![Figure 2. The ARF/p53 and Atm/53 axes cooperate as proapoptotic growth restraints in Myc-driven tumorigenesis. (A) Genomic p53 status by allele-specific PCR in primary Eμ-myc lymphomas that formed in an Atm+/+; p53+/− or an Atm−/−; p53+/− background (normal tissue [N] compared with the matched tumor tissue [T] for every given animal); MEFs of the indicated p53 genotypes as controls. (B) Frequency of homozygous INK4a/ARF deletions that cancel ARF expression in control (ctrl) and Atm−/− lymphomas detected by multiplex PCR of exon 1β and 2 (control, 8 of 19 cases; Atm−/−, 5 of 14 cases tested). (C) Lymphoma incidence in lethally irradiated recipient mice of retrovirally bcl2-infected Eμ-myc transgenic Atm+/+ and (control [ctrl]; n = 7; black) Atm−/− (n = 6; red) hematopoietic stem cells. Note the very early onset due to the Bcl2 moiety (see Schmitt et al45 for comparison with onset data upon mock infection). Immunoblot analysis testing for Bcl2 expression in lymphomas generated from transplanted bcl2- or mock-infected Eμ-myc hematopoietic stem cells (representative samples shown). (D) Immunoblot analysis of DDR components in ARF−/− Eμ-myc lymphoma cell lysates exposed to adriamycin (ADR; 0.2 μg/mL for 5 hours) in vitro or left untreated.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/110/8/10.1182_blood-2007-02-075614/4/zh80190707470002.jpeg?Expires=1722587543&Signature=Yuk~JqdkZfV2w6KhyG956HEMhn6~LyNHuR5nU4jKK3KS9dPFh5ORPHHgA0DHiwXNa9-X9-403zBuCYIr0iSG31Hpmb0eIhPVNn~AmrlVyscqHm5~pUgUjOYo3d--hnSQAUCgqCn-QsCvqZ57w14mW1heQcbSu3EWogPth0h-CsKwChkGIzmccpEAlLDtz~Gm1fu~I23Fd0X2U75IRy5QfOJ4Dhfnw2UxcMACofIvTQnMLnjJkdiMZEQVOb~VXAUErCq8ETBoEIMd-bb55tBVCiNRe14B2FVhWzhIGRzLrbmDpI1lMjgEtwA5ODTi7lpDdfmw7ens4IS57U5E3bVBDg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
The ARF/p53 and Atm/53 axes cooperate as proapoptotic growth restraints in Myc-driven tumorigenesis. (A) Genomic p53 status by allele-specific PCR in primary Eμ-myc lymphomas that formed in an Atm+/+; p53+/− or an Atm−/−; p53+/− background (normal tissue [N] compared with the matched tumor tissue [T] for every given animal); MEFs of the indicated p53 genotypes as controls. (B) Frequency of homozygous INK4a/ARF deletions that cancel ARF expression in control (ctrl) and Atm−/− lymphomas detected by multiplex PCR of exon 1β and 2 (control, 8 of 19 cases; Atm−/−, 5 of 14 cases tested). (C) Lymphoma incidence in lethally irradiated recipient mice of retrovirally bcl2-infected Eμ-myc transgenic Atm+/+ and (control [ctrl]; n = 7; black) Atm−/− (n = 6; red) hematopoietic stem cells. Note the very early onset due to the Bcl2 moiety (see Schmitt et al45 for comparison with onset data upon mock infection). Immunoblot analysis testing for Bcl2 expression in lymphomas generated from transplanted bcl2- or mock-infected Eμ-myc hematopoietic stem cells (representative samples shown). (D) Immunoblot analysis of DDR components in ARF−/−Eμ-myc lymphoma cell lysates exposed to adriamycin (ADR; 0.2 μg/mL for 5 hours) in vitro or left untreated.
