Epitope mapping, expression and post-translational modifications of two isoforms of CD33 (CD33M and CD33m) on lymphoid and myeloid human cells

Pérez-Oliva, Ana B.; Martínez‐Esparza, María; Vicente-Fernández, José J; Corral-San-Miguel, Rubén; García‐Peñarrubia, Pilar; Hernández‐Caselles, Trinidad

doi:10.1093/glycob/cwq220

Cited by 63 publications

(69 citation statements)

References 27 publications

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“…We used tagged versions of the CD33 proteins to distinguish those from endogenously expressed CD33 in some of these cell lines and to be able to track the CD33 ∆E2 and CD33 ∆E2,E7a variants. While previous studies suggested that one CD33 antibody (clone Him3-4) specifically recognizes the C 2 - set Ig-like domain and could be used to detect CD33 variants that lack exon 2 [9], in our experiments Him3- 4 only recognized CD33 FL and CD33 E7a but not CD33 ∆E2 or CD33 ∆E2,E7a when expressed in virally-transduced ALL cell lines that are devoid of endogenous CD33 (Jurkat, RCH-ACV, REH, or RS4;11: Figure 3) and only recognized CD33 FL but not CD33 ∆E2 when expressed in virally-transduced HEK293T cells (Figure 4). As shown in Figure 5, engineered sublines expressed high amounts of CD33 FL and CD33 E7a in all cell lines.…”

Section: Resultsmentioning

confidence: 99%

Expression and functional characterization of CD33 transcript variants in human acute myeloid leukemia

et al. 2016

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With the demonstration of improved survival of some acute myeloid leukemia (AML) patients with the CD33 antibody-drug conjugate, gemtuzumab ozogamicin (GO), CD33 has been validated as a target for antigen-specific immunotherapy. Since previous studies identified a CD33 splice variant missing exon 2 (CD33∆E2) and, consequently, the immune-dominant membrane-distal V-set domain, we investigated the expression and functional characteristics of CD33 transcript variants in AML. In primary AML specimens, we not only found full-length CD33 (CD33FL) and CD33∆E2 but also corresponding variants containing an alternate exon 7 predicted to encode a CD33 protein lacking most of the intracellular domain (CD33E7a and, not previously described, CD33∆E2,E7a) in almost all cases. In acute leukemia cell sublines engineered to express individual CD33 splice variants, all splice variants had endocytic properties. CD33FL and CD33E7a mediated similar degrees of GO cytotoxicity, whereas CD33∆E2 and CD33∆E2,E7a could not serve as target for GO. Co-expression of CD33∆E2 did not interfere with CD33FL endocytosis and did not impact CD33FL-mediated GO cytotoxicity. Together, our findings document a greater-than-previously thought complexity of CD33 expression in human AML. They identify CD33 variants that lack exon 2 and are not recognized by current CD33-directed therapeutics as potential target for future unconjugated or conjugated antibodies.

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Section: Resultsmentioning

confidence: 99%

Expression and functional characterization of CD33 transcript variants in human acute myeloid leukemia

et al. 2016

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“…We also performed CD14 immunostaining by incubation of cells with FITC-conjugated 61D3, and after a washing step, they were stained with PE conjugated MФP9- mAb. The fluorescence intensity was analyzed by flow cytometry, and compared to that displayed by direct staining with the fluorochrome-conjugated 3G8- PE-Cy5 or MФP9-PE mAb on neutrophils or monocytes, respectively [21]. …”

