Figure 2
Figure 2. CXCL4 and CXCL4L1 expression by HEK-293 and HMVEC transfectants. (A) CXCL4 and CXCL4L1 mRNA expression by HEK-293 transfectants, as assessed by real-time qRT-PCR. Columns represent mean values (± SEM) of 10 selected clones. (B) Expression of CXCL4/CXCL4L1 in HEK-293 transfectants, as detected by immunofluorescence. Absence of signal in mock transfectants (left), strong cytoplasmic signal in CXCL4 transfectants (green, middle panel), staining in a region adjacent to plasmatic membrane in CXCL4L1 transfectants (green, right). Bar represents 50 μm. (C) High-power magnification of immunofluorescence performed on CXCL4 (left) or CXCL4L1 transfectants (right). Bar represents 20 μm. (D) Confocal microscopy of HMVECs transfected with CXCL4-GFP. GFP fluorescence (green) was localized in the cytoplasm; concanavalin A stains the membrane (red). Merged image (yellow) demonstrates absence of coexpression; bar represents 20 μm. At the extreme part of the figure a high-power magnification of a detail of the merged image is shown; bar represents 5 μm. (E) Confocal microscopy of HMVECs transfected with CXCL4L1-GFP. GFP fluorescence (green) was localized in the cytoplasm and on cytoplasmic membrane, as demonstrated by merged image (yellow; bar represents 20 μm). At the extreme part of the figure a high-power magnification of a detail of the merged image is shown (bar represents 5 μm). Images in panels B and C were acquired using an LSM 510 Meta confocal microscope (Zeiss) equipped with a 20 ×/0.50 NA Plan-Neofluor objective lens (Zeiss). Images in panel D and E were acquired using an LSM 510 Meta laser scanning confocal microscope equipped with a 40×/1.30 NA oil Plan-Neofluor objective lens. An electronic zoom is shown in the extreme panel. LSM 510 Meta confocal microscope software version 3.0 (Zeiss) was used to capture all the images.

CXCL4 and CXCL4L1 expression by HEK-293 and HMVEC transfectants. (A) CXCL4 and CXCL4L1 mRNA expression by HEK-293 transfectants, as assessed by real-time qRT-PCR. Columns represent mean values (± SEM) of 10 selected clones. (B) Expression of CXCL4/CXCL4L1 in HEK-293 transfectants, as detected by immunofluorescence. Absence of signal in mock transfectants (left), strong cytoplasmic signal in CXCL4 transfectants (green, middle panel), staining in a region adjacent to plasmatic membrane in CXCL4L1 transfectants (green, right). Bar represents 50 μm. (C) High-power magnification of immunofluorescence performed on CXCL4 (left) or CXCL4L1 transfectants (right). Bar represents 20 μm. (D) Confocal microscopy of HMVECs transfected with CXCL4-GFP. GFP fluorescence (green) was localized in the cytoplasm; concanavalin A stains the membrane (red). Merged image (yellow) demonstrates absence of coexpression; bar represents 20 μm. At the extreme part of the figure a high-power magnification of a detail of the merged image is shown; bar represents 5 μm. (E) Confocal microscopy of HMVECs transfected with CXCL4L1-GFP. GFP fluorescence (green) was localized in the cytoplasm and on cytoplasmic membrane, as demonstrated by merged image (yellow; bar represents 20 μm). At the extreme part of the figure a high-power magnification of a detail of the merged image is shown (bar represents 5 μm). Images in panels B and C were acquired using an LSM 510 Meta confocal microscope (Zeiss) equipped with a 20 ×/0.50 NA Plan-Neofluor objective lens (Zeiss). Images in panel D and E were acquired using an LSM 510 Meta laser scanning confocal microscope equipped with a 40×/1.30 NA oil Plan-Neofluor objective lens. An electronic zoom is shown in the extreme panel. LSM 510 Meta confocal microscope software version 3.0 (Zeiss) was used to capture all the images.

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