Figure 5
Figure 5. Increased expansion of HSCs in Slug−/− mice after 5-FU treatment. (A) A representation of flow cytometric analysis of Lin−Sca-1+ HSCs in Slug+/+, Slug+/−, and Slug−/− BM 7 days after a single injection of 5-FU (300 mg/kg body weight). (B) The ratio of remaining Lin−Sca-1+ cells at 7 days after 5-FU treatment in 3 groups of mice (Slug+/+ mice, n = 5; Slug+/− mice, n = 4; Slug−/−, n = 5). (C) Total numbers of surviving Lin−Sca-1+ cells 7 days after 5-FU treatment in Slug+/+ (n = 5), Slug+/− (n = 4), and Slug−/− (n = 5) mice. (D) Analysis of apoptotic rate in primitive hematopoietic cell population in BM using an annexin V–based apoptosis assay. BM cells were harvested from Slug−/− and Slug+/+ mice at 0, 3, and 7 days after 5-FU treatment. Primitive hematopoietic cells were gated as Lin−Sca-1+c-Kit+ (for 0 day) or Lin−Sca-1+ (for 3 and 7 days after 5-FU treatment), and the apoptotic cells were identified by a fluorescence-labeled annexin V. Apoptotic primitive hematopoietic cells (annexin V+ Lin−Sca-1+c-Kit+ or annexin V+ Lin−Sca-1+) were analyzed by flow cytometry and represent a percentage. There is no significant difference in the percentage of annexin V+ Lin−Sca-1+c-Kit+ cells (0 day) and annexin V+ Lin−Sca-1+ cells (3 and 7 days after 5-FU treatment) from Slug+/+ and Slug−/− mice. The data shown are the mean of the triplicate. (E) Analysis of Lin−Sca-1+ cell population in S phase. Total BM cells were harvested from Slug+/+ and Slug−/− mice at 5 days after 5-FU treatment and then assayed for Edu incorporation (n = 3). The ratio of Edu+ cell in Lin−Sca-1+ cell population was determined by flow cytometry. All data are expressed as mean ± SD. *P < .05 and **P < .01 for Slug−/− vs Slug+/+.

Increased expansion of HSCs in Slug−/− mice after 5-FU treatment. (A) A representation of flow cytometric analysis of LinSca-1+ HSCs in Slug+/+, Slug+/−, and Slug−/− BM 7 days after a single injection of 5-FU (300 mg/kg body weight). (B) The ratio of remaining LinSca-1+ cells at 7 days after 5-FU treatment in 3 groups of mice (Slug+/+ mice, n = 5; Slug+/− mice, n = 4; Slug−/−, n = 5). (C) Total numbers of surviving LinSca-1+ cells 7 days after 5-FU treatment in Slug+/+ (n = 5), Slug+/− (n = 4), and Slug−/− (n = 5) mice. (D) Analysis of apoptotic rate in primitive hematopoietic cell population in BM using an annexin V–based apoptosis assay. BM cells were harvested from Slug−/− and Slug+/+ mice at 0, 3, and 7 days after 5-FU treatment. Primitive hematopoietic cells were gated as LinSca-1+c-Kit+ (for 0 day) or LinSca-1+ (for 3 and 7 days after 5-FU treatment), and the apoptotic cells were identified by a fluorescence-labeled annexin V. Apoptotic primitive hematopoietic cells (annexin V+ LinSca-1+c-Kit+ or annexin V+ LinSca-1+) were analyzed by flow cytometry and represent a percentage. There is no significant difference in the percentage of annexin V+ LinSca-1+c-Kit+ cells (0 day) and annexin V+ LinSca-1+ cells (3 and 7 days after 5-FU treatment) from Slug+/+ and Slug−/− mice. The data shown are the mean of the triplicate. (E) Analysis of LinSca-1+ cell population in S phase. Total BM cells were harvested from Slug+/+ and Slug−/− mice at 5 days after 5-FU treatment and then assayed for Edu incorporation (n = 3). The ratio of Edu+ cell in LinSca-1+ cell population was determined by flow cytometry. All data are expressed as mean ± SD. *P < .05 and **P < .01 for Slug−/− vs Slug+/+.

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