S100A10 regulates plasminogen-dependent macrophage invasion

O’Connell, Paul A.; Surette, Alexi P.; Liwski, Robert; Svenningsson, Per; Waisman, David M.

doi:10.1182/blood-2010-01-264754

Cited by 125 publications

(156 citation statements)

References 45 publications

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“…Also, in the absence of MMP9, macrophages were completely unable to respond to Plg for increased 3D invasion and matrix degradation, indicating its importance in the downstream proteolytic events initiated by uPA/Plg. Consistent with our data, Thio-Mw in the presence of Plg generate active MMP9 (63), and if these macrophages are elicited from MMP9 2/2 mice, they fail to respond to Plg for increased 3D invasion (64). In that study, MMP9 2/2 ThioMw had no defect in 3D invasion, which differs from our finding with MMP9 2/2 BMM and with uPA 2/2 Thio-Mw.…”

Section: Discussioncontrasting

confidence: 56%

Urokinase Plasminogen Activator Is a Central Regulator of Macrophage Three-Dimensional Invasion, Matrix Degradation, and Adhesion

Fleetwood

Achuthan

Schultz

et al. 2014

The Journal of Immunology

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Urokinase plasminogen activator (uPA) and its receptor (uPAR) coordinate a plasmin-mediated proteolytic cascade that has been implicated in cell adhesion, cell motility, and matrix breakdown, for example, during inflammation. As part of their function during inflammatory responses, macrophages move through tissues and encounter both two-dimensional (2D) surfaces and more complex three-dimensional (3D) interstitial matrices. Based on approaches employing uPA gene–deficient macrophages, plasminogen supplementation, and neutralization with specific protease inhibitors, it is reported in this study that uPA activity is a central component of the invasion of macrophages through a 3D Matrigel barrier; it also has a nonredundant role in macrophage-mediated matrix degradation. For murine macrophages, matrix metalloproteinase-9 activity was found to be required for these uPA-mediated effects. Evidence for a unique role for uPA in the inverse relationship between macrophage adhesion and 2D migration was also noted: macrophage adhesion to vitronectin was enhanced by uPA and blocked by plasminogen activator inhibitor-1, the latter approach also able to enhance in turn the 2D migration on this matrix protein. It is therefore proposed that uPA can have a key role in the inflammatory response at several levels as a central regulator of macrophage 3D invasion, matrix remodeling, and adhesion.

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Section: Discussioncontrasting

confidence: 56%

Urokinase Plasminogen Activator Is a Central Regulator of Macrophage Three-Dimensional Invasion, Matrix Degradation, and Adhesion

Fleetwood

Achuthan

Schultz

et al. 2014

The Journal of Immunology

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“…This suggestion is currently under investigation in our laboratory. Several Plg receptors have been shown to participate in Plainduced migration in vivo and in vitro (12)(13)(14)(15)45). These receptors have two common properties: they possess a carboxyl-terminal lysine residue that can bind Plg and they are not transmembrane proteins but become expressed on the cell surface by yet undefined pathways (46).…”

Section: Discussionmentioning

confidence: 99%

Plasmin Induces In Vivo Monocyte Recruitment through Protease-Activated Receptor-1–, MEK/ERK-, and CCR2-Mediated Signaling

Carmo

Costa

Vago

et al. 2014

The Journal of Immunology

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The plasminogen (Plg)/plasmin (Pla) system is associated with a variety of biological activities beyond the classical dissolution of fibrin clots, including cell migration, tissue repair, and inflammation. Although the capacity of Plg/Pla to induce cell migration is well defined, the mechanism underlying this process in vivo is elusive. In this study, we show that Pla induces in vitro migration of murine fibroblasts and macrophages (RAW 264.7) dependent on the MEK/ERK pathway and by requiring its proteolytic activity and lysine binding sites. Plasmin injection into the pleural cavity of BALB/c mice induced a time-dependent influx of mononuclear cells that was associated with augmented ERK1/2 and IκB-α phosphorylation and increased levels of CCL2 and IL-6 in pleural exudates. The inhibition of protease activity by using a serine protease inhibitor leupeptin or two structurally different protease-activated receptor-1 antagonists (SCH79797 and RWJ56110) abolished Pla-induced mononuclear recruitment and ERK1/2 and IκB-α phosphorylation. Interestingly, inhibition of the MEK/ERK pathway abolished Pla-induced CCL2 upregulation and mononuclear cell influx. In agreement with a requirement for the CCL2/CCR2 axis to Pla-induced cell migration, the use of a CCR2 antagonist (RS504393) prevented the Plg/Pla-induced recruitment of mononuclear cells to the pleural cavity and migration of macrophages at transwell plates. Therefore, Pla-induced mononuclear cell recruitment in vivo was dependent on protease-activated receptor-1 activation of the MEK/ERK/NF-κB pathway, which led to the release of CCL2 and activation of CCR2.