Section: Methodsmentioning

confidence: 99%

GPI-anchor and GPI-anchored protein expression in PMM2-CDG patients

Morena‐Barrio

Hernández‐Caselles

Corral

et al. 2013

Orphanet J Rare Dis

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BackgroundMutations in PMM2 impair phosphomannomutase-2 activity and cause the most frequent congenital disorder of glycosylation, PMM2-CDG. Mannose-1-phosphate, that is deficient in this disorder, is also implicated in the biosynthesis of glycosylphosphatidyl inositol (GPI) anchors.ObjectiveTo evaluate whether GPI-anchor and GPI-anchored proteins are defective in PMM2-CDG patients.MethodsThe expression of GPI-anchor and seven GPI-anchored proteins was evaluated by flow cytometry in different cell types from twelve PMM2-CDG patients. Additionally, neutrophil CD16 and plasma hepatic proteins were studied by Western blot. Transferrin glycoforms were evaluated by HPLC.ResultsPatients and controls had similar surface expression of GPI-anchor and most GPI-anchored proteins. Nevertheless, patients displayed a significantly diminished binding of two anti-CD16 antibodies (3G8 and KD1) to neutrophils and also of anti-CD14 (61D3) to monocytes. Interestingly, CD16 immunostaining and asialotransferrin levels significantly correlated with patients’ age. Analysis by flow cytometry of CD14 with MΦP9, and CD16 expression in neutrophils by Western blot using H-80 ruled out deficiencies of these antigens.ConclusionsPMM2 mutations do not impair GPI-anchor or GPI-anchored protein expression. However, the glycosylation anomalies caused by PMM2 mutations might affect the immunoreactivity of monoclonal antibodies and lead to incorrect conclusions about the expression of different proteins, including GPI-anchored proteins. Neutrophils and monocytes are sensitive to PMM2 mutations, leading to abnormal glycosylation in immune receptors, which might potentially affect their affinity to their ligands, and contribute to infection. This study also confirms less severe hypoglycosylation defects in older PMM2-CDG patients.

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“…The expression of siglecs has been demonstrated on various cell types in a restricted pattern. Thus, Siglec-1 is expressed on macrophages, Siglec-2 on B lymphocytes, Siglec-3 on cells of the lymphoid and myeloid cells such as macrophages, monocytes and microglia (Varki and Angata 2006;Perez-Oliva et al 2011) and MAG/Siglec-4 on myelin-forming cells, the Schwann cells and oligodendrocytes (Matani et al 2007). Siglecs are single-pass (type 1) transmembrane proteins with variable numbers (1-16) of Ig-like constant region type 2 (C2-set Ig-like) domains and an amino-terminal Ig-like variable (V-set Ig-like) domain that bears the sialic-acid-binding site (Crocker 2005;Varki and Angata 2006;Crocker et al 2007;Varki 2009).…”

Section: Sgag-binding Receptorsmentioning

confidence: 99%

Microglial carbohydrate-binding receptors for neural repair

2012

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Microglia are the resident immune cells of the central nervous system (CNS) and perform typical scavenging and innate immune functions. Their capacity to eliminate extracellular aggregates and apoptotic neural material without inflammation is crucial for brain tissue homeostasis and repair. To fulfill these tasks, microglia express a whole set of recognition receptors including toll-like (TLRs), carbohydrate-binding, Fc, complement and cytokine receptors. Receptors recognizing carbohydrate structures are strongly involved in microglial repair function. Carbohydrate-binding receptors can be divided into two major subgroups: the sulfated glycosaminoglycan (SGAG)-binding receptors and the lectins (Siglecs, galectins, selectins). SGAG-binding receptors recognize anionic structural motifs within extended SGAG chains. Siglecs bind to the sialic acid cap of the intact glycocalyx. Other lectin family members such as galectins recognize lactosamine units typically exposed after alteration of the glycocalyx. Dependent on the type of microglial carbohydrate-binding receptors that are stimulated, either a pro-inflammatory cytotoxic or an anti-inflammatory repair-promoting response is evoked. The carbohydrate-binding receptors are also crucial in regulating microglial function such as phagocytosis during neurodegenerative or neuroinflammatory processes. A balance between microglial carbohydrate-binding receptor signaling via an immunoreceptor tyrosine-based activation motif or an immunoreceptor tyrosine-based inhibitory motif is required to polarize microglial cells appropriately so that they create a microenvironment permissive for neural regenerative events.

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Epitope mapping, expression and post-translational modifications of two isoforms of CD33 (CD33M and CD33m) on lymphoid and myeloid human cells

Cited by 63 publications

References 27 publications

Expression and functional characterization of CD33 transcript variants in human acute myeloid leukemia

Expression and functional characterization of CD33 transcript variants in human acute myeloid leukemia

GPI-anchor and GPI-anchored protein expression in PMM2-CDG patients

Microglial carbohydrate-binding receptors for neural repair

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