Figure 1
Figure 1. FTVI treatment increases Treg fucosylation. Fucosylation is characterized by the presence of sLeX residues, as assessed by flow cytometry, with antibody HECA-452 (BD Biosciences, San Jose, CA), raised against CLA, shown to be sLeX30. The left side of each contour plot shows the isotype control, and the right side the results of staining (percentage CLA-positive cells). (A) Positive control. CB CD34+ cells show an endogenous rate of 56.5% CLA+ cells that increases to 100% on treatment with FTVI enzyme. (B) Expanded Tregs. Untreated ex vivo-expanded Tregs show minimal endogenous fucosylation of 6.6% that increases to 65.5% on treatment with FTVI. (C) Fucosylation of Tregs leads to increased ability to bind E-selectin ligand. Expanded Tregs were treated with FTVI enzyme for 30 minutes, followed by biotin CLA–streptavidin phycoerythrin. Unlabeled selectins (E, P, L) with APC anti-Fc were used to study selectin binding ability in untreated Tregs (left) or fucosylated Tregs (right). Significant increase in the binding ability of fucosylated Tregs to E-selectin ligand was demonstrated (41% vs 2%) (upper). A high level of endogenous expression of P-selectin ligand was seen in untreated Tregs (81.7%) that increased on fucosylation (92.9%) (lower). No change was seen in the total L-selectin ligand expression (middle). (D) Increased E-selectin binding in fucosylated Tregs. Average values from 3 independent experiments show that the extent of fucosylation is related to the binding ability of E-, P-, or L- selectin. (E) Fucosylated Tregs suppress immune response in alloMLR similar to untreated Tregs. No differences in the degree of suppression of alloMLR was identified at the varying ratio of T-effector (Teff) and Treg (untreated or fucosylated). The x-axis denotes the varying ratio of Teff:Treg. Y-axis denotes counts per minute (mean ± SEM; n = 3).

FTVI treatment increases Treg fucosylation. Fucosylation is characterized by the presence of sLeX residues, as assessed by flow cytometry, with antibody HECA-452 (BD Biosciences, San Jose, CA), raised against CLA, shown to be sLeX30. The left side of each contour plot shows the isotype control, and the right side the results of staining (percentage CLA-positive cells). (A) Positive control. CB CD34+ cells show an endogenous rate of 56.5% CLA+ cells that increases to 100% on treatment with FTVI enzyme. (B) Expanded Tregs. Untreated ex vivo-expanded Tregs show minimal endogenous fucosylation of 6.6% that increases to 65.5% on treatment with FTVI. (C) Fucosylation of Tregs leads to increased ability to bind E-selectin ligand. Expanded Tregs were treated with FTVI enzyme for 30 minutes, followed by biotin CLA–streptavidin phycoerythrin. Unlabeled selectins (E, P, L) with APC anti-Fc were used to study selectin binding ability in untreated Tregs (left) or fucosylated Tregs (right). Significant increase in the binding ability of fucosylated Tregs to E-selectin ligand was demonstrated (41% vs 2%) (upper). A high level of endogenous expression of P-selectin ligand was seen in untreated Tregs (81.7%) that increased on fucosylation (92.9%) (lower). No change was seen in the total L-selectin ligand expression (middle). (D) Increased E-selectin binding in fucosylated Tregs. Average values from 3 independent experiments show that the extent of fucosylation is related to the binding ability of E-, P-, or L- selectin. (E) Fucosylated Tregs suppress immune response in alloMLR similar to untreated Tregs. No differences in the degree of suppression of alloMLR was identified at the varying ratio of T-effector (Teff) and Treg (untreated or fucosylated). The x-axis denotes the varying ratio of Teff:Treg. Y-axis denotes counts per minute (mean ± SEM; n = 3).

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