key: cord-0949320-ul3nz6qu
authors: Oommen, Anup; Cunningham, Stephen; Joshi, Lokesh
title: Transcriptomic Analysis of Respiratory Tissue and Cell Line Models to Examine Glycosylation Machinery during SARS-CoV-2 Infection
date: 2021-01-08
journal: Viruses
DOI: 10.3390/v13010082
sha: 4710ca840a93eb9c7e352dc9d6fff69c3f056d87
doc_id: 949320
cord_uid: ul3nz6qu

Glycosylation, being the most abundant post-translational modification, plays a profound role affecting expression, localization and function of proteins and macromolecules in immune response to infection. Presented are the findings of a transcriptomic analysis performed using high-throughput functional genomics data from public repository to examine the altered transcription of the human glycosylation machinery in response to SARS-CoV-2 stimulus and infection. In addition to the conventional in silico functional enrichment analysis methods we also present results from the manual analysis of biomedical literature databases to bring about the biological significance of glycans and glycan-binding proteins in modulating the host immune response during SARS-CoV-2 infection. Our analysis revealed key immunomodulatory lectins, proteoglycans and glycan epitopes implicated in exerting both negative and positive downstream inflammatory signaling pathways, in addition to its vital role as adhesion receptors for SARS-CoV-2 pathogen. A hypothetical correlation of the differentially expressed human glycogenes with the altered host inflammatory response and the cytokine storm-generated in response to SARS-CoV-2 pathogen is proposed. These markers can provide novel insights into the diverse roles and functioning of glycosylation pathways modulated by SARS-CoV-2, provide avenues of stratification, treatment, and targeted approaches for COVID-19 immunity and other viral infectious agents.

Of the four major classes of biomolecules (nucleic acids, proteins, glycans, and lipids), the glycans conjugated to proteins and lipids provide a ubiquitous biological interface at cell surfaces, where they are instrumental in intermolecular and cell-cell recognition events that define and control cell interactions and functions [1] . Indeed, with greater than 70% of circulating proteins being glycosylated, including most cytokines and all immunoglobulins, the role of glycosylation in immune function is key, extending beyond the first-contact cell surface interaction [2] . Though not template-driven, the synthesis and presence of glycans on cell surfaces and macromolecules is driven by a known and diverse set of genes, collectively referred to as 'glycogenes', which encode the glycosylation machinery. Glycan recognition and function is typically mediated by complementary glycan-binding proteins (GBPs), which present specific glycan recognition domains conferring glycan-binding specificity. In addition, functional domains translate glycan recognition into functional cellular responses, positioning the role of glycans and GBPs as key components of the immune system [3] . Greater understanding of the glycans, GBPs and their associated molecular

GenePattern (http://software.broadinstitute.org/cancer/software/genepattern/) [30] and Galaxy (https://usegalaxy.org/) [31] were utilized for data processing as detailed in their respective user manuals. Where datasets had existing processed result files available through the GEO database these were used. Hierarchical clustering of the normalized gene expression data was performed using the Heatmap w ggplot tool in Galaxy Version 2.2.1. The mapping of differentially expressed glycogenes (DEGs) to known signaling pathways and cellular processes, and gene set enrichment analysis (GSEA), were performed using the g:Profiler web server [32] . Using the "Retrieve/ID mapping tool" [33] available in the UniProt Knowledgebase [34] detailed gene/protein function and other related database reference IDs were extracted for the DEGs. Pathway analysis was performed using the Reactome biological pathways (https://reactome.org/) [35] . The induced network module function available in ConsensusPathDB-(CPDB-http://cpdb.molgen.mpg.de/) [36] was used to identify any possible functional relationship between DEGs coding for lectins through the protein-protein interaction and biochemical reactions. Network analysis and visualization was performed with Cytoscape software (http://www.cytoscape.org/) [37] .

