![Figure 1. Overexpression of CDK6. (A) Quantitative real-time PCR was performed using the LightCycler system with FastStart DNA Master SYBR Green I kit according to the manufacturer's instructions (Roche Diagnostics, Mannheim, Germany). Primers from the CDK6 gene are as follows: forward (5′-AGAAGAAGACTGGCCTAGAG) and reverse (5′-TGGAAGTATGGGTGAGACAGG). Primers from the β-2-microglobulin (β2-MG) gene used to evaluate correcting target molecule amounts are as follows: forward (5′-CCAGCAGAGAATGGAAAGTC) and reverse (5′-GATGCTGCTTACATGTCTCG). Amplification of specific transcripts was confirmed by a melting curve analysis. For PCR calibration, a serial 10-fold dilution series for each gene (ranging from 106 to 10 copies) was amplified and the assay was found to be linear over at least 5 orders of magnitude (CDK6 slope, –3.47; β2-MG slope, –3.43). The absolute copy amount of each sample was obtained by the mean of the following ratio: ([copy number of the CDK6 gene]/[copy number of β2-MG]) × 100. (B) Total cellular proteins were analyzed by Western blotting using anti-CDK6 antibody (Santa Cruz Biotechnology, Santa Cruz, CA). The same blot was probed for actin to control for equal protein loading. In all samples, tumor cells represented more than 80% of the nucleated cells. RNA and protein were extracted from bone marrow or blood samples from patients with the CDK6 gene rearrangement (FIO, DUP, LAN), from patients with B-CLL without the CDK6 gene rearrangement (B-CLL1 to B-CLL4), and from normal mononuclear peripheral blood cells (C1 to C5).](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/102/4/10.1182_blood-2003-04-1220/6/h81634897001.jpeg?Expires=1726822502&Signature=PRpUZlsccnpZ46HdybqcbQ-cZ8ddymNRSOtnAOZKE07BqkBkeq3zC0YOe4KdNVkYKNwazmTADvKNckMdd~9SU-WwCPUmTAAp2i~48mHdf2vFJg80PcvOV0gJoqHXG5gpmE3HMpnbRP9sl3n63UaMBhVJ~iZdofYuTnOz5OB5w66m194opu9tH4VJgTfKOBRIrzEm08G7cp1Y~8jnSyTKHKklTee223WTdGhH8XksGaejaWVVOCYGabL7cHCY~RCTWDqopPvdkgIyBKxrozFQH0xXddM~RA4jcPGX9y1eSIcYPjriLdnu8VgvVIk-~nWahxqkjk8wqbG6KmsrA5FqYQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Overexpression of CDK6. (A) Quantitative real-time PCR was performed using the LightCycler system with FastStart DNA Master SYBR Green I kit according to the manufacturer's instructions (Roche Diagnostics, Mannheim, Germany). Primers from the CDK6 gene are as follows: forward (5′-AGAAGAAGACTGGCCTAGAG) and reverse (5′-TGGAAGTATGGGTGAGACAGG). Primers from the β-2-microglobulin (β2-MG) gene used to evaluate correcting target molecule amounts are as follows: forward (5′-CCAGCAGAGAATGGAAAGTC) and reverse (5′-GATGCTGCTTACATGTCTCG). Amplification of specific transcripts was confirmed by a melting curve analysis. For PCR calibration, a serial 10-fold dilution series for each gene (ranging from 106 to 10 copies) was amplified and the assay was found to be linear over at least 5 orders of magnitude (CDK6 slope, –3.47; β2-MG slope, –3.43). The absolute copy amount of each sample was obtained by the mean of the following ratio: ([copy number of the CDK6 gene]/[copy number of β2-MG]) × 100. (B) Total cellular proteins were analyzed by Western blotting using anti-CDK6 antibody (Santa Cruz Biotechnology, Santa Cruz, CA). The same blot was probed for actin to control for equal protein loading. In all samples, tumor cells represented more than 80% of the nucleated cells. RNA and protein were extracted from bone marrow or blood samples from patients with the CDK6 gene rearrangement (FIO, DUP, LAN), from patients with B-CLL without the CDK6 gene rearrangement (B-CLL1 to B-CLL4), and from normal mononuclear peripheral blood cells (C1 to C5).
