Fig. 4.
Fig. 4. Effect of SDF-1 on HHV-7 infection. (A) SDF-1–dependent CXCR4 downmodulation (left panel) and inhibition of HHV-7 infection (right panel). SupT1 cells were preincubated with SDF-1 (2.5 μg/mL) for 30 minutes at room temperature and then either remained uninfected or inoculated with HHV-7. Before HHV-7–infection, surface CXCR4 was analyzed by flow cytometry (left panel). Horizontal axis, surface CXCR4 expression detected by PE fluorescence intensity; vertical axis, relative cell number. Negative control (Cont) is represented by cells stained with irrelevant isotype-matched control MoAb. The right panel shows HHV-7 expression determined by specific RT-PCR in SupT1 cells preincubated with nothing (lane 1), 2.5 μg/mL of SDF-1 (lane 2), 25 μg/mL of control mouse IgG2a (lane 3), and 25 μg/mL of 12G5 anti-CXCR4 MoAb (lane 4). Equivalent amounts of RNA, extracted at 40 hours PI, were used as template for RT-PCR using either HHV-7–specific primers (U10 ORF) or β-actin primers. Control reaction, performed by amplifying the same RNA samples before RT (−RT) is also shown; lane BL, blank. The data are representative of three separate experiments. (B) CD4+ SupT1 or CD4− BC7 cells were inoculated with HHV-7 and monitored for HHV-7 expression and replication by specific viral RT-PCR at 40 hours PI (left panels) and by indirect immunofluorescence at 8 days PI (microphotographs). For RT-PCR, equivalent amounts of RNA samples, before (−) and after (+) RT, were used as template for the amplification reactions. PCR products for HHV-7/U10 ORF and β-actin are shown; lane BL, blank. Immunofluorescence microscopy was performed as described by using the 5E1 HHV-7–specific MoAb; negative reactions are counterstained with Evans blue. The data are representative of three experiments from separate infections.

Effect of SDF-1 on HHV-7 infection. (A) SDF-1–dependent CXCR4 downmodulation (left panel) and inhibition of HHV-7 infection (right panel). SupT1 cells were preincubated with SDF-1 (2.5 μg/mL) for 30 minutes at room temperature and then either remained uninfected or inoculated with HHV-7. Before HHV-7–infection, surface CXCR4 was analyzed by flow cytometry (left panel). Horizontal axis, surface CXCR4 expression detected by PE fluorescence intensity; vertical axis, relative cell number. Negative control (Cont) is represented by cells stained with irrelevant isotype-matched control MoAb. The right panel shows HHV-7 expression determined by specific RT-PCR in SupT1 cells preincubated with nothing (lane 1), 2.5 μg/mL of SDF-1 (lane 2), 25 μg/mL of control mouse IgG2a (lane 3), and 25 μg/mL of 12G5 anti-CXCR4 MoAb (lane 4). Equivalent amounts of RNA, extracted at 40 hours PI, were used as template for RT-PCR using either HHV-7–specific primers (U10 ORF) or β-actin primers. Control reaction, performed by amplifying the same RNA samples before RT (−RT) is also shown; lane BL, blank. The data are representative of three separate experiments. (B) CD4+ SupT1 or CD4 BC7 cells were inoculated with HHV-7 and monitored for HHV-7 expression and replication by specific viral RT-PCR at 40 hours PI (left panels) and by indirect immunofluorescence at 8 days PI (microphotographs). For RT-PCR, equivalent amounts of RNA samples, before (−) and after (+) RT, were used as template for the amplification reactions. PCR products for HHV-7/U10 ORF and β-actin are shown; lane BL, blank. Immunofluorescence microscopy was performed as described by using the 5E1 HHV-7–specific MoAb; negative reactions are counterstained with Evans blue. The data are representative of three experiments from separate infections.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal