327-37. doi: 10.1093/aob/mcu097. Epub 2014 Jun 7.

Abstract

BACKGROUND AND AIMS

Rhamnogalacturonan II (RGII) is a structurally complex pectic sub-domain composed of more than 12 different sugars and 20 different linkages distributed in five side chains along a homogalacturonan backbone. Although RGII has long been described as highly conserved over plant evolution, recent studies have revealed variations in the structure of the polysaccharide. This study examines the fine structure variability of RGII in wine, focusing on the side chains A and B obtained after sequential mild acid hydrolysis. Specifically, this study aims to differentiate intrinsic structural variations in these RGII side chains from structural variations due to acid hydrolysis.

METHODS

RGII from wine (Vitis vinifera Merlot) was sequentially hydrolysed with trifluoroacetic acid (TFA) and the hydrolysis products were separated by anion-exchange chromatography (AEC). AEC fractions or total hydrolysates were analysed by MALDI-TOF mass spectrometry.

KEY RESULTS

The optimal conditions to recover non-degraded side chain B, side chain A and RGII backbone were 0·1 m TFA at 40 °C for 16 h, 0·48 m TFA at 40 °C for 16 h (or 0·1 m TFA at 60 °C for 8 h) and 0·1 m TFA at 60 °C for 16 h, respectively. Side chain B was particularly prone to acid degradation. Side chain A and the RGII GalA backbone were partly degraded by 0·1 m TFA at 80 °C for 1-4 h. AEC allowed separation of side chain B, methyl-esterified side chain A and non-methyl-esterified side chain A. The structure of side chain A and the GalA backbone were highly variable.

CONCLUSIONS

Several modifications to the RGII structure of wine were identified. The observed dearabinosylation and deacetylation were primarily the consequence of acidic treatment, while variation in methyl-esterification, methyl-ether linkages and oxidation reflect natural diversity. The physiological significance of this variability, however, remains to be determined.

摘要

背景与目的

鼠李糖半乳糖醛酸聚糖II(RGII)是一种结构复杂的果胶亚结构域,由12种以上不同的糖类和20种不同的连接方式组成,沿同型半乳糖醛酸聚糖主链分布在五个侧链中。尽管长期以来RGII在植物进化过程中被描述为高度保守,但最近的研究揭示了该多糖结构的变异。本研究考察葡萄酒中RGII的精细结构变异性,重点关注顺序温和酸水解后得到的侧链A和侧链B。具体而言,本研究旨在区分这些RGII侧链的内在结构变异与酸水解导致的结构变异。

方法

用三氟乙酸(TFA)对葡萄酒(酿酒葡萄美乐)中的RGII进行顺序水解,水解产物通过阴离子交换色谱(AEC)分离。通过基质辅助激光解吸电离飞行时间质谱(MALDI - TOF MS)分析AEC馏分或总水解产物。

关键结果

回收未降解的侧链B、侧链A和RGII主链的最佳条件分别为40℃下0.1 m TFA处理16 h、40℃下0.48 m TFA处理16 h(或60℃下0.1 m TFA处理8 h)以及60℃下0.1 m TFA处理16 h。侧链B尤其容易发生酸降解。侧链A和RGII的半乳糖醛酸(GalA)主链在80℃下0.1 m TFA处理1 - 4 h时会部分降解。AEC能够分离侧链B、甲基酯化的侧链A和非甲基酯化的侧链A。侧链A和GalA主链结构高度可变。

结论

确定了葡萄酒中RGII结构的几种修饰。观察到的脱阿拉伯糖基化和脱乙酰化主要是酸性处理的结果,而甲基酯化、甲基醚键连接和氧化的变异反映了自然多样性。然而,这种变异性的生理意义仍有待确定。

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