Microcell-Mediated Chromosome Transfer Identifies EPB41L3 as a Functional Suppressor of Epithelial Ovarian Cancers

Dimitra Dafou; Barbara Grun; John Sinclair; Kate Lawrenson; Elizabeth C. Benjamin; Estrid Hogdall; Susanne Kruger-Kjaer; Lise Christensen; Heidi M. Sowter; Ahmed Al-Attar; Richard Edmondson; Stephen Darby; Andrew Berchuck; Peter W. Laird; C. Leigh Pearce; Susan J. Ramus; Ian J. Jacobs; Simon A. Gayther

doi:10.1593/neo.10340

Neoplasia: An International Journal for Oncology Research (Jul 2010)

Microcell-Mediated Chromosome Transfer Identifies EPB41L3 as a Functional Suppressor of Epithelial Ovarian Cancers

Dimitra Dafou,
Barbara Grun,
John Sinclair,
Kate Lawrenson,
Elizabeth C. Benjamin,
Estrid Hogdall,
Susanne Kruger-Kjaer,
Lise Christensen,
Heidi M. Sowter,
Ahmed Al-Attar,
Richard Edmondson,
Stephen Darby,
Andrew Berchuck,
Peter W. Laird,
C. Leigh Pearce,
Susan J. Ramus,
Ian J. Jacobs,
Simon A. Gayther

Affiliations

Dimitra Dafou: EGA Institute for Women’s Health, Gynaecological Cancer Research Laboratories, University College London, London, UK
Barbara Grun: EGA Institute for Women’s Health, Gynaecological Cancer Research Laboratories, University College London, London, UK
John Sinclair: Cancer Proteomics Laboratory, University College London, London, UK
Kate Lawrenson: EGA Institute for Women’s Health, Gynaecological Cancer Research Laboratories, University College London, London, UK
Elizabeth C. Benjamin: Department of Histopathology, Royal Free/JCL Medical School, London, UK
Estrid Hogdall: Institute of Cancer Epidemiology, Danish CancerSociety, Copenhagen, Denmark
Susanne Kruger-Kjaer: Institute of Cancer Epidemiology, Danish CancerSociety, Copenhagen, Denmark
Lise Christensen: Department of Pathology, Bispebjerg Hospital, University of Copenhagen, Copenhagen, Denmark
Heidi M. Sowter: University of Derby, Faculty of Education, Health and Science, Kedleston Road, Derby, UK
Ahmed Al-Attar: Academic Department of Clinical Oncology, University of Nottingham, Nottingham University Hospitals, Nottingham, UK
Richard Edmondson: Northern Institute for Cancer Research, Newcastle Upon Tyne, UK
Stephen Darby: Northern Institute for Cancer Research, Newcastle Upon Tyne, UK
Andrew Berchuck: Division of Preventive Medicine, The Duke Comprehensive Cancer Center, Durham, NC, USA
Peter W. Laird: University of Southern California, USC Epigenome Center, Los Angeles, CA, USA
C. Leigh Pearce: University of Southern California, Department of Preventive Medicine, Keck School of Medicine, Los Angeles, CA, USA
Susan J. Ramus: EGA Institute for Women’s Health, Gynaecological Cancer Research Laboratories, University College London, London, UK
Ian J. Jacobs: EGA Institute for Women’s Health, Gynaecological Cancer Research Laboratories, University College London, London, UK
Simon A. Gayther: EGA Institute for Women’s Health, Gynaecological Cancer Research Laboratories, University College London, London, UK

DOI: https://doi.org/10.1593/neo.10340
Journal volume & issue: Vol. 12, no. 7
pp. 579 – 589

Abstract

Read online

We used a functional complementation approach to identify tumor-suppressor genes and putative therapeutic targets for ovarian cancer. Microcell-mediated transfer of chromosome 18 in the ovarian cancer cell line TOV21 G induced in vitro and in vivo neoplastic suppression. Gene expression microarray profiling in TOV21 +19 hybrids identified 14 candidate genes on chromosome 18 that were significantly overexpressed and therefore associated with neoplastic suppression. Further analysis of messenger RNA and protein expression for these genes in additional ovarian cancer cell lines indicated that EPB41L3 (erythrocyte membrane protein band 4.1-like 3, alternative names DAL-1 and 4.1 B) was a candidate ovarian cancer-suppressor gene. Immunoblot analysis showed that EPB41L3 was activated in TOV21 +18 hybrids, expressed in normal ovarian epithelial cell lines, but was absent in 15 (78%) of 19 ovarian cancer cell lines. Using immunohistochemistry, 66% of 794 invasive ovarian tumors showed no EPB41L3 expression compared with only 24% of benign ovarian tumors and 0% of normal ovarian epithelial tissues. EPB41L3 was extersively methylated it ovarian cancer cell Hires and primary ovarian tumors compared with normal tissues (P = 00004), suggesting this may be the mechanism of gene inactivation it ovarian cancers. Constitutive reexpressior of EPB41L3 it a three-dimensional multicellular spheroid model of ovarian cancer caused significant growth suppressior and induced apoptosis. Transmission and scanning electron microscopy demonstrated many similarities between EPB41L3-expressing cells and chromosome 18 donor-recipient hybrids, suggesting that EPB41L3 is the gene responsible for reoplastic suppression after chromosome 18 transfer. Finally, ar irducible model of EPB41L3 expression it three-dimersioral spheroids confirmed that reexpression of EPB41L3 induces extensive apoptotic cell death it ovarian cancers.

Published in Neoplasia: An International Journal for Oncology Research

ISSN: 1522-8002 (Print); 1476-5586 (Online)
Publisher: Elsevier
Country of publisher: United States
LCC subjects: Medicine: Internal medicine: Neoplasms. Tumors. Oncology. Including cancer and carcinogens
Website: http://www.journals.elsevier.com/neoplasia/

About the journal