Figure 2.
Figure 2. Molecular analysis of tumor and blood. (A) Southern blot analysis with an enhanced green fluorescent protein (eGFP) probe to determine copy number of the proviral genome in DNA extracted from the left kidney, which was heavily infiltrated with tumor cells. DNA (10 μg) from the tumor and from copy number control DNA obtained from Jurkat cells containing known copies per cell of the GFP gene were digested with NheI, which cuts once in each proviral LTR, and then hybridized with an eGFP probe. The copy number was calculated as 0.9 copies by phosphoimager scanning and comparison of band intensity to the Jurkat DNA copy number controls. The second panel shows 10μg tumor DNA digested with EcoR1, which cuts once within the proviral genome and therefore generates a unique band for each integration site based on the relative position of the first EcoR1 site in flanking genomic DNA. (B) Scheme of MgirL22Y retroviral vector (which contains eGFP), the internal ribosomal entry site (IRES), and the mutant dihydrofolate reductase gene (L22Y). Shown is the binding site of the probe as well as cutting sites of NheI and EcoRI. (C) BCL2-A1 is a small gene with one intron and 2 exons. The insertion occurred in the intron in the gene opposing DNA strand in chromosome band 15q25.1.

Molecular analysis of tumor and blood. (A) Southern blot analysis with an enhanced green fluorescent protein (eGFP) probe to determine copy number of the proviral genome in DNA extracted from the left kidney, which was heavily infiltrated with tumor cells. DNA (10 μg) from the tumor and from copy number control DNA obtained from Jurkat cells containing known copies per cell of the GFP gene were digested with NheI, which cuts once in each proviral LTR, and then hybridized with an eGFP probe. The copy number was calculated as 0.9 copies by phosphoimager scanning and comparison of band intensity to the Jurkat DNA copy number controls. The second panel shows 10μg tumor DNA digested with EcoR1, which cuts once within the proviral genome and therefore generates a unique band for each integration site based on the relative position of the first EcoR1 site in flanking genomic DNA. (B) Scheme of MgirL22Y retroviral vector (which contains eGFP), the internal ribosomal entry site (IRES), and the mutant dihydrofolate reductase gene (L22Y). Shown is the binding site of the probe as well as cutting sites of NheI and EcoRI. (C) BCL2-A1 is a small gene with one intron and 2 exons. The insertion occurred in the intron in the gene opposing DNA strand in chromosome band 15q25.1.

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