Mice harboring the heterozygous Cxcr4^+/1013 mutation were generated as previously described (15, 16, 25). This mouse model was selected because it bears a point mutation in the second exon of Cxcr4, which is frequently observed in patients with WHIM syndrome, and was inserted using a knock-in strategy. Littermate wild type (WT) mice were used as controls in all experiments. All mice were 8 -16 weeks old. Daily observation was performed to ensure that no animal was left in a state of pain or suffering during experimentation.

All in vivo mouse experiments were conducted at Université Paris Cité, Institut de Recherche Saint-Louis (Paris, France) from March 2022 to May 2023. Studies were conducted in compliance with the European Union guide for the care and use of laboratory animals, which have been reviewed and approved by an institutional review committee (Comité d’éthique Paris-Nord N°121, France).

Cxcr4^+/1013 and Cxcr4^WT mice received CXCR4 antagonist X4-185 at 10 mg/kg/day (X4 Pharmaceuticals) (17, 26) or vehicle daily for 7 or 28 days in a row (5 days on/2 days off). Vehicle only was given as control in all experiments (H20-NaCl-0.4% pH4 or phosphate-buffered saline [PBS]). X4-185 is an orally bioavailable, small molecule CXCR4 antagonist of molecular weight ~400 g/mol. In internal control experiments, mice were injected intraperitoneally with plerixafor (AMD3100) (5 mg/kg/day) (Sigma-Aldrich, Darmstadt, Germany) for 21 days (15, 25, 27). Mice were bled 7 days before the start of the experiments, 3 hours after the first dose, then every 7 days 3 hours after the dose. Euthanasia was performed by increasing gradient of CO₂. At sacrifice, BM, spleens, and blood were harvested and processed for numeration on an MS9-5 counter (Melet Schloesing, Laboratoires, Osny, France), and flow cytometry. BM cells were extracted by centrifugation from intact femurs, tibia, and hips to separate marrow and bone fractions. Spleens were manually isolated. Cell collection was performed in PBS supplemented with 2% fetal bovine serum and filtered through a 70-μm nylon strainer to remove debris and fat. The peripheral blood was collected by submandibular puncture. Red blood cell lysis was performed using an ammonium-chloride-potassium buffer.

Single cell suspensions were stained with appropriate antibodies in PBS supplemented with 2% bovine serum albumin and 2 mM ethylenediaminetetraacetic acid for cell surface staining. The list of antibodies used in the study is shown in Supplementary Table S1 . Analyses were carried out on an LSRII Fortessa flow cytometer (BD Biosciences, Franklin Lakes, NJ, USA), and data were analyzed with the FlowJo software (TreeStar, Ashland, OR, USA).

To determine Reactive Oxygen Species (ROS) levels, whole blood was loaded with 0.5 µg/mL Dihydrorodamine 123 (cat#D1054, Sigma-Aldrich) and incubated for 15 minutes at 37°C. Subsequently, 200 nM phorbol 12-myristate 13-acetate was added, and the samples were incubated for an additional 45 minutes at 37°C to induce the ROS production. For unstimulated samples, incubation with PBS was performed. Then, 2 mL of red blood cell lysis buffer was added, and the mixture was incubated at room temperature. After 10 minutes, the reaction was halted by adding 4 mL of PBS, and samples were centrifuged at 200 g for 5 minutes. The red blood cell lysis procedure was repeated a second time. The fluorescence levels were measured using flow cytometry (BD FACSCanto™ II, BD Biosciences). The gating strategy of granulocytes was based on forward and side scatter plots of the lysed whole blood.

To quantify phagocytic activity, pHrodo™ BioParticles™ Conjugates for Phagocytosis (Cat# P35367, Thermo Fisher Scientific, Waltham, MA, USA) was used. Whole blood was incubated with pHrodo BioParticles for 15 minutes at 37°C. Negative controls were incubated for 15 minutes on ice. Then, all the samples were placed on ice to stop the uptake process. Subsequently, 2 mL of red blood cell lysis buffer was added, and the mixture was incubated on ice for 15 minutes. The reaction was halted by adding 4 mL of PBS and samples were centrifuged at 200 g for 5 minutes. The fluorescence levels were measured using flow cytometry (BD FACSCanto™ II). The gating strategy of granulocytes was based on forward and side scatter plots of the lysed whole blood.

The data were presented as mean ± standard error of the mean (SEM) and the number of mice per experiments was indicated in the figure legends. All statistical analyses were conducted using Prism software (GraphPad Software, Boston, MA, USA). The significance of differences between two independent groups was calculated using Mann-Whitney test. P values <0.05 were considered statistically significant.

