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Glycomics by ion mobility tandem mass spectrometry of chondroitin sulfate disaccharide domain in biglycan
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AbstractBiglycan (BGN), a small leucine‐rich repeat proteoglycan, is involved in a variety of pathological processes including malignant transformation, for which the upregulation of BGN was found related to cancer cell invasiveness. Because the functions of BGN are mediated by its chondroitin/dermatan sulfate (CS/DS) chains through the sulfates, the determination of CS/DS structure and sulfation pattern is of major importance. In this study, we have implemented an advanced glycomics method based on ion mobility separation (IMS) mass spectrometry (MS) and tandem MS (MS/MS) to characterize the CS disaccharide domains in BGN. The high separation efficiency and sensitivity of this technique allowed the discrimination of five distinct CS disaccharide motifs, of which four irregulated in their sulfation pattern. For the first time, trisulfated unsaturated and bisulfated saturated disaccharides were found in BGN, the latter species documenting the non‐reducing end of the chains. The structural investigation by IMS MS/MS disclosed that in one or both of the CS/DS chains, the non‐reducing end is 3‐O‐sulfated GlcA in a rather rare bisulfated motif having the structure 3‐O‐sulfated GlcA‐4‐O‐sulfated GalNAc. Considering the role played by BGN in cancer cell spreading, the influence on this process of the newly identified sequences will be investigated in the future.
Title: Glycomics by ion mobility tandem mass spectrometry of chondroitin sulfate disaccharide domain in biglycan
Description:
AbstractBiglycan (BGN), a small leucine‐rich repeat proteoglycan, is involved in a variety of pathological processes including malignant transformation, for which the upregulation of BGN was found related to cancer cell invasiveness.
Because the functions of BGN are mediated by its chondroitin/dermatan sulfate (CS/DS) chains through the sulfates, the determination of CS/DS structure and sulfation pattern is of major importance.
In this study, we have implemented an advanced glycomics method based on ion mobility separation (IMS) mass spectrometry (MS) and tandem MS (MS/MS) to characterize the CS disaccharide domains in BGN.
The high separation efficiency and sensitivity of this technique allowed the discrimination of five distinct CS disaccharide motifs, of which four irregulated in their sulfation pattern.
For the first time, trisulfated unsaturated and bisulfated saturated disaccharides were found in BGN, the latter species documenting the non‐reducing end of the chains.
The structural investigation by IMS MS/MS disclosed that in one or both of the CS/DS chains, the non‐reducing end is 3‐O‐sulfated GlcA in a rather rare bisulfated motif having the structure 3‐O‐sulfated GlcA‐4‐O‐sulfated GalNAc.
Considering the role played by BGN in cancer cell spreading, the influence on this process of the newly identified sequences will be investigated in the future.
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