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首页> 外文期刊>Journal of the American Society for Mass Spectrometry >Discrimination of Isomers of Released N- and O-Glycans Using Diagnostic Product Ions in Negative Ion PGC-LC-ESI-MS/MS
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Discrimination of Isomers of Released N- and O-Glycans Using Diagnostic Product Ions in Negative Ion PGC-LC-ESI-MS/MS

机译:释放<重点型=“斜体”> N - 和<重点型=“斜体”> O - 聚糖使用负离子PGC-LC-ESI-MS /的诊断产品离子/ 聚糖的辨别 多发性硬化症

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摘要

Profiling cellular protein glycosylation is challenging due to the presence of highly similar glycan structures that play diverse roles in cellular physiology. As the anomericity and the exact linkage type of a single glycosidic bond can influence glycan function, there is a demand for improved and automated methods to confirm detailed structural features and to discriminate between structurally similar isomers, overcoming a significant bottleneck in the analysis of data generated by glycomics experiments. We used porous graphitized carbon-LC-ESI-MS/MS to separate and detect released N - and O -glycan isomers from mammalian model glycoproteins using negative mode resonance activation CID-MS/MS. By interrogating similar fragment spectra from closely related glycan isomers that differ only in arm position and sialyl linkage, product fragment ions for discrimination between these features were discovered. Using the Skyline software, at least two diagnostic fragment ions of high specificity were validated for automated discrimination of sialylation and arm position in N -glycan structures, and sialylation in O -glycan structures, complementing existing structural diagnostic ions. These diagnostic ions were shown to be useful for isomer discrimination using both linear and 3D ion trap mass spectrometers when analyzing complex glycan mixtures from cell lysates. Skyline was found to serve as a useful tool for automated assessment of glycan isomer discrimination. This platform-independent workflow can potentially be extended to automate the characterization and quantitation of other challenging glycan isomers. Graphical Abstract ?.
机译:由于存在高度相似的聚糖结构,谱分析细胞蛋白糖基化是挑战性的,这些糖类结构在细胞生理学中发挥不同的作用。作为单糖苷键的异构性和精确的连杆型可以影响聚糖功能,需要改进和自动化的方法,以确认详细的结构特征和区分结构上类似的异构体,克服了产生的数据分析中的显着瓶颈通过糖类实验。我们使用多孔石墨化的碳-LC-ESI-MS / MS以使用负模式共振激活CID -SS / MS分离和检测从哺乳动物模型糖蛋白的释放的N - 和O-庚醇异构体。通过从密切相关的甘油异构体询问类似的片段光谱,仅在臂位置和唾液酸连杆中不同,因此发现这些特征之间的辨别的产物片段离子。使用天际线软件,验证了至少两个高特异性的诊断片段离子,用于自动辨别唾液酸化和臂位置的唾液酸化和臂位置,含有o庚烷结构的唾液酸化,互补现有的结构诊断离子。当在分析来自细胞裂解物的复合聚糖混合物时,这些诊断离子可用于使用线性和3D离子阱质谱仪的异构体辨别。发现天际线作为自动评估甘草异构体歧视的有用工具。该平台无关的工作流程可能会延长以自动化其他具有挑战性的聚糖异构体的表征和定量。图形概要 ?。

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