Seven array datasets were identified from the GEO database (July 2020), with the filter criteria of having at least three minimum samples for both control and SARS-CoV-2 treated/infected conditions (Supplementary Table S1 ). From these datasets, data from biological samples and cell lines, relevant only to the upper respiratory tract infection, were selected yielding six data points for subsequent data processing using the DESeq2 algorithm available in Genepattern genomics tool (Supplementary Table S1 ). From the DESeq2 analysis results (normalized, log2 fold changed, Benjamini-Hochberg adjusted p-value) significant genes with adjusted p value ≤ 0.1 and uncorrected p value ≤ 0.05 were identified for each data points (Supplementary Table S2 ). Using the gene set from the GlycoGAIT database (Supplementary Table S6 ), DEGs for each data points were identified which constitute~3% of the total differentially expressed genes under the selected p value cut off, except for the lung samples (Supplementary Table S2 ). Data analysis of each data points using the frequency distribution function in Excel revealed that distribution of differentially expressed genes from the SARS-CoV-2 infected cell lines and organoids are largely represented within the range of −0.5 to +0.5 log twofold change values. On the contrary for the biopsy samples (nasopharyngeal and lung) the gene distribution was higher above the ±0.5 log twofold change cut-off values (Supplementary Table S2) . Moreover, the clustered heatmap of the DEGs revealed that the gene expression pattern obtained from the nasopharyngeal swab and the Calu cell line show close similarity and were also the two data sources that showed maximum number of significant differentially expressed genes including the glycogenes (Supplementary Table S2 ). Higher level gene family association of the DEGs revealed that glycosyltransferases, lectins, proteoglycans, glycosidases and sulfotransferases as the maximum represented groups, majorly in the Calu cell line and the nasopharyngeal samples ( Figure 1A ,B, Supplementary Table S3 ). significant genes with adjusted p value ≤ 0.1 and uncorrected p value ≤ 0.05 were identified for each data points (Supplementary Table S2 ). Using the gene set from the GlycoGAIT database (Supplementary Table S6 ), DEGs for each data points were identified which constitute ~3% of the total differentially expressed genes under the selected p value cut off, except for the lung samples (Supplementary Table S2 ). Data analysis of each data points using the frequency distribution function in Excel revealed that distribution of differentially expressed genes from the SARS-CoV-2 infected cell lines and organoids are largely represented within the range of −0.5 to +0.5 log twofold change values. On the contrary for the biopsy samples (nasopharyngeal and lung) the gene distribution was higher above the ±0.5 log twofold change cut-off values (Supplementary Table S2 ). Moreover, the clustered heatmap of the DEGs revealed that the gene expression pattern obtained from the nasopharyngeal swab and the Calu cell line show close similarity and were also the two data sources that showed maximum number of significant differentially expressed genes including the glycogenes (Supplementary Table S2 ). Higher level gene family association of the DEGs revealed that glycosyltransferases, lectins, proteoglycans, glycosidases and sulfotransferases as the maximum represented groups, majorly in the Calu cell line and the nasopharyngeal samples ( Figure 1A ,B, Supplementary Table S3 ). For focused analysis on glycogenes, a stringent log2 fold change cut-off values ≤ −0.58 and ≥0.58 (fold change ≥ 1.5-fold) was performed. Detailed gene set enrichment analysis of the resulting DEGs using the g:Profiler toolset, highlighted specific cellular processes such as the glycosaminoglycan, proteoglycan, glycolipid, N-glycan and O-glycan metabolic processes as the maximum represented biological categories (Supplementary Table S4) . Similarly, acetylglucosaminyltransferases, acetylgalactosaminyltransferases, carbohydrate binding, sulfotransferases were the most significant and more specific GO: molecular functions identified from the g:Profiler toolset (Figure 2A ,B); Supplementary Table S4 ). Combined analysis of the gene family association and gene enrichment analysis results revealed that the maximum represented glycosyltransferase gene family were associated with the glycolipid, N-glycan and O-glycan metabolic processes, which also included the fucosyltransferases and sialyltransferases involved in the synthesis of diverse glycan epitopes.

(A) A genome-wide overview analysis from the Reactome database highlighted metabolic pathways associated with glycosylation modifications and additionally a number of immune related pathways including the immune-regulatory interaction between lymphoid and nonlymphoid cells, majorly represented by the DEGs transcribing for the lectin proteins (Supplementary Figure S1 ). Among the 56 metabolic processes that were mapped to the Reactome database, pathways with maximum number of intersecting DEGs were those associated with N-linked glycosylation (precursor biosynthesis, antennae elongation, trimming and complex type N-glycan synthesis); glycosaminoglycan metabolism (chondroitin/keratan/dermatan/heparin sulfate metabolism); O-linked glycosylation (biosynthesis and termination) and glycosylphosphatidylinositol (GPI) anchor biosynthesis. The DEGs associated with fructosyltransferase genes where mapped majorly to the blood group and Lewis antigen biosynthesis pathways (Supplementary Table S4 ). A representative pathway image of the cellular process from the Reactome database-"Blood group system biosynthesis", highlighted using the gene expression data obtained from the human nasopharyngeal swab of Covid-19 patients is given in Supplementary Figure S2 .