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“…41 Analysis of cell surface ANXA2 has identified intact ANXA2 but failed to observe any truncated ANXA2. 37,39,40 Recently, we examined the molecular weight forms of ANXA2 at the endothelial cell surface by Western blotting. 41 Although native ANXA2 was easily detected, we were unable to detect any lower molecular weight (truncated) forms of ANXA2.…”

Section: The Role Of Anxa2 In Fibrinolysismentioning

confidence: 99%

“…34 Shortly after these reports, another group demonstrated the presence of S100A10 on the surface of endothelial cells and the reversible interaction of the C-terminal lysine of S100A10 with both tPA and plasminogen. 35,36 This group established that S100A10 was present in a heterotetrameric complex with ANXA2 on the surface of many cells 35,[37][38][39][40][41] and demonstrated that purified AIIt bound tPA and plasminogen via the C-terminal lysine of the S100A10 subunit without the participation of the ANXA2 subunit. 36,42,43 With the development of methods to deplete cells of ANXA2 and the report of defective fibrinolysis in the ANXA2 knockout mouse, 44 it appeared that ANXA2 might play a role in cellular fibrinolysis.…”

Section: Historical Perspectivementioning

confidence: 99%

The role of the annexin A2 heterotetramer in vascular fibrinolysis

Madureira¹,

Surette²,

Phipps³

et al. 2011

Blood

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107

127

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The vascular endothelial cells line the inner surface of blood vessels and function to maintain blood fluidity by producing the protease plasmin that removes blood clots from the vasculature, a process called fibrinolysis. Plasminogen receptors play a central role in the regulation of plasmin activity. The protein complex annexin A2 heterotetramer (AIIt) is an important plasminogen receptor at the surface of the endothelial cell. AIIt is composed of 2 molecules of annexin A2 (ANXA2) bound together by a dimer of the protein S100A10. Recent work performed by our laboratory allowed us to clarify the specific roles played by ANXA2 and S100A10 subunits within the AIIt complex, which has been the subject of debate for many years. The ANXA2 subunit of AIIt functions to stabilize and anchor S100A10 to the plasma membrane, whereas the S100A10 subunit initiates the fibrinolytic cascade by colocalizing with the urokinase type plasminogen activator and receptor complex and also providing a common binding site for both tissue-type plasminogen activator and plasminogen via its C-terminal lysine residue. The AIIt mediated colocalization of the plasminogen activators with plasminogen results in the rapid and localized generation of plasmin to the endothelial cell surface, thereby regulating fibrinolysis. (Blood. 2011;118(18):4789-4797) IntroductionThe vascular endothelium consists of a single cell layer lining all vessels that separates the blood from the tissues. It is estimated to be composed of ϳ 10 13 cells, representing a weight of 1.5 kg and an area of 4000 to 7000 m 2 . 1 Endothelial cells play a role in primary hemostasis, coagulation, fibrinolysis, and regulation of vasomotor tone. In addition to regulating the flow of nutrients, the vascular endothelium regulates many diverse biologically active molecules. These functions of the endothelium are achieved through the presence of membrane-bound receptors for various proteins, lipidtransporting complexes, hormones, and metabolites, as well as through specific extracellular proteins and receptors that regulate cell-cell and cell-matrix interactions. 2 Whereas exposure to inflammatory and/or septic stimuli rapidly leads to procoagulant behavior, unperturbed endothelial cells provide an anticoagulant environment. After vascular insult, endothelial cells express tissue factor and initiate the coagulation cascade that results in thrombin activation and fibrin clot deposition. At the same time, anticoagulant pathways and fibrinolysis are activated to avoid disseminated coagulation and to also limit fibrin accumulation. [3][4][5] Fibrinogen is a large glycoprotein that constitutes the main component of a fibrin clot. Each fibrinogen molecule is composed of 2 sets of A␣-, B␤-, and ␥-polypeptide chains that form a protein containing 2 distal D regions connected to a central E region by a coiled-coil segment. 6 Fibrin is produced on cleavage of the fibrinopeptides by thrombin, which results in the formation of double-stranded half-staggered oligomers that lengthen into protofibrils...

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S100A10 regulates plasminogen-dependent macrophage invasion

Cited by 125 publications

References 45 publications

Urokinase Plasminogen Activator Is a Central Regulator of Macrophage Three-Dimensional Invasion, Matrix Degradation, and Adhesion

Urokinase Plasminogen Activator Is a Central Regulator of Macrophage Three-Dimensional Invasion, Matrix Degradation, and Adhesion

Plasmin Induces In Vivo Monocyte Recruitment through Protease-Activated Receptor-1–, MEK/ERK-, and CCR2-Mediated Signaling

The role of the annexin A2 heterotetramer in vascular fibrinolysis

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