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Negative electrospray ionization mass spectrometry: a method for sequencing and determining linkage position in oligosaccharides from branched hemicelluloses

机译:负电喷雾电离质谱法:一种测序和确定支链半纤维素寡糖中连接位置的方法

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Xyloglucans of apple, tomato, bilberry and tamarind were hydrolyzed by commercial endo -1-4-D-endoglucanase. The xylo-gluco-oligosaccharides (XylGos) released were separated on CarboPac PA 200 column in less than 15min, and, after purification, they were structurally characterized by negative electrospray ionization mass spectrometry using a quadrupole time-of-flight (ESI-Q-TOF), a hybrid linear ion trap (LTQ)/Orbitrap and a hybrid quadrupole Fourier transform ion cyclotron resonance (FT-ICR) mass spectrometers. In order to corroborate the fragmentation routes observed on XylGos, some commercial galacto-manno-oligosaccharides (GalMOs) and glucurono-xylo-oligosaccharides were also studied. The fragmentation pathways of the ionized GalMos were similar to those of XylGos ones. The product ion spectra were mainly characterized by prominent double cleavage (D) ions corresponding to the entire inner side chains. The directed fragmentation from the reducing end to the other end was observed for the main glycosylated backbone but also for the side-chains, allowing their complete sequencing. Relevant cross-ring cleavage ions from X-0,2(j) -type revealed to be diagnostic of the 1-2-linked- glycosyl units from XylGos together with the 1-2-linked glucuronic acid unit from glucuronoxylans. Resonant activation in the LTQ Orbitrap allowed not only determining the type of all linkages but also the O-acetyl group location on fucosylated side-chains. Moreover, the fragmentation of the different side chains using the MSn capabilities of the LTQ/Orbitrap analyzer also allowed differentiating terminal arabinosyl and xylosyl substituents inside S and U side-chains of XylGos, respectively. The CID spectra obtained were very informative for distinction of isomeric structures differing only in their substitution pattern. These features together makes the fragmentation in negative ionization mode a relevant and powerful technique useful to highlight the subtle structural changes generally observed during the development of plant organs such as during fruit ripening and for the screening of cell wall mutants with altered hemicellulose structure. Copyright (c) 2015 John Wiley & Sons, Ltd.
机译:苹果,番茄,越桔和罗望子树的木葡聚糖被商品化的内生的-1-4-D-内葡聚糖酶水解。释放的木糖葡萄糖寡糖(XylGos)在不到15分钟的时间内在CarboPac PA 200色谱柱上分离,纯化后,使用四极杆飞行时间(ESI-Q- TOF),混合线性离子阱(LTQ)/ Orbitrap和混合四极傅里叶变换离子回旋共振(FT-ICR)质谱仪。为了证实在XylGos上观察到的片段化途径,还研究了一些商品化的半乳甘露糖寡糖(GalMOs)和葡糖醛酸木糖寡糖。电离的GalMos的碎裂途径与XylGos的碎裂途径相似。产物离子光谱的主要特征是与整个内侧链相对应的突出的双裂解(D)离子。对于主要的糖基化骨架,还观察到了从还原端到另一端的定向片段化,而且还观察到了侧链,从而可以对其进行完整测序。 X-0,2(j)-型的相关的交叉环裂解离子显示出对来自XylGos的1-2-连接的糖基单元与来自葡糖醛酸木聚糖的1-2-连接的葡糖醛酸单元的诊断。 LTQ Orbitrap中的共振激活不仅可以确定所有键的类型,还可以确定岩藻糖基化侧链上的O-乙酰基位置。此外,使用LTQ / Orbitrap分析仪的MSn功能裂解不同的侧链也分别区分了XylGos的S和U侧链内部的末端阿拉伯糖基和木糖基取代基。所获得的CID光谱对于区分仅在其取代模式上有所不同的异构体结构很有帮助。这些特征一起使负电离模式下的片段化成为一种重要的相关技术,可用于突出植物器官发育过程中通常观察到的细微结构变化,例如在果实成熟过程中以及用于筛选具有改变的半纤维素结构的细胞壁突变体。版权所有(c)2015 John Wiley&Sons,Ltd.

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