![Figure 4. CDK6 protein levels are down-regulated in c-JunΔ/Δ p185BCR-ABL–transformed cell lines. (A) Immunoblot analysis for CDK6, CDK4, CDK2, CYCLIN D2, CYCLIN D3, p16INK4a, p15INK4b, p21, and p27 protein expression in c-Junfl/fl- and c-JunΔ/Δ p185BCR-ABL–transformed cells. β-ACTIN served as the loading control. (B) Immunoblot analysis for c-JUN and CDK6 protein expression in c-Junfl/fl and c-JunΔ/Δ (top panel) and c-Junwt/wt and c-JunAA/AA (bottom panel) p185BCR-ABL–transformed cells. β-ACTIN served as the loading control. (C) c-JUN and CDK6 protein levels of c-JunΔ/Δ and c-Junfl/fl cell lines after 2, 4, 6, and 8 weeks of transformation. β-ACTIN served as the loading control. One representative set of data is depicted. (D) [3H]-thymidine incorporation of the same cell lines was measured (n = 3; 2-tailed t test: c-Junfl/fl vs c-JunΔ/Δ 6 weeks, P = .002; c-Junfl/fl vs c-JunΔ/Δ 8 weeks, P = .0016). (E) Cdk6 mRNA levels of c-JunΔ/Δ and c-Junfl/fl cells 2, 4, 6, and 8 weeks after p185BCR-ABL transformation were analyzed by quantitative PCR (n = 3; 2-tailed t test: c-Junfl/fl 2 weeks vs c-JunΔ/Δ 2 weeks, P = .0385; c-Junfl/fl 2 weeks vs c-Junfl/fl 8 weeks, P = .0293; c-JunΔ/Δ 2 weeks vs c-JunΔ/Δ 8 weeks, P = .0024). The fold change compared with c-JunΔ/Δ 2-week Cdk6 mRNA level is shown. Results were normalized by comparison with their Gapdh mRNA expression.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/117/15/10.1182_blood-2010-07-299644/4/zh89991168840004.jpeg?Expires=1724233622&Signature=AfZhv2YsdtFs8uEMaUJiZqnyrJk0wfp3Eh4QHyvXTrUiWwZ7gLpS9e2RmvYV~iVsYUCTl6t9hjzta~is5EduAq5vVJ3QFpNBuJlgfRTCaWIesLNyzVoG35q9odMy9dq4dwPEggkvqt7awjP34iPcNE84h-LKdM~WRKv4LUfedWIuYZ0-ube1WKPObKCU1O-fgEaEk5wiG-hPYhcDpDProSO86qZ4rfU0pqX3~tptndDSNrsObMS8F812c7hOecBCNk2~VqGQvARi5VM-qlSpM6sfD3wWrNAaeojEk~EYpyGcw~KpAnduEoT3GPwqolW8VfEjLsHnHAVzrVPKLtykhA__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
CDK6 protein levels are down-regulated in c-JunΔ/Δp185BCR-ABL–transformed cell lines. (A) Immunoblot analysis for CDK6, CDK4, CDK2, CYCLIN D2, CYCLIN D3, p16INK4a, p15INK4b, p21, and p27 protein expression in c-Junfl/fl- and c-JunΔ/Δp185BCR-ABL–transformed cells. β-ACTIN served as the loading control. (B) Immunoblot analysis for c-JUN and CDK6 protein expression in c-Junfl/fl and c-JunΔ/Δ (top panel) and c-Junwt/wt and c-JunAA/AA (bottom panel) p185BCR-ABL–transformed cells. β-ACTIN served as the loading control. (C) c-JUN and CDK6 protein levels of c-JunΔ/Δ and c-Junfl/fl cell lines after 2, 4, 6, and 8 weeks of transformation. β-ACTIN served as the loading control. One representative set of data is depicted. (D) [3H]-thymidine incorporation of the same cell lines was measured (n = 3; 2-tailed t test: c-Junfl/fl vs c-JunΔ/Δ 6 weeks, P = .002; c-Junfl/fl vs c-JunΔ/Δ 8 weeks, P = .0016). (E) Cdk6 mRNA levels of c-JunΔ/Δ and c-Junfl/fl cells 2, 4, 6, and 8 weeks after p185BCR-ABL transformation were analyzed by quantitative PCR (n = 3; 2-tailed t test: c-Junfl/fl 2 weeks vs c-JunΔ/Δ 2 weeks, P = .0385; c-Junfl/fl 2 weeks vs c-Junfl/fl 8 weeks, P = .0293; c-JunΔ/Δ 2 weeks vs c-JunΔ/Δ 8 weeks, P = .0024). The fold change compared with c-JunΔ/Δ 2-week Cdk6 mRNA level is shown. Results were normalized by comparison with their Gapdh mRNA expression.
