Figure 3.
Internalization pathways of virus in mature and immature MDDCs. Immature (A,C) and mature (B) MDDCs were incubated with AT-2 HIV-1ADA (3 μg p24/106 DCs, 1 hour at 37°C) and free virus was washed away. The cells were gently resuspended, and approximately 2.5 × 104 cells adhered to alcian blue–treated slides immediately (0 h) or after an additional 2-hour incubation (2 h). Cells were fixed in 4% paraformaldehyde and incubated with biotinylated CD4-IgG2 (Progenics Pharmaceutical) in addition to murine monoclonals specific for MR, DC-SIGN, EEA1, and LAMP-2 at room temperature in the presence of saponin. After washing, bound biotinylated CD4-IgG2 was detected with streptavidin-horseradish peroxidase (HRP) and HRP located using the FITC-TSA amplification kit (green).22 Murine monoclonals were detected with goat antimouse Alexa Fluor 594 (red) and nuclei were stained with DAPI (blue). Overlays of the green and red stains are shown in panels A and B. Separate stains for envelope (env) and LAMP-2 on immature DCs (0 h as an example) are shown in panel C to highlight the limited colocalization of these stains. Original magnification × 100. Double staining for LAMP-2 or MR and envelope was reproduced using 8 different donors, and DC-SIGN and EEA1 repeated with 5 donors. Comparable results were obtained using AT-2 SIV CP-mac–loaded DCs from 2 additional donors (not shown). Murine Ig isotype controls showed no background staining with goat antimouse Alexa Fluor 594 (not shown).

Internalization pathways of virus in mature and immature MDDCs. Immature (A,C) and mature (B) MDDCs were incubated with AT-2 HIV-1ADA (3 μg p24/106 DCs, 1 hour at 37°C) and free virus was washed away. The cells were gently resuspended, and approximately 2.5 × 104 cells adhered to alcian blue–treated slides immediately (0 h) or after an additional 2-hour incubation (2 h). Cells were fixed in 4% paraformaldehyde and incubated with biotinylated CD4-IgG2 (Progenics Pharmaceutical) in addition to murine monoclonals specific for MR, DC-SIGN, EEA1, and LAMP-2 at room temperature in the presence of saponin. After washing, bound biotinylated CD4-IgG2 was detected with streptavidin-horseradish peroxidase (HRP) and HRP located using the FITC-TSA amplification kit (green).22  Murine monoclonals were detected with goat antimouse Alexa Fluor 594 (red) and nuclei were stained with DAPI (blue). Overlays of the green and red stains are shown in panels A and B. Separate stains for envelope (env) and LAMP-2 on immature DCs (0 h as an example) are shown in panel C to highlight the limited colocalization of these stains. Original magnification × 100. Double staining for LAMP-2 or MR and envelope was reproduced using 8 different donors, and DC-SIGN and EEA1 repeated with 5 donors. Comparable results were obtained using AT-2 SIV CP-mac–loaded DCs from 2 additional donors (not shown). Murine Ig isotype controls showed no background staining with goat antimouse Alexa Fluor 594 (not shown).

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