![Figure 2. CXCL12 binds to CXCR7 in PB CD34+ cells. Fresh PB CD34+ cells were incubated in serum- and cytokine-free medium supplemented with CXCL12AF647 (10 ng/mL) for 3 hours and CXCL12-, CXCL11-, CXCR4-, and/or CXCR7- (9C4 and 11G8) blocking antibodies, CXCR7 inhibitors, isotype controls, or CCX704 control. Analysis was performed on a BD Fortessa flow cytometer. (A) Histograms show CXCL12AF647 binding CD34+ cells in each condition. Results are representative of 1 experiment of the 3 performed. (B) Histograms show MFI of cells determined by a BD Fortessa flow cytometer in each experimental condition and expressed as mean ± SD (n = 4). Control was normalized at 100 arbitrary units in each experimental condition. (C) Histograms illustrate CXCL12AF647 binding inhibition in CD34+ cells for each condition. The percentage of CXCL12AF647 binding inhibition was determined using the formula previously described24: (1−[MFI−MFINC]/[MFIPC−MFINC])*100. MFI corresponds to mean fluorescence intensity of cells incubated with CXCL12AF647 and CXCL12, CXCL11, CXCR4, and/or CXCR7 (9C4 and 11G8) blocking antibodies or CXCR7 inhibitors; MFIPC to the cells incubated with CXCL12AF647 and respective controls; and MFINC to cell autofluorescence. Asterisks indicate significance vs control conditions (*P ≤ .05, **P ≤ .01, ***P ≤ .001). Deltas indicate significance between experimental conditions (ΔP ≤ .05, ΔΔP ≤ .01, ΔΔΔP ≤ .001).](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/123/2/10.1182_blood-2013-05-500496/4/191f2.jpeg?Expires=1723181069&Signature=Zf4YAEcBUexzAydU9uLhHllEiaZ1KeSnxC0g0vB6XyOdhbSzL7dyG5QR8S89hW~wms0mv3ybonY3ojTtMqHh5upacpnINFZVyLhptWjwRLLWVm6ONlhxi0f~4Un7dpXtTS3pGb7aBM56OghARjNs6CB6nrzfqFKK35L3jbh8gHG7AWP8lvtbqCrxLZLcw2kAnu2GDOF3qArwC5kNRD~9EkMCn8h2DypAh5Z3NXA-9RhbT1RnSoF~VFhL4xaK6dqHb8JulLoedwemfjb93oVxuUKSD5CybDHqpudsihZd1PRaGSxbY~WLTDy7bHqQ9Nf5bbjXNFuiGCWZ8NFVhVLjmQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
CXCL12 binds to CXCR7 in PB CD34+cells. Fresh PB CD34+ cells were incubated in serum- and cytokine-free medium supplemented with CXCL12AF647 (10 ng/mL) for 3 hours and CXCL12-, CXCL11-, CXCR4-, and/or CXCR7- (9C4 and 11G8) blocking antibodies, CXCR7 inhibitors, isotype controls, or CCX704 control. Analysis was performed on a BD Fortessa flow cytometer. (A) Histograms show CXCL12AF647 binding CD34+ cells in each condition. Results are representative of 1 experiment of the 3 performed. (B) Histograms show MFI of cells determined by a BD Fortessa flow cytometer in each experimental condition and expressed as mean ± SD (n = 4). Control was normalized at 100 arbitrary units in each experimental condition. (C) Histograms illustrate CXCL12AF647 binding inhibition in CD34+ cells for each condition. The percentage of CXCL12AF647 binding inhibition was determined using the formula previously described24 : (1−[MFI−MFINC]/[MFIPC−MFINC])*100. MFI corresponds to mean fluorescence intensity of cells incubated with CXCL12AF647 and CXCL12, CXCL11, CXCR4, and/or CXCR7 (9C4 and 11G8) blocking antibodies or CXCR7 inhibitors; MFIPC to the cells incubated with CXCL12AF647 and respective controls; and MFINC to cell autofluorescence. Asterisks indicate significance vs control conditions (*P ≤ .05, **P ≤ .01, ***P ≤ .001). Deltas indicate significance between experimental conditions (ΔP ≤ .05, ΔΔP ≤ .01, ΔΔΔP ≤ .001).
