A Role of Kindlin-3 in Integrin αMβ2 Outside-In Signaling and the Syk-Vav1-Rac1/Cdc42 Signaling Axis

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Abstract

Integrins mediate cell-cell and cell-extracellular matrix attachments. Integrins are signaling receptors because their cytoplasmic tails are docking sites for cytoskeletal and signaling proteins. Kindlins are a family of band 4.1-ezrin-radixin-moesin-containing intracellular proteins. Apart from regulating integrin ligand-binding affinity, recent evidence suggests that kindlins are involved in integrin outside-in signaling. Kindlin-3 is expressed in platelets, hematopoietic cells and endothelial cells. In humans, loss of kindlin-3 expression accounts for the rare autosomal disease leukocyte adhesion deficiency (LAD) type III that is characterized by bleeding disorders and defective recruitment of leukocytes into sites of infection. Studies have shown that the loss of kindlin-3 expression leads to poor ligand-binding properties of β1, β2 and β3 integrin subfamilies. The leukocyte-restricted β2 integrin subfamily comprises four members, namely αLβ2, αMβ2, αXβ2 and αDβ2. Integrin αMβ2 mediates leukocyte adhesion, phagocytosis, degranulation and it is involved in the maintenance of immune tolerance. Here we provide further evidence that kindlin-3 is required for integrin αMβ2-mediated cell adhesion and spreading using transfected K562 cells that expressed endogenous kindlin-3 but not β2 integrins. K562 stable cell line expressing si-RNA targeting kindlin-3, but not control-si-RNA, and transfected with constitutively activated integrin αMβ2N329S adhered and spread poorly on iC3b. We also show that kindlin-3 is required for the integrin αMβ2-Syk-Vav1 signaling axis that regulates Rac1 and Cdc42 activities. These findings reinforce a role for kindlin-3 in integrin outside-in signaling. © 2013 Xue et al.

Figures

  • Figure 1. Knockdown of kindlin-3 expression in K562 cells expressing integrin aMb2. (A) qPCR analyses of kindlin-3 mRNA expression level in ctrl-KM and k3-KM cells. (B) Expression levels of kindlin-3 and other proteins in these cells were determined by immunoblotting. Actin was used as loading control. (C) Cell surface expression of integrin aMb2 was determined by flow cytometry. Shaded and open histograms represent control IgG and mAb LPM19c stainings, respectively. GP: gated positive; GM: geo-mean; EI: expression index. (D) To determine extracellular activation of integrin aMb2 on ctrl-KM and k3-KM cells. Cells were treated with Mn2+ (1 mM) or without and stained with mAb KIM127 at 37uC. Control IgG (ctrl-IgG) and mAb LPM19c were included for each condition. The %GP, GM and EI of mAb KIM127 staining are shown. One representative experiment out of two independent experiments is shown. doi:10.1371/journal.pone.0056911.g001
  • Figure 2. Reduced kindlin-3 expression diminished integrin aMb2-mediated cell adhesion. (A) and (B) show adhesion data of ctrl-KM and k3-KM cells on iC3b and BSA, respectively. Each data point represents the mean 6 SD of three independent experiments. mAbs LPM19c and KIM185 were used at 10 mg/ml each. (C) Shear flow analyses of ctrl-KM and k3-KM cells in flow chambers coated with iC3b. Each data point is the mean 6 SD of number of cells in four fields and a representative plot of two independent experiments is shown. doi:10.1371/journal.pone.0056911.g002
  • Figure 3. Kindlin-3 is required for integrin aMb2-mediated cell spreading. ECIS measurements of ctrl-KM and k3-KM cells spreading on iC3b or BSA. Each data point represents the mean 6 SD of technical triplicates at 1 min intervals. mAbs LPM19c and KIM185 were used at 10 mg/ml each. A plot of a representative experiment from three independent experiments is shown for each ligand. doi:10.1371/journal.pone.0056911.g003
  • Figure 4. Kindlin-3 is involved in integrin aMb2 outside-in signaling. (A) Flow cytometry analyses of aMb2N329S in cells transduced with control or kindlin-3-targeting siRNA. Shaded and open histograms represent control IgG and LPM19c stainings, respectively. GP: gated positive; GM: geo-mean; EI: expression index. (B) Cell adhesion assay on iC3b. (C) ECIS measurements on iC3b. In (B) and (C), each data point represents mean 6 SD of technical triplicates. mAb LPM19c was used at 10 mg/ml. (A–C), a single representative experiment from three independent experiments is shown. doi:10.1371/journal.pone.0056911.g004
  • Figure 5. Kindlin-3 regulates the integrin aMb2-Syk-Vav1 signaling axis. KM, ctrl-KM and k3-KM cells were seeded into iC3bcoated TC dishes in the presence of irrelevant mouse IgG (IgG) or mAb KIM185 (10 mg/ml each) and incubated under culture conditions for 30 min. Cells were harvested and lysed followed by immunoprecipitation (IP) using either anti-Syk or anti-Vav1 antibody with mouse IgG or rabbit anti-GST antibody as irrelevant IgG, respectively. Tyr-phosphorylated Syk and Vav1 were probed as described under materials and methods. IB: immunoblotting. A representative experiment from two independent experiments is shown. doi:10.1371/journal.pone.0056911.g005
  • Figure 6. Integrin aMb2-induced RhoGTPase activation involves kindlin-3. Ctrl-KM and k3-KM cells were allowed to adhere to iC3b-coated TC dishes in the presence of mAb KIM185 (10 mg/ml). (A), (C) and (E) are immunoblots of cell lysates for Rac1, Cdc42 and RhoA, respectively. (B), (D) and (F) are pull-down experiments using cell lysates and RBD or PBD-conjugated beads. IB: immunoblotting. A representative experiment from two independent experiments is shown. doi:10.1371/journal.pone.0056911.g006

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Xue, Z. H., Feng, C., Liu, W. L., & Tan, S. M. (2013). A Role of Kindlin-3 in Integrin αMβ2 Outside-In Signaling and the Syk-Vav1-Rac1/Cdc42 Signaling Axis. PLoS ONE, 8(2). https://doi.org/10.1371/journal.pone.0056911

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