Lectins were the second category of maximum represented DEGs identified from the SARS-CoV-2 infected biopsy samples, cell lines and organoid relevant to the respiratory tract tissues (Supplementary Table S3 ). The C-type lectin receptors (Group II and Group V-NK cell receptor categories-CLEC) and the sialic acid binding I-type lectin receptors (SIGLEC) were the predominant ones with upregulated gene expression pattern (Supplementary Table S3 ). In order to delineate more detailed functional significance of the differentially regulated lectins, we used the induced network module feature from the CPDB database [36] . The protein-protein interaction network revealed molecular network association of lectin DEGs with both the negative regulatory and immunostimulatory signaling pathways. For example, the network captures the interaction between the galactose binding lectins (LGALS 1/2/3) with the negative regulatory protein tyrosine phosphatase (PTPN) signaling pathway while the CLECs and SIGLECs were found to be associated with the immunostimulatory signaling pathways mediated by the toll like receptors (TLRs), Killer Cell Lectin Like Receptor (KLRs), MHC class I-related molecules and the intracellular non-receptor tyrosine kinase signaling pathways ( Figure 3 ). Though the role of such interactions needs to be experimental assessed in a SARS-CoV-2 infected airway epithelium system, the analysis network findings highlight the prospective immunomodulatory role of these lectins, which are well-characterized positive/negative regulators of innate and adaptive immunity [38] .

Significant DEGs, grouped under the glycosylation associated cellular function pathways, were also manually analyzed for the association with human pathogenic viruses and immune system in order to understand the physiological relevance in response to SARS-CoV-2 infection from the biological samples (biopsies and cell lines) representing the upper respiratory tract (Supplementary Table S5 ). Manual compilation of the glycan epitope association for the DEGs, enabled the identification of the clinical significance of the transcriptomic changes for few genes in relation with immune response and viral infection conditions (Supplementary Table S5 ). For example, serglycin (SRGN) (increased expression pattern across samples), is one of the main proteoglycans of the cytotoxic granules in CTLs and NK cells and is known to regulate the kinetics of antiviral CD8 + T-cell responses. Moreover, serglycin proteoglycan with sulfated glycosaminoglycans of either heparin, heparan sulfate or chondroitin sulfate types attached to it is a major regulator of the mast cell secretory granule homeostasis [39] . Recent studies reported the presence of activated mast cells in the lungs of deceased patients with COVID-19, which are correlated with the release of pathogenic mediators linked to pulmonary edema, inflammation and thromboses [40] . Given the heparan sulfate-dependent enhanced attachment and infection of SARS-CoV-2 virus [41] , it will be interesting to evaluate a model where serglycin as a critical mediator between SARS-CoV-2 infection, mast cell activation and the pulmonary pathology. of SARS-CoV-2 virus [41] , it will be interesting to evaluate a model where serglycin as a critical mediator between SARS-CoV-2 infection, mast cell activation and the pulmonary pathology. Table S5 ). These antigens also plays a crucial role in regulating the lytic function of cytotoxic T lymphocytes as well as leukocyte adhesion and migration and hence might also correlate with the SAR-CoV-2 infection and immune overdrive (Supplementary Table S5) .

Upregulated expression of genes encoding lectins which are previously reported to function as adhesive receptors for SARS-CoV-2 (such as SIGLEC5, MASP2, CLEC4M) were identified. Among them the mannose binding lectin serine protease 2 (MASP-2) has also been implicated in the altered lectin complement pathway resulting in accelerated inflammatory responses and lung damages involved in COVID-19 pathogenesis [42] . Few other C-type, I-type and S-type lectins in the list were found to be either induced by or associated with the adhesion of other viral strains such as the influenza virus, Ebola virus, Hepatitis C virus, Human Immunodeficiency Virus. Among Galectins, increased expression of LGALS9 elicited by SARS-CoV-2 infection correlate with that observed during the HIV-1 infection which was reported to mediate T-cell inflammation and exhaustion [43] Table S5 ). These antigens also plays a crucial role in regulating the lytic function of cytotoxic T lymphocytes as well as leukocyte adhesion and migration and hence might also correlate with the SAR-CoV-2 infection and immune overdrive (Supplementary Table S5) .

