Figure 5
Figure 5. Fludarabine impacts on the growth of MEC1 cells in vitro and in vivo. (A) MEC1 cells were plated in vitro in 48-well plates with increasing concentrations of fludarabine and a luminescent assay was performed 72 hours later to demonstrate MEC1 cells' sensitivity to the drug. EC50 indicates half maximal effective concentration (11.9 g/mL). (B) Tumor growth curves obtained in Rag2−/−γc−/− male mice that received a transplant subcutaneously in the left flank of MEC1 cells (10 × 106). Twenty-one days later, mice bearing MEC1 tumor were randomly assigned to one of the following intraperitoneal treatments (5 animals/group): saline solution (PBS), fludarabine alone (34 mg/kg) daily on days 21 to 25, or fludarabine (0.625 mg/kg) + cyclophosphamide (6.25 mg/kg) daily on days 21 to 23. The treatment was repeated 3 times every 2 weeks. Tumor size was evaluated by measuring perpendicular diameters by a caliper. Animals were killed when the tumor volume reached 1000 mm3. Measurements were stopped when 75% of originally treated mice were still surviving. *Statistically significant differences calculated using the Student t test: day 23, PBS versus fludarabine, P = .01; day 29, PBS versus fludarabine, P = .012, and PBS versus fludarabine + cyclophosphamide, P = .038. Data are representative of at least 2 independent experiments. (C) Kaplan-Meier survival curves for Rag2−/−γc−/− male mice challenged subcutaneously in the left flank with MEC1 cells. Twenty-one days later, mice bearing MEC1 tumor were randomly assigned to one of the following intraperitoneal treatments (5 animals/group): PBS, fludarabine alone (34 mg/kg) daily on days 21 to 25, or fludarabine (0.625 mg/kg) + cyclophosphamide (6.25 mg/kg) daily on days 21 to 23. The treatment was repeated 3 times every 2 weeks. Tumor size was evaluated by measuring perpendicular diameters by a caliper. Animals were killed when the tumor volume reached 1000 mm3.

Fludarabine impacts on the growth of MEC1 cells in vitro and in vivo. (A) MEC1 cells were plated in vitro in 48-well plates with increasing concentrations of fludarabine and a luminescent assay was performed 72 hours later to demonstrate MEC1 cells' sensitivity to the drug. EC50 indicates half maximal effective concentration (11.9 g/mL). (B) Tumor growth curves obtained in Rag2−/−γc−/− male mice that received a transplant subcutaneously in the left flank of MEC1 cells (10 × 106). Twenty-one days later, mice bearing MEC1 tumor were randomly assigned to one of the following intraperitoneal treatments (5 animals/group): saline solution (PBS), fludarabine alone (34 mg/kg) daily on days 21 to 25, or fludarabine (0.625 mg/kg) + cyclophosphamide (6.25 mg/kg) daily on days 21 to 23. The treatment was repeated 3 times every 2 weeks. Tumor size was evaluated by measuring perpendicular diameters by a caliper. Animals were killed when the tumor volume reached 1000 mm3. Measurements were stopped when 75% of originally treated mice were still surviving. *Statistically significant differences calculated using the Student t test: day 23, PBS versus fludarabine, P = .01; day 29, PBS versus fludarabine, P = .012, and PBS versus fludarabine + cyclophosphamide, P = .038. Data are representative of at least 2 independent experiments. (C) Kaplan-Meier survival curves for Rag2−/−γc−/− male mice challenged subcutaneously in the left flank with MEC1 cells. Twenty-one days later, mice bearing MEC1 tumor were randomly assigned to one of the following intraperitoneal treatments (5 animals/group): PBS, fludarabine alone (34 mg/kg) daily on days 21 to 25, or fludarabine (0.625 mg/kg) + cyclophosphamide (6.25 mg/kg) daily on days 21 to 23. The treatment was repeated 3 times every 2 weeks. Tumor size was evaluated by measuring perpendicular diameters by a caliper. Animals were killed when the tumor volume reached 1000 mm3.

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