Elastase Controls the Binding of the Vitamin D-Binding Protein (Gc-Globulin) to Neutrophils: A Potential Role in the Regulation of C5a Co-Chemotactic Activity

DiMartino, Stephen J.; Shah, Anisha B.; Trujillo, Glenda; Kew, Richard R.

doi:10.4049/jimmunol.166.4.2688

Cited by 51 publications

(65 citation statements)

References 65 publications

(60 reference statements)

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“…In addition, azurophil granules are the last granule population to be mobilized and fuse with the plasma membrane during phagocytosis and/or cell activation (Faurschou and Borregaard, 2003). Azurophil granules also are the storage compartment for elastase (Faurschou and Borregaard, 2003), and we have demonstrated that this protease cleaves the DBP binding site (but not DBP) and sheds it into the extracellular milieu (DiMartino et al, 2001). Inhibition of elastase causes large amounts of DBP to accumulate on the cell surface (a 5-fold increase after 60 min) and also inhibits C5a chemotactic cofactor activity (DiMartino et al, 2001).…”

Section: Discussionmentioning

confidence: 80%

“…However, DBP by itself lacks chemotactic activity (Kew et al, 1995a;Kew and Webster, 1988). Plasma-derived DBP also binds to the surface of many cell types including neutrophils (DiMartino and Kew, 1999;DiMartino et al, 2001;White and Cooke, 2000). DBP appears to bind with low affinity to multiple cell surface ligands such as chondroitin sulfate proteoglycans (DiMartino and Kew, 1999), megalin (Nykjaer et al, 1999;Nykjaer et al, 2001), cubulin (Nykjaer et al, 2001), CD44 and annexin A2 (McVoy and Kew, 2005).…”

Section: Introductionmentioning

confidence: 99%

“…Neutrophils transiently generate co-chemotactic activity for C5a on the cell surface within 15-20 min of DBP binding (Kew et al, 1995a). These cells also utilize membrane-bound elastase to shed the DBP-binding site complex into the extracellular milieu (DiMartino et al, 2001). Both plasma membrane binding and subsequent shedding of DBP are essential in order for the protein to function as a chemotactic cofactor for C5a (DiMartino et al, 2001;Kew et al, 1995a).…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Upregulation of Vitamin D binding protein (Gc-globulin) binding sites during neutrophil activation from a latent reservoir in azurophil granules

DiMartino

Trujillo

McVoy

et al. 2007

Molecular Immunology

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Vitamin D binding protein (DBP) is a multifunctional plasma transport protein that is also found on the surface of many cell types. Cell surface DBP significantly enhances chemotactic activity of complement (C) peptides C5a and C5a des Arg. However, both DBP binding and C5a chemotaxis enhancement can vary among neutrophil donors. To test if activation during cell purification is responsible for this variability, neutrophils were isolated using both standard and LPS-free protocols. Cells isolated by the LPS-free method had no DBP-enhanced chemotaxis to C5a or DBP binding to plasma membranes. Moreover, neutrophils treated with LPS bound more avidity to immobilized DBP than sham-treated cells. Subcellular fractionation of neutrophils (standard protocol) revealed a heavy plasma membrane (HM) band that contained components of light plasma membranes and all three granules. The HM band possessed most of the DBP binding activity (58%), and activation of cells with ionomycin greatly increased DBP binding to HM. Azurophil granules contained 33% of the total DBP binding sites and there was a highly significant positive correlation (r = 0.988) between release of the granule marker myeloperoxidase and DBP binding. These results indicate that fusion of granules with the plasma membrane forms HM that contains DBP binding sites.