It was shown that transient inhibition of CXCR4 signaling reversed circulating leukopenia in Cxcr4^+/1013 mice (15). However, whether CXCR4 antagonism durably corrects leukopenia in Cxcr4^+/1013 mice following chronic administration has not been investigated. To this end, Cxcr4^+/1013 and littermate WT mice were treated with vehicle or the orally bioavailable CXCR4 antagonist X4-185 by daily gavage at 10 mg/kg/day for 7 days, and blood cell counts were measured 3 hours after the last dose ( Figure 1A ). Cxcr4^+/1013 mice exhibited profound circulating panleukopenia, with lymphocytes being the most impacted leukocyte subtype. Specifically, Cxcr4^+/1013 mice had 75%, 80%, 56% and 66% fewer leukocytes, lymphocytes, granulocytes, and monocytes, respectively, than their WT littermates ( Figures 1B–E ). Membrane expression levels of CXCR4 on neutrophils, B cells, CD4⁺-T cells and CD8⁺-T cells from peripheral blood and BM were similar between Cxcr4^+/1013 and WT mice ( Supplementary Figures S1A, B ), in line with our previous reports (15). This finding suggests that peripheral blood leukopenia observed in Cxcr4 ^+/1013 mice is likely due to CXCR4 GOF rather than changes in CXCR4 expression. CXCR4 antagonism led to a significant increase in absolute number of all these subsets in Cxcr4^+/1013 mice ( Figures 1B–E ; Table 1 ). While CXCR4 antagonism corrected peripheral blood leukopenia in Cxcr4^+/1013 mice ( Figures 1B–E ), it did not appear to affect the count of red blood cells or platelets in both Cxcr4^+/1013 and WT mice ( Supplementary Figures S2A, B ).

Altogether, these results indicate that CXCR4 antagonism corrected the peripheral blood leukopenia in Cxcr4^+/1013 mice.

Next, we explored the effect of CXCR4 antagonism on granulopoiesis and neutrophil function. Cxcr4^+/1013 mice were neutropenic, displaying 61% less circulating mature neutrophils than WT mice ( Figure 2A ). The observed neutropenia in Cxcr4^+/1013 mice was not associated with defective granulocyte maturation nor accumulation of mature neutrophils in the BM ( Figure 2B ). Treatment with CXCR4 antagonist significantly increased the number of mature neutrophils in the blood of Cxcr4^+/1013 mice ( Figure 2A ; Table 1 ) while, in parallel, decreased the number of mature neutrophils in BM ( Figure 2B ). A similar tendency was observed in WT mice. These findings support BM as an important reservoir for CXCR4 antagonist-mobilized neutrophils, in line with other reports (27, 28). It is worth noting that treatment with CXCR4 antagonist did not affect granulocyte subset cell counts (promyelocytes, myelocytes and metamyelocytes) in BM of both Cxcr4^+/1013 and WT mice, indicating that neutrophil differentiation and maturation remained intact during treatment ( Figure 2B ).

At the functional level, blood Cxcr4^+/1013 neutrophils exhibited similar capacities to conduct phagocytosis of S. aureus BioParticles or to produce ROS compared to their WT counterparts, and these functions were not altered with CXCR4 antagonist treatment ( Figures 2C, D ). These findings support the notion that the enhanced risk of recurrent infections due to pathogenic bacteria in patients with WHIM syndrome is driven by their low leukocyte counts in peripheral blood rather than reduction of phagocytic or ROS neutrophil functions.

Altogether, these results show that CXCR4 antagonism corrected peripheral blood neutropenia and mobilized functional neutrophils, likely from the BM, without impairing BM granulopoiesis in Cxcr4^+/1013 mice.

CXCR4 GOF mutations are associated with T-cell lymphopenia in mice, which may result from alteration in T-cell trafficking through secondary lymphoid organs and/or accumulation of T cells in primary lymphoid organs (15–18). It has been shown that transient blockade of CXCR4 signaling resulted in a reversion of circulating T-cell lymphopenia in Cxcr4^+/1013 mice (15, 18). However, the impact of CXCR4 antagonism on T cell abnormalities within the secondary lymphoid organs of this WHIM mouse model has not been thoroughly investigated. In the current study, we focused on investigating whether chronic administration of CXCR4 antagonist could modulate T-cell abnormalities in the spleen and peripheral blood of Cxcr4^+/1013 mice. In agreement with a recent report (18), Cxcr4^+/1013 mice exhibited severe T-cell lymphopenia that affected more CD8⁺ than CD4⁺ T cells, which were reduced by 82% and 55%, respectively, compared with WT mice ( Figures 3A, B ; Supplementary Figures S3A, B ). Accordingly, circulating CD4/CD8 T-cell ratios were increased by ~3-fold in Cxcr4^+/1013 mice compared to WT mice ( Figure 3C ; Supplementary Figure S3C ). CXCR4 antagonism corrected peripheral blood CD4⁺ and CD8⁺ T-cell lymphopenia in these mice and even restored the circulating CD4/CD8 T-cell ratios to WT levels after 7 days ( Supplementary Figures S3A–C ; Table 1 ) and 28 days of treatment ( Figures 3A–C ).

