Figure 7
Exofucosylation (GPS) of mouse LSK cells enforces HCELL expression, yielding higher E-selectin binding and increased homing to marrow. (A) Flow cytometric analysis of E-Ig binding on BT-LSK and GPS-treated LSK (GPS-LSK) cells. EDTA control displayed a mean fluorescence intensity = 3.1. Results displayed are representative of at least n = 5 flow cytometric experiments. (B) GPS-LSK and BT-LSK cells were lysed, and Western blot analysis was performed on whole cell lysates and blotted with E-selectin and CD44. (C) CD44 was immunoprecipitated (with IM7 and KM114) from equivalent amounts of cell lysates from GPS-treated (+) or untreated (−) mouse LSK cell lysates that had been either treated with N-glycosidase F (+) or not (−). Immunoprecipitates were then electrophoresed and blotted with E-Ig and CD44. Staining with E-Ig was performed in the presence of Ca2+. (D) GPS-LSK (black bars) or BT-LSK (white bars) were labeled reciprocally with CFDA-SE and/or CTO and injected intravenously in a 1:1 ratio competitively into C57BL6 mice. Bone marrow was analyzed 16 hours after the injection to determine the percentage of carboxyfluorescein succinimidyl ester and CTO-positive cells present within a defined gate-representing mouse LSK cells. Mice that did not receive cells were used to determine the background signal. Error bars represent the SEM. Data are representative of 6 mice. Parallel control experiments measuring the competition of BT cells to untreated cells did not show any advantage or disadvantage of either cell type (supplemental Figure 4).

Exofucosylation (GPS) of mouse LSK cells enforces HCELL expression, yielding higher E-selectin binding and increased homing to marrow. (A) Flow cytometric analysis of E-Ig binding on BT-LSK and GPS-treated LSK (GPS-LSK) cells. EDTA control displayed a mean fluorescence intensity = 3.1. Results displayed are representative of at least n = 5 flow cytometric experiments. (B) GPS-LSK and BT-LSK cells were lysed, and Western blot analysis was performed on whole cell lysates and blotted with E-selectin and CD44. (C) CD44 was immunoprecipitated (with IM7 and KM114) from equivalent amounts of cell lysates from GPS-treated (+) or untreated (−) mouse LSK cell lysates that had been either treated with N-glycosidase F (+) or not (−). Immunoprecipitates were then electrophoresed and blotted with E-Ig and CD44. Staining with E-Ig was performed in the presence of Ca2+. (D) GPS-LSK (black bars) or BT-LSK (white bars) were labeled reciprocally with CFDA-SE and/or CTO and injected intravenously in a 1:1 ratio competitively into C57BL6 mice. Bone marrow was analyzed 16 hours after the injection to determine the percentage of carboxyfluorescein succinimidyl ester and CTO-positive cells present within a defined gate-representing mouse LSK cells. Mice that did not receive cells were used to determine the background signal. Error bars represent the SEM. Data are representative of 6 mice. Parallel control experiments measuring the competition of BT cells to untreated cells did not show any advantage or disadvantage of either cell type (supplemental Figure 4).

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