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Sialic Acid Linkage Isomer Discrimination of N-glycans derived from Rat Cochlea using SialoCapper-ID Kit

Applications | 2021 | ShimadzuInstrumentation
Consumables, MALDI, LC/TOF, LC/MS
Industries
Clinical Research
Manufacturer
Shimadzu

Summary

Importance of the Topic


Glycan sialic acids, particularly N-acetylneuraminic and N-glycolyl variants, are critical in cell–cell communication and pathogen interactions. Linkage isomers (α2,3 vs α2,6) can modulate biological functions and serve as disease biomarkers, but their analysis is challenging.

Objectives and Study Overview


This work demonstrates a streamlined approach to identify sialic acid linkage on PA-labeled N-glycans from rat cochlea tissue. The goal is to bypass complex chromatographic separation by combining selective chemical derivatization with MALDI-TOF MS.

Methodology and Instrumentation


Two-dimensional HPLC (DEAE anion exchange, reversed-phase ODS, normal-phase amide) and LC-MS were first used to elucidate glycan structures. Sialic acid residues were then derivatized by the SALSA sequential amidation: isopropylamine for α2,6 and methylamine for α2,3 linkages. Excess reagents were removed by HILIC-SPE cleanup. MALDI-TOF MS (Shimadzu MALDI-8020 with CHCA matrix and sodium chloride) provided MS1 measurements.

Main Results and Discussion


After derivatization, α2,6 linkages displayed a mass shift of +41 Da, while α2,3 linkages added +13 Da. Mono- and di-sialylated glycans (e.g. PA-Hex6HexNAc4dHex1NeuAc1 and PA-Hex6HexNAc6dHex1NeuAc2) were successfully discriminated by comparing observed m/z values with theoretical predictions. This approach eliminated the need for retention time matching against glycan standards.

Benefits and Practical Applications


  • No requirement for specialized glycan standards for linkage analysis
  • Compatibility with existing PA-labeling workflows without additional LC steps
  • Rapid throughput via direct MALDI-MS acquisition

Future Trends and Opportunities


Integration of SialoCapper-ID derivatization with high-throughput MALDI imaging and LC-MS platforms could broaden applications to diverse biological samples and clinical diagnostics. Automation of the derivatization workflow and extension to other glycan classes are promising directions.

Conclusion


The SialoCapper-ID Kit enables rapid, linkage-specific derivatization of sialic acids on PA-labeled N-glycans, facilitating direct discrimination by MALDI-TOF MS without extensive chromatographic steps. This method enhances glycan profiling capabilities in research and diagnostic settings.

Instrumentation Used


  • MALDI-TOF mass spectrometer: Shimadzu MALDI-8020
  • HPLC systems: DEAE anion exchange, reversed-phase ODS, normal-phase amide columns
  • HILIC-SPE cleanup chips

References


  1. Nonomura Y, et al. Characterisation of N-glycans in the epithelial-like tissue of the rat cochlea. Sci Rep. 9:1551 (2019)
  2. Nishikaze T, et al. Differentiation of sialyl linkage isomers by one-pot sialic acid derivatization for MS-based glycan profiling. Anal Chem. 89:2353-2360 (2017)
  3. Hanamatsu H, et al. Sialic acid linkage specific derivatization of glycosphingolipid glycans by ring-opening aminolysis of lactones. Anal Chem. 90:13193-13199 (2018)

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