Upregulated expression of genes encoding lectins which are previously reported to function as adhesive receptors for SARS-CoV-2 (such as SIGLEC5, MASP2, CLEC4M) were identified. Among them the mannose binding lectin serine protease 2 (MASP-2) has also been implicated in the altered lectin complement pathway resulting in accelerated inflammatory responses and lung damages involved in COVID-19 pathogenesis [42] . Few other C-type, I-type and S-type lectins in the list were found to be either induced by or associated with the adhesion of other viral strains such as the influenza virus, Ebola virus, Hepatitis C virus, Human Immunodeficiency Virus. Among Galectins, increased expression of LGALS9 elicited by SARS-CoV-2 infection correlate with that observed during the HIV-1 infection which was reported to mediate T-cell inflammation and exhaustion [43] as is the case with COVID-19. From an immune regulatory perspective, previous reports implicate both positive and negative regulatory functions for various DEGs belonging to Table S5 ).

The downregulated DEGs primarily represent the biological processes involved in glycan precursor biosynthetic pathways such as the N-glycan precursor biosynthetic processes, O-linked biosynthetic process, GPI-anchor biosynthesis as well as fucose, mannose and galactose metabolism (Supplementary Table S5 ). Defective GPI-anchor biosynthetic pathway as well as the N-glycan chain transfer to the nascent polypeptide chain were shown previously to affect the infectivity of pathogenic viruses like HIV-1 and Hepatitis C virus [40, 41] . Whether this downregulated expression pattern represent an adaptive feedback mechanism can only be speculated and can be subjected to targeted experimental validation to explore the regulatory mechanism under SARS-CoV-2 infection condition.

Similar to the strategies previously applied for curbing the spread of viral infections, current research efforts are directed towards the development of therapeutic antibodies and vaccines for effective COVID-19 treatment [44, 45] . Kinetics of immune response from mild, moderate to severe COVID-19 patients ranges from augmented humoral and cellular immunity to lymphopenia affecting CD4+ T cells, CD8+ T cells, B cells and natural killer cells [46] [47] [48] [49] . Furthermore, the degree of lymphopenia and pro-inflammatory cytokine storm was reported to be higher in severe COVID-19 patients and correlated with the adverse outcomes such as immune mediated lung injury and acute respiratory distress syndrome in these patients [50] [51] [52] [53] . Reduction in the level of ACE2, following the binding and internalization of SARS coronavirus is considered as a critical factor that alters Renin-angiotensin system and concomitant disease pathogenesis such as lung oedemas, elevated macrophage infiltration, cytokine production and endothelial dysfunction [54, 55] . The exponential growth in the cytokine storm in lung tissues and systemic circulation beget the pulmonary pathology of SARS-CoV-2 infection alveolar damage with cellular fibromyxoid exudates, desquamation of pneumocytes and hyaline membrane formation which are the salient features of ARDS [52, 56] . A recent review on the altered expression of different cytokines in COVID-19 patients concluded that SARS-CoV-2 infection could be characterized by the depletion of antiviral defenses (such as delayed IFN-α and -β response as well as an elevated production of inflammatory cytokines [57] . Further to, altered procoagulant-anticoagulant pathways associated with the cytokine storm also drives the development of microthrombosis, disseminated intravascular coagulation, and multi-organ failure as evidenced in severe cases of COVID-19 subjects [58, 59] . Despite extensive characterization of the altered immunological features underlying the spectrum of disease associated with COVID-19, the role played by alteration in glycosylation PTM remains to be addressed.

