Figure 3
Figure 3. PRELI induces the mitochondrial apoptosis pathway in Th cells and is partly inhibited by IL-4. (A) Overexpression of PRELI induces mitochondria-mediated apoptosis and this is partly counteracted by IL-4. CD4+ cells nucleofected with pIRES-H2Kk or PRELI overexpression vector were sorted and activated as in Figure 2A, cultured with or without IL-4 for 24 hours, and stained and analyzed by flow cytometry. (B) Knockdown of PRELI and IL-4 treatment has additive effects on the mitochondrial apoptosis pathway. CD4+ cells nucleofected with scramble or PRELI-siRNAs were cultured, stained, and analyzed as in panel A. (A,B) Cell viability = PI-negative cells. Bars represent the mean values plus or minus SEM of 4 to 5 independent experiments, except that caspase-3 was measured in 2 independent overexpression experiments that included IL-4 treatment. In addition, caspase-3 was measured in 5 independent PRELI overexpression experiments without the IL-4 treatment (data not shown). In these experiments PRELI significantly increased the proportion of cells with active caspase-3 (*P < .05). In graphs of annexin V, bars represent the average fold changes plus or minus SEM of annexin V intensity between the untreated control sample and the other samples. The values of the untreated control samples were set as 1. Δψm was measured from living cell populations according to FSC/SSC plots (overexpression experiments) or total cell population (siRNA experiments). The percentage of cells with reduced Δψm was determined as described in Figure 2A. Statistical significances were calculated using the 2-tailed paired t test. OE indicates overexpression.

PRELI induces the mitochondrial apoptosis pathway in Th cells and is partly inhibited by IL-4. (A) Overexpression of PRELI induces mitochondria-mediated apoptosis and this is partly counteracted by IL-4. CD4+ cells nucleofected with pIRES-H2Kk or PRELI overexpression vector were sorted and activated as in Figure 2A, cultured with or without IL-4 for 24 hours, and stained and analyzed by flow cytometry. (B) Knockdown of PRELI and IL-4 treatment has additive effects on the mitochondrial apoptosis pathway. CD4+ cells nucleofected with scramble or PRELI-siRNAs were cultured, stained, and analyzed as in panel A. (A,B) Cell viability = PI-negative cells. Bars represent the mean values plus or minus SEM of 4 to 5 independent experiments, except that caspase-3 was measured in 2 independent overexpression experiments that included IL-4 treatment. In addition, caspase-3 was measured in 5 independent PRELI overexpression experiments without the IL-4 treatment (data not shown). In these experiments PRELI significantly increased the proportion of cells with active caspase-3 (*P < .05). In graphs of annexin V, bars represent the average fold changes plus or minus SEM of annexin V intensity between the untreated control sample and the other samples. The values of the untreated control samples were set as 1. Δψm was measured from living cell populations according to FSC/SSC plots (overexpression experiments) or total cell population (siRNA experiments). The percentage of cells with reduced Δψm was determined as described in Figure 2A. Statistical significances were calculated using the 2-tailed paired t test. OE indicates overexpression.

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