Figure 1
Figure 1. p19INK4D expression in erythroid and megakaryocyte human cells. (A) The absolute expression level of p19INK4D per 100 ng total RNA was measured relatively to different dilutions of plasmids (corresponding to 102 to 106 copies) harboring a p19INK4D cDNA. The graph represents the expression level of p19INK4D in immature (CD36+GPA−) and mature (CD36+GPA+) erythroid cells and in mature (CD41+CD42+) MKs. The error bars represent the standard deviation of the mean of 3 experiments each performed in triplicate wells. (B-E) CD34+ cells were cultured with TPO for 9 days. Then, CD41- and CD42-positive cells stained with Hoechst were sorted on their ploidy level (from 2N to 16N). (B) mRNA levels of p15INK4B, p16INK4A, p18INK4C, and p19INK4D and their variants were quantified by real-time RT-PCR. Their relative expression was calculated in comparison with HPRT mRNA. (C) mRNA levels of p18INK4Cv2 and p19INK4D were quantified by RT-PCR in each ploidy class (from 2N to 16N) and normalized to their expression in diploid (2N) cell fraction. (D) The protein level of p19INK4D in different ploidy fractions was measured relatively to HDAC-1, a protein that we found stable during ploidization. The graph represents the ratio between p19INK4D and HDAC-1 levels for each ploidy class. The data illustrate 1 of 2 representative experiments that produced similar results. (E) To investigate the expression level of p19INK4D during differentiation, total cell population was harvested on day 3 (D3), day 6 (D6), and day 9 (D9) and submitted to Western blot analysis. (F) The expression level of p19INK4D mRNA was investigated by QRT-PCR in diploid (2N) cells sorted at day 6 in culture in 3 MK populations corresponding to very immature (CD34+CD41+CD42−), immature (CD34+CD41+CD42+), to more mature (CD34−CD41+CD42+) cells. The error bars represent the standard deviation of the mean of 3 repeated experiments each performed in triplicate wells.

p19INK4D expression in erythroid and megakaryocyte human cells. (A) The absolute expression level of p19INK4D per 100 ng total RNA was measured relatively to different dilutions of plasmids (corresponding to 102 to 106 copies) harboring a p19INK4D cDNA. The graph represents the expression level of p19INK4D in immature (CD36+GPA) and mature (CD36+GPA+) erythroid cells and in mature (CD41+CD42+) MKs. The error bars represent the standard deviation of the mean of 3 experiments each performed in triplicate wells. (B-E) CD34+ cells were cultured with TPO for 9 days. Then, CD41- and CD42-positive cells stained with Hoechst were sorted on their ploidy level (from 2N to 16N). (B) mRNA levels of p15INK4B, p16INK4A, p18INK4C, and p19INK4D and their variants were quantified by real-time RT-PCR. Their relative expression was calculated in comparison with HPRT mRNA. (C) mRNA levels of p18INK4Cv2 and p19INK4D were quantified by RT-PCR in each ploidy class (from 2N to 16N) and normalized to their expression in diploid (2N) cell fraction. (D) The protein level of p19INK4D in different ploidy fractions was measured relatively to HDAC-1, a protein that we found stable during ploidization. The graph represents the ratio between p19INK4D and HDAC-1 levels for each ploidy class. The data illustrate 1 of 2 representative experiments that produced similar results. (E) To investigate the expression level of p19INK4D during differentiation, total cell population was harvested on day 3 (D3), day 6 (D6), and day 9 (D9) and submitted to Western blot analysis. (F) The expression level of p19INK4D mRNA was investigated by QRT-PCR in diploid (2N) cells sorted at day 6 in culture in 3 MK populations corresponding to very immature (CD34+CD41+CD42), immature (CD34+CD41+CD42+), to more mature (CD34CD41+CD42+) cells. The error bars represent the standard deviation of the mean of 3 repeated experiments each performed in triplicate wells.

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