Double minute chromosomes can be produced from precursors derived from a chromosomal deletion.

“…In addition, in vitro studies imply that many of the structural chromosomal abnormalities occurring in tumors and tumorigenic cell lines (Bishop, 1987;Tlsty et al, 1989) may result from molecular mechanisms common to those mediating extrachromosomal gene amplification. For example, recent studies have provided firm evidence that some extrachromosomal elements have the potential to integrate into chromosomes, resulting in either HSRs, ECRs (Carroll et al, 1988;Ruiz and Wahl, 1990;Von Hoff et al, 1990;Windle et al, 1991), or other chromosome abnormalities such as ring chromosomes (Windle et al, 1991). These studies support earlier observations of gene amplification in hamster cell lines in which Biedler (1982) observed that the extrachromosomal circular DMs rapidly integrated into chromosomes, resulting in HSR structures (Biedler, 1982).…”

Section: Introductionmentioning

confidence: 52%

“…Amplification of a region of DNA via an extrachromosomal element often results in a deletion at the corresponding chromosomal locus (Carroll et al, 1988;Hunt et al, 1990;Heard et al, 1991). If a deletion is present, its respective size could provide information as to the size of the initial amplicon.…”

Section: Discussionmentioning

confidence: 99%

“…Several studies of cultured cell lines have provided a molecular chronology of events in which submicroscopic circular DNAs precede the appearance of cytogenetically detectable DM structures (Carroll et al, 1987(Carroll et al, , 1988. In addition, pulsed-field gel electrophoresis (PFGE) data from neuroblastoma biopsies imply that the multimerization of MYCN circles in vivo can generate DM structures .…”

Section: Introductionmentioning

confidence: 99%

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Double minute chromosomes carrying the human multidrug resistance 1 and 2 genes are generated from the dimerization of submicroscopic circular DNAs in colchicine-selected KB carcinoma cells.

Schoenlein

Shen

Barrett

et al. 1992

MBoC

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This study characterizes amplified structures carrying the human multidrug resistance (MDR) genes in colchicine-selected multidrug resistant KB cell lines and strongly supports a model of gene amplification in which small circular extrachromosomal DNA elements generated from contiguous chromosomal DNA regions multimerize to form cytologically detectable double minute chromosomes (DMs). The human MDR1 gene encodes the 170-kDa Pglycoprotein, which is a plasma membrane pump for many structurally unrelated chemotherapeutic drugs. MDR1 and its homolog, MDR2, undergo amplification when KB cells are subjected to stepwise selection in increasing concentrations of colchicine. The structure of the amplification unit at each step of drug selection was characterized using both highvoltage gel electrophoresis and pulsed-field gel electrophoresis (PFGE) techniques. An 890-kb submicroscopic extrachromosomal circular DNA element carrying the MDR1 and MDR2 genes was detected in cell line KB-ChR-8-5-1 1, the earliest step in drug selection in which conventional Southern/hybridization analyses detected MDR gene amplification. When KB-ChR-8-5-11 was subjected to stepwise increases in colchicine, this circular DNA element dimerized as detected by PFGE with and without digestion with Not 1, which linearizes the 890-kb amplicon. This dimerization process, which also occurred at the next step of colchicine selection, resulted in the formation of cytologically detectable DMs revealed by analysis of Giemsa-stained metaphase spreads.

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“…These studies led to the identification of at least two different initial gene amplification mechanisms (Coquelle et al, 1997;Carroll et al, 1988;Ma et al, 1993;Ruiz and Wahl, 1988;Smith et al, 1992;Toledo et al, 1992Toledo et al, , 1993Trask and Hamlin, 1989;Windle et al, 1991). The breakage-fusion-bridge (BFB) cycle mechanism, first described by McClintock (1942), accumulates copies organized as large inverted repeats on a chromosome arm where one normal gene copy maps in non-amplified cells (Coquelle et al, 1997;Ma et al, 1993;Toledo et al, 1992Toledo et al, , 1993.…”

Section: Introductionmentioning

confidence: 99%

Induction of multiple double-strand breaks within an hsr by meganucleaseI-SceI expression or fragile site activation leads to formation of double minutes and other chromosomal rearrangements

et al. 2002

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Gene amplification is frequently associated with tumor progression, hence, understanding the underlying mechanisms is important. The study of in vitro model systems indicated that different initial mechanisms accumulate amplified copies within the chromosomes (hsr) or on extra-chromosomal elements (dmin). It has long been suggested that formation of dmin could also occur following hsr breakdown. In order to check this hypothesis, we developed an approach based on the properties of the I-SceI meganuclease, which induces targeted DNA double-strand breaks. A clone containing an I-SceI site, integrated by chance close to an endogenous dhfr gene locus, was used to select for methotrexate resistant mutants. We recovered clones in which the I-SceI site was passively co-amplified with the dhfr gene within the same hsr. We show that I-SceIinduced hsr breakdown leads to the formation of dmin and creates different types of chromosomal rearrangements, including inversions. This demonstrates, for the first time, a direct relationship between double-strand breaks and inversions. Finally, we show that activation of fragile sites by aphidicolin or hypoxia in hsr-containing cells also generates dmin and a variety of chromosomal rearrangements. This may constitute a valuable model to study the consequences of breaks induced in hsr of cancer cells in vivo.

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Double minute chromosomes can be produced from precursors derived from a chromosomal deletion.

Cited by 216 publications

References 49 publications

Fusion of NUP214 to ABL1 on amplified episomes in T-cell acute lymphoblastic leukemia

Fusion of NUP214 to ABL1 on amplified episomes in T-cell acute lymphoblastic leukemia

Double minute chromosomes carrying the human multidrug resistance 1 and 2 genes are generated from the dimerization of submicroscopic circular DNAs in colchicine-selected KB carcinoma cells.

Induction of multiple double-strand breaks within an hsr by meganucleaseI-SceI expression or fragile site activation leads to formation of double minutes and other chromosomal rearrangements

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