Figure 1.
Figure 1. FOXO3A is highly expressed in cHL. (A) Gene expression profiling (GEP) data were mined and analyzed with help of the GENEVESTIGATOR software. The following data sets were used for analysis: CB and CC (GSE15271, GSE38697, GSE56314); M (GSE1266, GSE45113, GSE17186, GSE64028); PC (GSE12366, GSE45537, GSE56464, GSE5900), cHL (GSE14879). FOXO1: probe set 202724_s_at; FOXO3A: probe set 204131_s_at; FOXO4: probe set 205451_at; FOXO6: probe set 239657_x_at. CB (n = 15); centrocytes (CC; n = 15); memory B cells (M; n = 38); PC (n = 13); microdissected HRS cells of cHL (cHL; n = 4). Data are represented as mean fluorescence ± standard deviation (SD). Means of FOXO3A levels in GC B cells and cHL were compared using an online software (https://www.medcalc.org/calc/comparison_of_means.php; 10.23.2017). ****P < .0001. (B-H) FOXO1 and FOXO3A mRNA and protein expression in CD19+ B cells and B- or T-cell–derived cHL cell lines. FOXO1 (B) and FOXO3A (C) mRNA levels were measured by RT-qPCR and expressed as ratio to RPL13A. Data are shown as mean ± SD of 3 independent experiments. FOXO1 and FOXO3A expressions of all cHL cell lines except for FOXO3A in L540 significantly differed from CD19+ B cells with P < .01. Statistical significances were analyzed by 2-tailed t tests. (D) FOXO3A/FOXO1 mRNA ratio in B cells and cHL. Data were extracted from experiments shown in panels B and C. (E) FOXO1 and FOXO3A protein expression was measured by immunoblot. The most representative of 3 independent analyses is shown. TUBB served as loading control. (F-G) The immunoblots were quantified using ImageJ 64 software. FOXO1 (F) and FOXO3A (G) values were normalized to TUBB. Data are shown as mean ± SD of all 3 experiments and values for KM-H2 were set to 1. (H) The apparent FOXO3A-to-FOXO1 protein ratio for each sample was calculated as: (FOXO3A/TUBB)/(FOXO1/TUBB). The apparent ratio does not represent the molar FOXO3A-to-FOXO1 ratio but permits to compare relative expression of FOXO proteins in different samples.

FOXO3A is highly expressed in cHL. (A) Gene expression profiling (GEP) data were mined and analyzed with help of the GENEVESTIGATOR software. The following data sets were used for analysis: CB and CC (GSE15271, GSE38697, GSE56314); M (GSE1266, GSE45113, GSE17186, GSE64028); PC (GSE12366, GSE45537, GSE56464, GSE5900), cHL (GSE14879). FOXO1: probe set 202724_s_at; FOXO3A: probe set 204131_s_at; FOXO4: probe set 205451_at; FOXO6: probe set 239657_x_at. CB (n = 15); centrocytes (CC; n = 15); memory B cells (M; n = 38); PC (n = 13); microdissected HRS cells of cHL (cHL; n = 4). Data are represented as mean fluorescence ± standard deviation (SD). Means of FOXO3A levels in GC B cells and cHL were compared using an online software (https://www.medcalc.org/calc/comparison_of_means.php; 10.23.2017). ****P < .0001. (B-H) FOXO1 and FOXO3A mRNA and protein expression in CD19+ B cells and B- or T-cell–derived cHL cell lines. FOXO1 (B) and FOXO3A (C) mRNA levels were measured by RT-qPCR and expressed as ratio to RPL13A. Data are shown as mean ± SD of 3 independent experiments. FOXO1 and FOXO3A expressions of all cHL cell lines except for FOXO3A in L540 significantly differed from CD19+ B cells with P < .01. Statistical significances were analyzed by 2-tailed t tests. (D) FOXO3A/FOXO1 mRNA ratio in B cells and cHL. Data were extracted from experiments shown in panels B and C. (E) FOXO1 and FOXO3A protein expression was measured by immunoblot. The most representative of 3 independent analyses is shown. TUBB served as loading control. (F-G) The immunoblots were quantified using ImageJ 64 software. FOXO1 (F) and FOXO3A (G) values were normalized to TUBB. Data are shown as mean ± SD of all 3 experiments and values for KM-H2 were set to 1. (H) The apparent FOXO3A-to-FOXO1 protein ratio for each sample was calculated as: (FOXO3A/TUBB)/(FOXO1/TUBB). The apparent ratio does not represent the molar FOXO3A-to-FOXO1 ratio but permits to compare relative expression of FOXO proteins in different samples.

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