Chromosome translocations and covert leukemic clones are generated during normal fetal development

Mori, Hiroshi; Colman, Sue; Xiao, Zhijian; Ford, Anthony M.; Healy, Lyn; Donaldson, Craig; Hows, Jill; Navarrete, Cristina; Greaves, Mel

doi:10.1073/pnas.112218799

Cited by 551 publications

(447 citation statements)

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“…For species C adenovirus to contribute to the earliest steps in development of childhood leukaemia, this virus must infect the fetus at least as frequently as the incidence of neonatal preleukaemic clones in the population, estimated at 1 -5% (Mori et al, 2002). In addition to being a likely fetal pathogen (Towbin et al, 1994;Van den Veyver et al, 1998;Oyer et al, 2000;Baschat et al, 2003;Reddy et al, 2005), adenovirus DNA is also detected in the amniotic fluid from apparently normal pregnancies.…”

Section: Discussionmentioning

confidence: 99%

Adenovirus DNA is detected at increased frequency in Guthrie cards from children who develop acute lymphoblastic leukaemia

et al. 2007

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Section: Discussionmentioning

confidence: 99%

Adenovirus DNA is detected at increased frequency in Guthrie cards from children who develop acute lymphoblastic leukaemia

et al. 2007

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“…The ETV6-CBFA2 fusion product was detected in neonatal blood spots obtained from children who have ETV6-CBFA2 ALL (Wiemels et al, 1999), suggesting that the events leading to the translocation occur in utero. The fusion product was also detected in anonymized cord blood samples at a frequency of a hundred times higher than that expected from the incidence of the corresponding leukaemia (Mori et al, 2002). This, the long postnatal latency period prior to the development of leukaemia, and murine models (Andreasson et al, 2001), suggest that subsequent to the creation of the fusion gene, secondary changes are required for leukaemogenesis.…”

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confidence: 84%

Expression profile of wild‐type ETV6 in childhood acute leukaemia

et al. 2003

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Summary. Comparative expression analysis of wild-type ETV6 in the disease state showed an absence of expression in ETV6-CBFA2 acute lymphoblastic leukaemia (ALL) when compared with non-ETV6-CBFA2 ALL and acute myeloid leukaemia. Fluorescent in-situ hybridization and loss of heterozygosity studies showed that 73% of the ETV 6-CBFA2 samples had a fully or partially deleted second ETV6 allele, explaining the lack of wild-type expression in these patients. Although the second ETV6 allele was identified in the remaining patients, no ETV6 expression was detected. These observations support the hypothesis that loss of ETV6 expression is a critical secondary event for leukaemogenesis in ETV6-CBFA2 ALL.Keywords: ETV6, ETV6-CBFA2, gene expression, acute leukaemia.The t(12;21)(p13;q22) translocation seen in childhood acute lymphoblastic leukaemia (ALL) results in the chimaeric fusion of ETV6 to CBFA2. The ETV6-CBFA2 fusion product was detected in neonatal blood spots obtained from children who have ETV6-CBFA2 ALL (Wiemels et al, 1999), suggesting that the events leading to the translocation occur in utero. The fusion product was also detected in anonymized cord blood samples at a frequency of a hundred times higher than that expected from the incidence of the corresponding leukaemia (Mori et al, 2002). This, the long postnatal latency period prior to the development of leukaemia, and murine models (Andreasson et al, 2001), suggest that subsequent to the creation of the fusion gene, secondary changes are required for leukaemogenesis. Fluorescent in-situ hybridization (FISH) studies have identified a number of secondary structural changes in cells with a t(12;21). These include a complete or partial deletion of the second ETV6 allele, an additional chromosome 21 and, more rarely, multiple copies of CBFA2 or the ETV6-CBFA2 fusion product (Ma et al, 2001). Of these, the loss of the ETV6 allele appears to be the best candidate as a second hit. There is evidence to show this is a postnatal event (Ford et al, 2001), and careful examination shows a loss of heterozygosity (LOH) of the ETV6 allele in 77% of those with a t(12;21) (Cavé et al, 1997), making this clearly the most frequent observed secondary change.Our study provided further evidence for this hypothesis by demonstrating that ETV6-CBFA2 leukaemic cells did not express wild-type ETV6, irrespective of whether a second ETV6 allele was present or absent as demonstrated by FISH and LOH. PATIENTS AND METHODSBone marrow was obtained with consent at disease (presentation/relapse with > 95% blast cells) and at remission (< 5% blast cells) from 38 patients. They were grouped as follows: group A (n ¼ 16), ETV6-CBFA2-positive ALL as identified by FISH and real-time reverse transcription polymerase chain reaction (RQ-RTPCR); group B (n ¼ 13), ETV6-CBFA2-negative ALL; and group C (n ¼ 9), acute myeloid leukaemia (AML). In some children, samples were available from the original diagnostic bone marrow as well as from subsequent relapse(s). For the purposes of this study, these have been...

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“…However, characterization of sorted cells from leukemic bone marrow of childhood high-risk ALL/ t(4;11) suggested an origin in a primitive lymphoidrestricted progenitor cell (Hotfilder et al, 2005). Moreover, studies in monozygotic twins with leukaemia, carrying an identical MLL-AF4 chromosomal translocation, but different immunoglobulin rearrangements strongly supported the model that the primary MLL-AF4 target cell was a progenitor cell at a differentiation stage before efficient RAG expression (Mori et al, 2002;Greaves et al, 2003). This issue could be addressed using the Mll-AF4 invertor model and an inducible Cre driven by a promoter of a gene, such as Lmo2, expressed in bone marrow progenitor cells.…”

Section: Cellular Origin Of Mll-af4 Leukaemiasmentioning

confidence: 99%

A conditional model of MLL-AF4 B-cell tumourigenesis using invertor technology

et al. 2006

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MLL-AF4 fusion is the most common consequence of chromosomal translocations in infant leukaemia and is associated with a poor prognosis. MLL-AF4 is thought to be required in haematopoietic stem cells to elicit leukaemia and may be involved in tumour phenotype specification as it is only found in B-cell tumours in humans. We have employed the invertor conditional technology to create a model of MLL-AF4, in which a floxed AF4 cDNA was knocked into Mll in the opposite orientation for transcription. Cell-specific Cre expression was used to generate Mll-AF4 expression. The mice develop exclusively B-cell lineage neoplasias, whether the Cre gene was controlled by B-or T-cell promoters, but of a more mature phenotype than normally observed in childhood leukaemia. These findings show that the MLL-AF4 fusion protein does not have a mandatory role in multi-potent haematopoietic stem cells to cause cancer and indicates that MLL-AF4 has an instructive function in the phenotype of the tumour.

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Chromosome translocations and covert leukemic clones are generated during normal fetal development

Cited by 551 publications

References 35 publications

Adenovirus DNA is detected at increased frequency in Guthrie cards from children who develop acute lymphoblastic leukaemia

Adenovirus DNA is detected at increased frequency in Guthrie cards from children who develop acute lymphoblastic leukaemia

Expression profile of wild‐type ETV6 in childhood acute leukaemia

A conditional model of MLL-AF4 B-cell tumourigenesis using invertor technology

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