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Section: Discussionmentioning

confidence: 80%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Upregulation of Vitamin D binding protein (Gc-globulin) binding sites during neutrophil activation from a latent reservoir in azurophil granules

DiMartino

Trujillo

McVoy

et al. 2007

Molecular Immunology

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“…However, very little mechanistic information is available concerning how DBP enhances chemotaxis to the C5 derived peptides. Several studies from our laboratory have demonstrated that the binding of DBP to the neutrophil plasma membrane, and subsequent protease-mediated shedding of the binding site, are essential for the chemotaxis enhancement of C5a (DiMartino and Kew, 1999;DiMartino et al, 2001;Kew et al, 1995a;Kew et al, 1995b) More recently, we have demonstrated that DBP requires platelet-derived thrombospondin-1 for maximal cochemotactic activity (Trujillo and Kew, 2004). In addition, cell surface CD44 and annexin A2 are part of a DBP binding site complex and mediate the C5a chemotactic cofactor function of DBP (McVoy and Kew, 2005).…”

Section: Discussionmentioning

confidence: 99%

“…However, previous studies have shown that neutrophils transiently generate co-chemotactic activity for C5a/C5a des Arg on the cell surface within 15-20 min of DBP binding (Kew et al, 1995a). These cells also utilize membrane-bound elastase to shed the DBP-binding site into the extracellular milieu (DiMartino et al, 2001). Both plasma membrane binding and subsequent shedding of DBP are essential for the protein to function as a chemotactic cofactor for C5a.…”

Section: Introductionmentioning

confidence: 99%

Selective inhibition of the C5a chemotactic cofactor function of the Vitamin D binding protein by 1,25(OH)2 Vitamin D3

Shah

DiMartino

Trujillo

et al. 2006

Molecular Immunology

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The vitamin D binding protein (DBP) is a multifunctional plasma protein that can significantly enhance the chemotactic response to complement fragment C5a. The chemotactic cofactor function of DBP requires cell surface binding in order to mediate this process. The goal of this study was to investigate the effect of ligating DBP with its two primary physiological ligands, vitamin D and Gactin, on both binding to neutrophils and the ability to enhance chemotaxis to C5a. There was no difference in neutrophil binding between of the holo (bound) forms versus the apo (unbound) form of radioiodinated DBP, indicating that the cell binding region of DBP likely is distinct from the vitamin D sterol and G-actin binding sites. Likewise, G-actin, 25(OH)D 3 , and G-actin plus 25(OH) D 3 bound to DBP did not alter its capacity to enhance chemotaxis toward C5a. However, the active form of vitamin D (1,25(OH) 2 D 3 ) completely eliminated the chemotactic cofactor function of DBP. Dose response curves demonstrated that as little as 1 pM 1,25(OH) 2 D 3 significantly inhibited chemotaxis enhancement. Moreover, at physiological concentrations 1,25(OH) 2 D 3 needs to be bound to DBP to mediate the inhibitory effect. Neutrophil chemotaxis to optimal concentrations of C5a, formyl peptide, CXCL8 or leukotriene B 4 was not altered by 1,25(OH) 2 D 3 indicating that the active vitamin does not have a global inhibitory effect on neutrophil chemotaxis. Finally, inhibition of cell surface alkaline phosphatase with sodium orthovanadate completely reversed the inhibitory effect of 1,25(OH) 2 D 3 . These results indicate that the cell binding and co-chemotactic functions of DBP are not altered when the protein binds G-actin and/or vitamin D. Furthermore, the co-chemotactic signal from DBP can be eliminated or counteracted by 1,25(OH) 2 D 3 .

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Transcriptomic analysis reveal the responses of dendritic cells to VDBP

et al. 2022

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Elastase Controls the Binding of the Vitamin D-Binding Protein (Gc-Globulin) to Neutrophils: A Potential Role in the Regulation of C5a Co-Chemotactic Activity

Cited by 51 publications

References 65 publications

Upregulation of Vitamin D binding protein (Gc-globulin) binding sites during neutrophil activation from a latent reservoir in azurophil granules

Upregulation of Vitamin D binding protein (Gc-globulin) binding sites during neutrophil activation from a latent reservoir in azurophil granules

Selective inhibition of the C5a chemotactic cofactor function of the Vitamin D binding protein by 1,25(OH)2 Vitamin D3

Transcriptomic analysis reveal the responses of dendritic cells to VDBP

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