Figure 2.
Figure 2. IPCR analysis to detect etoposide-induced rearrangements initiating within the MLL bcr. (A) Schematic representation of the MLL gene locus on chromosome band 11q23. The 8.3-kb MLL bcr, flanked by BamHI sites, includes exons 5 to 11 and intervening introns. XbaI sites are 2.6 kb apart within the MLL bcr. Genomic DNA was digested with XbaI and circularized. Nested PCR reactions were carried out with F1-R1 primer pair, followed by F2-R2 primer pair. BH (BamH1); X (XbaI); F1, F2, R1, R2 are primers used for PCR (see “Materials and methods”). (B) Representative IPCR products. Lanes 1-7: untreated controls that give the expected 1.8-kb germ-line product. Lanes 8-18: etoposide-treated samples that all give alternative products representing possible rearrangements of MLL. Pretreatment of samples shown in lanes 8 to 18 with PvuII eliminated some or all detectable germ-line product to facilitate isolation of individual alternative sized products. Lanes 8-12: multiple independent CD34+ cell samples (long recovery) with all germ-line products eliminated by PvuII in lanes 8-9; lane 13: TF-1 (short recovery); lane 14: WS1 (short recovery); lanes 15-16: M059K (short recovery); lane 17: M059J (short recovery); and lane 18: cord blood mononuclear cells (short recovery). Parallel experiments in multiple hematologic and other adherent cell lines gave similar IPCR results (B), but individual repair clones have not been fully characterized.

IPCR analysis to detect etoposide-induced rearrangements initiating within the MLL bcr. (A) Schematic representation of the MLL gene locus on chromosome band 11q23. The 8.3-kb MLL bcr, flanked by BamHI sites, includes exons 5 to 11 and intervening introns. XbaI sites are 2.6 kb apart within the MLL bcr. Genomic DNA was digested with XbaI and circularized. Nested PCR reactions were carried out with F1-R1 primer pair, followed by F2-R2 primer pair. BH (BamH1); X (XbaI); F1, F2, R1, R2 are primers used for PCR (see “Materials and methods”). (B) Representative IPCR products. Lanes 1-7: untreated controls that give the expected 1.8-kb germ-line product. Lanes 8-18: etoposide-treated samples that all give alternative products representing possible rearrangements of MLL. Pretreatment of samples shown in lanes 8 to 18 with PvuII eliminated some or all detectable germ-line product to facilitate isolation of individual alternative sized products. Lanes 8-12: multiple independent CD34+ cell samples (long recovery) with all germ-line products eliminated by PvuII in lanes 8-9; lane 13: TF-1 (short recovery); lane 14: WS1 (short recovery); lanes 15-16: M059K (short recovery); lane 17: M059J (short recovery); and lane 18: cord blood mononuclear cells (short recovery). Parallel experiments in multiple hematologic and other adherent cell lines gave similar IPCR results (B), but individual repair clones have not been fully characterized.

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