Figure 5
Figure 5. Different intracellular localization of CXCL4 and CXCL4L1 in HEK transfectants. (A) Strong expression of CXCL4L1 (green) in the Golgi of CXCL4L1-HEK transfectants, as shown by costaining with the Golgi marker Bodipy (red). Colocalization is shown in yellow (bar represents 20 μm). (B) Virtually absent colocalization between the DCG marker VAMP-1/2/3 (red) and CXCL4L1 (green) in CXCL4L1-HEK transfectants. Colocalization is shown in yellow (bar represents 20 μm). (C) Absence of any effect of PMA treatment in CXCL4L1-HEK transfectants on CXCL4L1 (green) distribution and localization (bar represents 20 μm). (D) Marginal colocalization of CXCL4 (green) with the Golgi marker Bodipy (red) in CXCL4-HEK transfectants. Colocalization is shown in yellow (bar represents 20 μm). (E) Localization of CXCL4 (green) within DCGs in CXCL4-HEK transfectants, as demonstrated by strong costaining with the DCG marker VAMP-1/2/3. Colocalization is shown in yellow (bar represents 20 μm). (F) Treatment of CXCL4-HEK transfectants with PMA for 6 hours induces degranulation of CXCL4-containing DCGs. Colocalization of CXCL4 (green) within DCGs of CXCL4-HEK transfectants, as stained with VAMP-1/2/3 is shown in yellow (bar represents 20 μm). Images were acquired using an LSM 510 Meta confocal microscope (Zeiss) equipped with a 20×/0.50 Plan-Neofluor objective lens (Zeiss). LSM 510 Meta confocal microscope software version 3.0 (Zeiss) was used to capture all the images.

Different intracellular localization of CXCL4 and CXCL4L1 in HEK transfectants. (A) Strong expression of CXCL4L1 (green) in the Golgi of CXCL4L1-HEK transfectants, as shown by costaining with the Golgi marker Bodipy (red). Colocalization is shown in yellow (bar represents 20 μm). (B) Virtually absent colocalization between the DCG marker VAMP-1/2/3 (red) and CXCL4L1 (green) in CXCL4L1-HEK transfectants. Colocalization is shown in yellow (bar represents 20 μm). (C) Absence of any effect of PMA treatment in CXCL4L1-HEK transfectants on CXCL4L1 (green) distribution and localization (bar represents 20 μm). (D) Marginal colocalization of CXCL4 (green) with the Golgi marker Bodipy (red) in CXCL4-HEK transfectants. Colocalization is shown in yellow (bar represents 20 μm). (E) Localization of CXCL4 (green) within DCGs in CXCL4-HEK transfectants, as demonstrated by strong costaining with the DCG marker VAMP-1/2/3. Colocalization is shown in yellow (bar represents 20 μm). (F) Treatment of CXCL4-HEK transfectants with PMA for 6 hours induces degranulation of CXCL4-containing DCGs. Colocalization of CXCL4 (green) within DCGs of CXCL4-HEK transfectants, as stained with VAMP-1/2/3 is shown in yellow (bar represents 20 μm). Images were acquired using an LSM 510 Meta confocal microscope (Zeiss) equipped with a 20×/0.50 Plan-Neofluor objective lens (Zeiss). LSM 510 Meta confocal microscope software version 3.0 (Zeiss) was used to capture all the images.

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