Cancer and disease glycomics aim to delineate the pathophysiological glycosylation changes of significant translational values. Ability to efficiently map the altered glycosylation features particularly the terminal glyco-epitopes (glycotopes) not only is essential to drive basic glycobiology research but also can uncover valuable disease markers. Despite well-recognized biological importance, high precision and comprehensive mass spectrometry (MS)-based glycomic identification and quantitative mapping of terminal glycotopes particularly the sulfo-, sialylated glycotopes on various immune cell types remains technically challenging and rarely reported. In this thesis work, MS-based (sulfo)-glycomic platform previously developed in the laboratory was extended by developing and incorporating additional complementary analytical approaches in two different aspects. First, nanoLC-MS/MS analysis of native N-glycans on capillary poros graphitized carbon column was investigated and shown to be a more efficient and direct way to resolve the sialyl linkages of N-glycans carrying sulfo-sialylated glycotopes. This allows semi-quantitative mapping of the relative expression of specific sulfo-sialylated ligands of an inhibitory B cell receptor, CD22, on the peripheral blood mononuclear cells (PBMC) collected from B-CLL patients. However, de novo sequencing and identification of the sulfated glycotopes down to the level of defining the position of sulfate was found to be more readily accomplished by MS2/MS3 analysis of permethylated glycans at higher sensitivity. To home in on this latter aspect, the second and major part of this thesis work was devoted to explore the feasibility of more comprehensive mapping via alternative data acquisition method. An intelligent GlycOmics DIA (iGODIA) workflow, including dual positive/negative polarity analysis, tandem MS2/MS3, and Qual/Quan experiments, were investigated using permethylated non-sulfated and sulfated O-glycan from BSM as respective standards in positive and negative ion modes to establish optimum data independent acquisition (DIA) setup and instrument parameters. Further product dependent (pd)-MS3 were applied following DIA to resolve isomeric targeted glycotopes and various modes of relative quantification were experimented. In comparison against current LC-MS2-pd-MS3 data dependent acquisition mode, the advantages and extra benefits of this iGODIA workflow were clearly demonstrated when target-adapted against glycotopes on O-glycans of colon cancer stage III patients' tissue samples.