Detection and mapping of amplified DNA sequences in breast cancer by comparative genomic hybridization.

Kallioniemi, Anne; Kallioniemi, Olli; Piper, Jim; Tanner, Minna; Stokke, Trond; Chen, Ling; Smith, Helene S.; Pinkel, Dan; Gray, Joe W.; Waldman, Frederic M.

doi:10.1073/pnas.91.6.2156

Cited by 647 publications

(480 citation statements)

References 20 publications

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“…Thus, it would be of interest to know whether a simultaneous It remains to be determined whether there is an oncogene within the 17q23 breast cancer amplicon whose overexpression could drive tumorigenesis in transgenic mice. The 17q23 amplification occurs fairly frequently (B18%) in primary human breast cancers (Kallioniemi et al, 1994;Sinclair et al, 2003) and there are three potential oncogenes, RPS6KB1, TBX-2 and WIP1, which have been identified within this genomic locus (Sinclair et al, 2003). However, overexpression of either WIP1, Tbx2 or both in MMTVtransgenic mice is not sufficient for tumor formation (present study and data not shown).…”

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confidence: 48%

“…This site has been found to be a hot spot for gene amplifications in multiple types of human cancer. The initial observation of regional gain at chromosome 17q22-23 using a comparative genomic hybridization (CGH) technique detected amplification in B18% of primary breast tumors (Kallioniemi et al, 1994), giving its name to the locus as the 17q23 breast cancer amplicon. Three potential oncogenes, RPS6KB1, TBX-2 and WIP1 have been found within this genomic locus at chromosome 17q22-23 (Sinclair et al, 2003).…”

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confidence: 99%

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The role of the MKK6/p38 MAPK pathway in Wip1-dependent regulation of ErbB2-driven mammary gland tumorigenesis

et al. 2006

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There is increasing evidence for the role of wild-type p53 induced phosphatase 1 (Wip1) phosphatase in the regulation of tumorigenesis. To evaluate Wip1 as a breast cancer oncogene, we generated a mouse strain with targeted expression of Wip1 to the breast epithelium. We found that these mice are prone to cancer when intercrossed with transgenics expressing the ErbB2 oncogene but not conditional knockouts for Brca2. This tumor-prone phenotype of Wip1 is fully eliminated through attenuation of proliferation by activating the MKK6/p38 mitogenactivated protein kinases (MAPK) cascade in mice bearing a constitutively active form of MKK6. We propose that Wip1 phosphatase operates within the MKK6/p38 MAPK signaling pathway to promote ErbB2-driven mammary gland tumorigenesis.

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confidence: 48%

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confidence: 99%

The role of the MKK6/p38 MAPK pathway in Wip1-dependent regulation of ErbB2-driven mammary gland tumorigenesis

et al. 2006

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“…Inhibition of differentiation would be a prerequisite for the maintenance of proliferative capacity of immortalized cells; (iii) CROC1/UEV-1 maps to chromosome 20q13.2 (Sancho et al, 1998), a region which is moderately ampli®ed in many types of cancer (e.g. Kallioniemi et al, 1994;Muleris et al, 1994;Tanner et al, , 1995Brinkman et al, 1996) and highly ampli®ed in others, e.g. breast cancer, where it correlates with aggressiveness and poor prognosis (Tanner et al, 1995).…”

Section: Expression Of Cir1/croc1 In Human Tissues and Tumor-derived mentioning

confidence: 99%

Up-regulation of CIR1/CROC1 expression upon cell immortalization and in tumor-derived human cell lines

Broomfield

Lavery

et al. 1998

Oncogene

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Acquisition of the immortal phenotype by tumor cells represents an essential and potentially rate-limiting step in tumorigenesis. To identify changes in gene expression that are associated with the early stages of cell immortalization, we compared genetically matched pairs of pre-immortal and immortal human cell clones by mRNA di erential display. Two transcripts, denoted CIR1 and CIR2, were identi®ed which were up-regulated in immortal cells. Sequence analysis revealed CIR1 to be identical to the recently cloned CROC1/UEV-1 gene, whereas CIR2 corresponds to an as yet uncharacterized 1.2 kb mRNA. A 5 ± 6-fold elevation in CIR1/CROC1 expression and a 2 ± 3-fold elevation in CIR2 expression were observed in SV40-transformed human enbryonic kidney cells immediately following proliferative crisis, suggesting a potential role for these genes in immortalization. Expression of CIR1/CROC1 was found to be elevated also in a variety of immortal human tumorderived cell lines, as compared to their normal tissue counterparts. These results are compatible with induction of CIR1/CROC1 being an early event in the acquisition of immortality and with a role for this gene in the immortal phenotype of tumor cells.

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“…The relatively low CGH concordances and correlations involving 19q alterations resulted, in part, from using microsatellite markers and FISH probes that map to 19q13.3, a region in human gliomas that often contains deletions below the resolution of CGH. Furthermore, CGH has known artifacts at both 1p and 19q (Kallioniemi et al, 1994;Kim et al, 1995;Mohapatra et al, 1995).…”

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Localization of common deletion regions on 1p and 19q in human gliomas and their association with histological subtype

et al. 1999

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Allelic alterations of chromosomes 1 and 19 are frequent events in human di use gliomas and have recently proven to be strong predictors of chemotherapeutic response and prolonged survival in oligodendrogliomas (Cairncross et al., 1998; Smith et al., submitted). Using 115 human di use gliomas, we localized regions of common allelic loss on chromosomes 1 and 19 and assessed the association of these deletion intervals with glioma histological subtypes. Further, we evaluated the capacity of multiple modalities to detect these alterations, including loss of heterozygosity (LOH),¯uorescence in situ hybridization (FISH), and comparative genomic hybridization (CGH). The correlation coe cients for detection of 1p and 19q alterations, respectively, between modalities were: 0.98 and 0.87 for LOH and FISH, 0.79 and 0.60 for LOH and CGH, and 0.79 and 0.53 for FISH and CGH. Minimal deletion regions were de®ned on 19q13.3 (D19S412-D19S596) and 1p (D1S468-D1S1612). Loss of the 1p36 region was found in 18% of astrocytomas (10/55) and in 73% (24/33) of oligodendrogliomas (P50.0001), and loss of the 19q13.3 region was found in 38% (21/55) of astrocytomas and 73% (24/33) of oligodendrogliomas (P=0.0017). Loss of both regions was found in 11% (6/55) of astrocytomas and in 64% (21/33) of oligodendrogliomas (P50.0001). All gliomas with LOH on either 1p or 19q demonstrated loss of the corresponding FISH probe, 1p36 or 19q13.3, suggesting not only locations of putative tumor suppressor genes, but also a simple assay for assessment of 1p and 19q alterations as diagnostic and prognostic markers.

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Detection and mapping of amplified DNA sequences in breast cancer by comparative genomic hybridization.

Cited by 647 publications

References 20 publications

The role of the MKK6/p38 MAPK pathway in Wip1-dependent regulation of ErbB2-driven mammary gland tumorigenesis

The role of the MKK6/p38 MAPK pathway in Wip1-dependent regulation of ErbB2-driven mammary gland tumorigenesis

Up-regulation of CIR1/CROC1 expression upon cell immortalization and in tumor-derived human cell lines

Localization of common deletion regions on 1p and 19q in human gliomas and their association with histological subtype

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