Glycan binding proteins (GBPs) and the glycoconjugate structures play a crucial modulatory function in regulating the host immune responses under diverse inflammatory diseases [60] . In case of COVID-19 acute respiratory infection, several recent studies evidenced the essential role of glycoconjugate structures such as heparan sulfate and sialosides (sialic acid-containing carbohydrates) in mediating the attachment and infection of SARS-CoV-2 virus [61] [62] [63] . This enticed the attention of researchers in devising therapeutic strategies to curtail the virus infection [41, 64] . Additionally, it has also been reported that infectious SARS virions harness host histo-blood group antigens on S proteins [65] , which might presumably modulate the interaction with host cell glycoprotein receptors through carbohydrate-carbohydrate interactions [66] . The current transcriptomic based research analysis is aimed to generate a hypothetical view of the alteration in glycan machinery, which could be used to explain the relevance of glycosylation underlying the lung pathology and immune responses reported in COVID-19 subjects. Given the maximum number of gene representation from the nasopharyngeal samples followed by the Calu cell line, interpretation of the DEGs relevance is largely based on the gene expression pattern observed from these samples. Results from our manual literature-based analysis reveals a common pattern of glycan epitope structures shared between SARS-CoV-2 virus and other various pathogenic viruses for adhesion and infection of the host cells. Schematic representation of these diverse glycan epitope host ligands for pathogenic virus (Supplementary Table S5 , Figure 4 ).

Viruses 2021, 13, x FOR PEER REVIEW 10 of 16 based research analysis is aimed to generate a hypothetical view of the alteration in glycan machinery, which could be used to explain the relevance of glycosylation underlying the lung pathology and immune responses reported in COVID-19 subjects. Given the maximum number of gene representation from the nasopharyngeal samples followed by the Calu cell line, interpretation of the DEGs relevance is largely based on the gene expression pattern observed from these samples. Results from our manual literature-based analysis reveals a common pattern of glycan epitope structures shared between SARS-CoV-2 virus and other various pathogenic viruses for adhesion and infection of the host cells. Schematic representation of these diverse glycan epitope host ligands for pathogenic virus (Supplementary Table S5 , Figure 4 ). Increased expression pattern of major fucosyltransferases across the nasopharyngeal and lung samples as well as the cell lines may indicate a tendency of the SARS-CoV-2 infection to augment the inflammatory response by increasing the expression of glycan epitopes such as blood group antigens and Lewis X antigens that regulate the immune cell attraction to infected tissues [67] [68] [69] . The gene expression pattern of sialyltransferase from the nasopharyngeal samples was also insightful into the potential immunomodulatory nature of SARS-CoV-2 virus. Gene expression data from the nasopharyngeal sample showed an interesting pattern regarding the sialyltransferases, wherein there was an in- Increased expression pattern of major fucosyltransferases across the nasopharyngeal and lung samples as well as the cell lines may indicate a tendency of the SARS-CoV-2 infection to augment the inflammatory response by increasing the expression of glycan epitopes such as blood group antigens and Lewis X antigens that regulate the immune cell attraction to infected tissues [67] [68] [69] . The gene expression pattern of sialyltransferase from the nasopharyngeal samples was also insightful into the potential immunomodulatory nature of SARS-CoV-2 virus. Gene expression data from the nasopharyngeal sample showed an interesting pattern regarding the sialyltransferases, wherein there was an increase in expression of genes coding for α-2,3 sialyltransferases and α-2,8 sialyltransferases concomitant with decreased expression of genes coding for α-2,6 sialyltransferase enzymes involved in the synthesis of sialyl-Tn antigen. From an immune perspective, these sialyl-transferases are known to generate sialylated glycans involved in immune cell trafficking and inflammatory response [70, 71] . Previous glycomic analysis of the human lung and respiratory tract tissues revealed predominant expression of N-and O-glycans expressing α-2,3/α-2,6/α-2,8 linked sialoglycans [72, 73] . Moreover, immunomodulatory and viral adhesive functions were also attributed for these sialoglycans expressed in the human lung and respiratory tract tissues. The expression pattern of sialyltransferase reported in this study correlate with that of the metaplastic mucous cells in ferret airways infected with human H1N1 influenza virus [74] .

