eprintid: 4029 rev_number: 8 eprint_status: archive userid: 1 dir: disk0/00/00/40/29 datestamp: 2003-11-03 11:39:43 lastmod: 2014-04-03 13:20:32 status_changed: 2012-08-14 15:09:45 type: doctoralThesis metadata_visibility: show creators_name: De Castro Arce, Johanna title: RAR beta trans-repression of AP-1 transcription factor in HeLa cervical cancer cells : consequences on transcription of viral and cellular AP-1 controlled genes ispublished: pub subjects: ddc-570 divisions: i-850300 adv_faculty: af-14 keywords: RAR beta , AP-1 , c-JunRAR beta , AP-1 , c-Jun cterms_swd: RAR beta cterms_swd: AP-1 cterms_swd: c-Jun abstract: In many types of cancer, including cervical cancer, the nuclear retinoic receptor ß2 (RARß2) gene is epigenetically modified and unable to be significantly induced. RARß2 can act as a tumor suppressor, since loss of its expression is associated with human tumor progression. One mechanism of RARß2-mediated growth inhibition is based on its ability to constitutively repress the AP-1 transcription factor, but this mechanism has never been demonstrated in cervical cancer cells. In this thesis the biological consequences of reconstitute RARß2 receptor expression in cervical cancer cells was investigated. For this purpose, human papillomavirus HPV-18 positive HeLa cells were stably transfected with RARß2 cDNA under the control of the ß-actin promoter. The characterization of the RARß2 tranfectants revealed a strongly reduced AP-1 binding to the corresponding specific oligonucleotides, even in the absence of atRA treatment. In HeLa cells, the AP-1 reduction correlates with diminished HPV-18 oncogene transcription and slower cellular growth. Western blot analysis demonstrated that the only member of the AP-1 family consistently reduced in HeLa RARß2 clones was c-Jun, despite ongoing gene expression. In order to understand by which mechanism c-Jun is reduced, and since the phosphorylation of c-Jun is important for protein stabilization, HeLa RARß2 clones were treated with different c-Jun-N-terminal kinase (JNK) stimulators. The treatments resulted in a c-Jun increase at RNA and protein levels, and led to a reconstitution of AP-1 binding similar to non-transfected HeLa controls. However, the reconstitution of AP-1 binding levels did not have an inductor effect on the HPV-18 oncogenes, the expression of which has been postulated to be AP-1 dependent. Other classical AP-1 regulated genes such as metalloproteinases were up regulated as expected. In conclusion, the data of this thesis indicate that RARß2 induced a destabilization and accelerated degradation of c-Jun at the protein level responsible for the AP-1 reduction. The mechanism of AP-1 trans-repression in HeLa cells is different from that postulated for other cancer cell models. All changes produced in HeLa cells after RARß2 constitutive expression lead to reduced cell proliferation, which can be associated with the RARß2 tumor suppressor function. abstract_translated_lang: eng date: 2003 date_type: published id_scheme: DOI id_number: 10.11588/heidok.00004029 ppn_swb: 1643531514 own_urn: urn:nbn:de:bsz:16-opus-40290 date_accepted: 2003-10-28 advisor: HASH(0x559e37ccab30) language: eng bibsort: DECASTROARRARBETATRA2003 full_text_status: public citation: De Castro Arce, Johanna (2003) RAR beta trans-repression of AP-1 transcription factor in HeLa cervical cancer cells : consequences on transcription of viral and cellular AP-1 controlled genes. [Dissertation] document_url: https://archiv.ub.uni-heidelberg.de/volltextserver/4029/1/Thesis_UNI.pdf