Next, we quantified CD4⁺ and CD8⁺ T cells in the spleen of WT and Cxcr4^+/1013 mice. Cxcr4^+/1013 mice had lower CD8⁺ T-cell numbers in the spleen, while CD4⁺ T-cell numbers remained unchanged ( Figures 3D, E ; Supplementary Figures S3D, E ). Splenic CD4/CD8 T-cell ratios were also increased by ~1.4-fold compared with WT mice ( Figure 3F ; Supplementary Figure S3F ). Treatment with CXCR4 antagonist for 7 days did not appear to modulate splenic T cell abnormalities ( Supplementary Figures S3D, E ). However, prolonged CXCR4 antagonism for 28 days normalized splenic CD8-T cell numbers in Cxcr4^+/1013 mice and restored splenic CD4/CD8 T-cell ratios to WT levels ( Figures 3E, F ). In contrast, this prolonged treatment had no impact on splenic T-cell composition in WT mice ( Figures 3D–F ).

Our data thus indicate that prolonged CXCR4 antagonism can correct splenic T-cell abnormalities and normalize T-cell lymphopenia in peripheral blood in Cxcr4^+/1013 mice.

CXCR4 GOF mutations alter B-cell development and trafficking resulting in B-cell lymphopenia in mice (15–17). Consistent with these observations, we found that Cxcr4^+/1013 mice had severe B-cell lymphopenia in peripheral blood ( Figure 4A ). Treatment with a CXCR4 antagonist for 7 days resulted in an increased B-cell count in Cxcr4^+/1013 mice that reached levels seen in WT mice ( Figure 4A ; Table 1 ). Consistent with a previous report (15), IgM levels were slightly higher in Cxcr4^+/1013 mice compared to WT mice, while IgG1 levels were comparable to those in WT mice. Chronic treatment with CXCR4 antagonist had no significant impact on IgM and IgG1 levels ( Supplementary Figures S4A, B ).

The observed normalization of circulating B-cell count following CXCR4 antagonist treatment may result from correction of defective B-cell development and/or redistribution of B cells from primary and secondary lymphoid organs. An analysis of spleens from Cxcr4^+/1013 mice revealed multiple defects, including decreased spleen weight (~42%), cellularity (39%) and total B cell count (17%) compared with WT mice ( Supplementary Figures S5A, B ; Figure 4B ) (15). Chronic dosing with CXCR4 antagonist (28-days of treatment) rescued total splenic B -cell number in Cxcr4^+/1013 mice to levels observed in WT mice ( Figure 4B ).

It is well established that immature B cells migrating from the BM emerge in the spleen as transitional B cells and further develop into mature marginal zone (MZ) and follicular (FO) B cells (15). We questioned whether this process and distribution of B-cells were defective in Cxcr4^+/1013 mice and whether CXCR4 antagonism could correct any related defects observed. As previously reported (15), the frequency and number of FO B cells in Cxcr4^+/1013 mice were reduced by >50% compared with WT mice ( Figures 4C, E ). In contrast, the frequency and number of MZ B cells in Cxcr4^+/1013 mice were significantly increased compared with WT mice ( Figures 4D, F ). Chronic treatment with the oral CXCR4 antagonist X4-185 for 28 days resulted in correction of both frequency and absolute number of FO and MZ B cells to levels seen in WT mice ( Figures 4C–F ). Reminiscent of previous works (17, 27), no changes in the frequency and counts of splenic FO and MZ B cell were observed in the spleen of WT mice. Interestingly, chronic treatment with plerixafor (AMD3100), an injectable CXCR4 antagonist that has a shorter receptor occupancy time and more limited tissue distribution (as measured by volume of distribution) compared with the orally bioavailable CXCR4 antagonist X4-185 ( Supplementary Table S2 ; Supplementary Figure S6 ), was unable to correct splenic FO and MZ B-cell defects observed in Cxcr4^+/1013 mice over a 21-day treatment period ( Supplementary Figures S7A–D ).

These data demonstrate that prolonged treatment with CXCR4 antagonist X4-185 corrected splenic B-cell abnormalities in Cxcr4^+/1013 mice, while normalizing B-cell lymphopenia in the peripheral blood.