Figure 2
Figure 2. Expression of functional integrin αE(CD103)β7 influences the cellular shape and induces filopodia formation in a ligand-dependent fashion in vitro. (A) Wild-type or mutant αE(CD103) subunits were fused to YFP as outlined in “Plasmids.” K562 cells were cotransfected with the wild-type β7 subunit and either wild-type αE(CD103)/YFP, αE-open/YFP, αE-closed/YFP, or YFP alone as indicated. Adhesion experiments (determined as bound cells/20× field, n = 3 experiments) performed on E-cadherin– or FCS-coated surfaces demonstrate the functionality of the integrin αE-YFP-fusion-proteins. (B) K562 cells cotransfected with wild-type αE(CD103)/YFP and β7 subunits were plated on E-cadherin in the presence of a control mAb or a mAb directed against αE(CD103). Images were taken by confocal microscopy in z-stacks (top panels) and phase contrast microscopy (bottom panels). Arrows indicate examples of protrusions/filipodia in the E-cadherin contact zone. (C) The indicated transfectants were seeded on E-cadherin, and the formation of filopodia was monitored by confocal microscopy. The E-cadherin contact zone of a representative cell for each condition is shown. Scale bar = 10 μm. (D) The indicated transfectants were mixed and cocultured with PAM212 keratinocytes. Analysis was performed by confocal microscopy in z-steps of 0.2 to 0.5 μm. One section within the contact zone between the K562 and PAM212 is depicted, in the top row the fluorescence and in the bottom row the phase contrast image of the cells. Arrows indicate examples of protrusions/filopodia extended toward the keratinocytes. Scale bar = 10 μm.

Expression of functional integrin αE(CD103)β7 influences the cellular shape and induces filopodia formation in a ligand-dependent fashion in vitro. (A) Wild-type or mutant αE(CD103) subunits were fused to YFP as outlined in “Plasmids.” K562 cells were cotransfected with the wild-type β7 subunit and either wild-type αE(CD103)/YFP, αE-open/YFP, αE-closed/YFP, or YFP alone as indicated. Adhesion experiments (determined as bound cells/20× field, n = 3 experiments) performed on E-cadherin– or FCS-coated surfaces demonstrate the functionality of the integrin αE-YFP-fusion-proteins. (B) K562 cells cotransfected with wild-type αE(CD103)/YFP and β7 subunits were plated on E-cadherin in the presence of a control mAb or a mAb directed against αE(CD103). Images were taken by confocal microscopy in z-stacks (top panels) and phase contrast microscopy (bottom panels). Arrows indicate examples of protrusions/filipodia in the E-cadherin contact zone. (C) The indicated transfectants were seeded on E-cadherin, and the formation of filopodia was monitored by confocal microscopy. The E-cadherin contact zone of a representative cell for each condition is shown. Scale bar = 10 μm. (D) The indicated transfectants were mixed and cocultured with PAM212 keratinocytes. Analysis was performed by confocal microscopy in z-steps of 0.2 to 0.5 μm. One section within the contact zone between the K562 and PAM212 is depicted, in the top row the fluorescence and in the bottom row the phase contrast image of the cells. Arrows indicate examples of protrusions/filopodia extended toward the keratinocytes. Scale bar = 10 μm.

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