Based on these findings we hypothesize that SARS-CoV-2 infection results in the increased expression of α-2,3 and α-2,8 linked sialic acid structures in the human respiratory tract tissues aiding viral replication as observed in other similar avian viruses [75] . Similar to the alteration in bronchial mucins reported for patients suffering from chronic bronchitis and cystic fibrosis it will be interesting to evaluate whether human airway mucins from SARS-CoV-2 infected individuals express increased levels of sLex epitope, related to inflammation and infection [76] . Increased expression of B4GALNT2 gene, coding for the core enzyme involved in the synthesis of Sd(a) antigen, across different samples infected with SARS-CoV-2 is an interesting observation. Previous studies ascertained diverse cellular roles for B4GALNT2 associated Sd(a) antigen expression on cell surfaces which includes-prevention of H1N1 viral infection, reducing metastasis of cancer cells, lytic function of cytotoxic T-lymphocytes [77] . Hence, targeted gene expression studies as well as glyco-profiling of the airway epithelium infected with SARS-CoV-2 virus can validate whether Sd(a) antigens predominate sLe x antigens and the increased expression of B4GALNT2 is an adaptive mechanism to reduce the severity of the infection.

Gene expression pattern and the induced network model analysis results of the inflammatory CLECs and the anti-inflammatory SIGLECs mentioned in the current report is in alignment with the clinical phenotype of cytokine storm, neutrophil extracellular trap formation as well as the functional exhaustion of lymphocytes reported in severe cases of COVID-19 patients [46] [47] [48] [49] 78, 79] . Increased gene expression pattern of inflammatory CLECs in the nasopharyngeal samples may represent the molecular markers of innate immune function of airway epithelial cells and immune components [80, 81] . However, dual anti-inflammatory function have also been attributed to few CLECs such as CLEC7A (Dectin-1) and CLEC4E (Mincle) depending on the ligand and its interaction with the pattern recognition receptors [82] . Similarly, the anti-inflammatory function of differentially expressed SIGLECs to attenuate immune responses, may be an adaptive mechanism for preventing lymphocyte exhaustion or cell death under heightened inflammatory conditions [83] . Further to, a suppressive function of host antiviral innate immune response has also been attributed to few SIGLECs (such as the SIGLEC1 protein) [84] , which can be hypothesized to be induced by the SARS-CoV-2 infection conditions for evading the host innate immune response. Manual compilation of previous scientific reports also enabled us to identify the functional role of few differentially regulated lectins as potential adhesion receptors for various viral strains including the SARS-CoV-2 virus. Summarized view of the differentially expressed lectins and proteoglycans along with its previously established regulatory role on innate and adaptive immune responses could aid in exploring the role of glycoconjugate structures in dysregulated airway mucosal immunity elicited by SARS-CoV-2 infection [85] .

In the current study, results from the gene expression pattern are largely influenced by the nasopharyngeal swab samples. Since the nasopharyngeal swab samples represent a collection of diverse epithelial and immune cell types, cell type-specific analysis is essential to delineate the diverse inflammatory and anti-inflammatory functions of these glycogenes. Further analysis of the inflammatory pathways in conjunction with the experimental validation of the immune regulatory lectins should provide greater insights into the molecular mechanisms underlying compromised innate immune response in severe cases of COVID-19 patients [85] . Lectins such as CLECs and SIGLECs have been considered as potential immunotherapeutics in the field of cancer immunology and other chronic inflammatory diseases [86, 87] . Small molecules generated for these lectins could be even explored for therapeutically modulating COVID-19 immune dysregulation.

The current transcriptomic based study provides meaningful insights into the nature of gene expression alteration in glycosylation enzymes, proteoglycans, lectins and potential glycan markers that can be selected for targeted experiments to understand the immunomodulatory functions underlying SARS-CoV-2 infection. A list of potential CLECs, SIGLECs and Galectin lectins have been highlighted in the current research, which can be experimentally evaluated to modulate the cytokine storm or the lymphopenia pathology reported in COVID-19 subjects.

Supplementary Materials: The following are available online at https://www.mdpi.com/1999-4 915/13/1/82/s1, Table S1 : Transcriptomics Datasets; Table S2 : List of DEGs from 6 datapoints including glycogenes; Table S3 : List of differentially expressed glycogenes and gene family association.; Table S4 : Gene Enrichment Analysis Results; Table S5 : Selected List of DE Glycogenes and its physiological correlation with immune system and pathogenic virus; Table S6 : Glycomachinery Genepool; Figure S1 : Reacfoam-DEGs from the SARS-CoV-2 infected human nasopharyngeal swab; Figure 

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The authors declare no conflict of interest. The funders had no role in the design of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript, or in the decision to publish the results.