Fig. 1.
Fig. 1. Effects of ATRA and IFNs on the expression of Stat, p48, Jak 1, Jak 2, and Tyk 2 proteins in NB4 and HeLa cells. NB4 (4 ×105/mL) or HeLa (a confluent 25 cm2 flask) cells were treated for 4 days with medium alone (Medium) and medium containing ATRA (10−6 mol/L), IFNα (1,000 U/mL), and IFNγ (1,000 U/mL) as indicated. Cells were harvested, lysed, and subjected to Western blot analysis, using antibodies specific for Stat 1α, Stat 2, Stat 3, and Stat 4 (A), p48 (B), Jak1, Jak 2, and Tyk 2 (C). For Stat 3 and Jak 1, 100 μg of protein/lane were used, whereas for all the other samples, 10 mg of protein/lane were used. In (B), the apparent molecular weight of standard proteins (carbonic anhydrase [28 kD], ovalbumin [43 kD], bovine serum albumin [69 kD], and phosphorylase B [105 kD]) is indicated on the right. The apparent molecular weight of Stat proteins, Jak 1, Jak 2, and Tyk 2 is indicated on the right of (A) and (C). Western blots representative of at least two independent experiments are shown.

Effects of ATRA and IFNs on the expression of Stat, p48, Jak 1, Jak 2, and Tyk 2 proteins in NB4 and HeLa cells. NB4 (4 ×105/mL) or HeLa (a confluent 25 cm2 flask) cells were treated for 4 days with medium alone (Medium) and medium containing ATRA (10−6 mol/L), IFNα (1,000 U/mL), and IFNγ (1,000 U/mL) as indicated. Cells were harvested, lysed, and subjected to Western blot analysis, using antibodies specific for Stat 1α, Stat 2, Stat 3, and Stat 4 (A), p48 (B), Jak1, Jak 2, and Tyk 2 (C). For Stat 3 and Jak 1, 100 μg of protein/lane were used, whereas for all the other samples, 10 mg of protein/lane were used. In (B), the apparent molecular weight of standard proteins (carbonic anhydrase [28 kD], ovalbumin [43 kD], bovine serum albumin [69 kD], and phosphorylase B [105 kD]) is indicated on the right. The apparent molecular weight of Stat proteins, Jak 1, Jak 2, and Tyk 2 is indicated on the right of (A) and (C). Western blots representative of at least two independent experiments are shown.

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