Abstract

The Jun Kinase/Stress-activated protein kinase pathway (JNK/SAPK) has been implicated as mediating stress-responses, survival, proliferation, and apoptosis. Previous studies, principally by C. Der and co-workers and M. Karin, in which this laboratory participated, have shown the JNK pathway is required for the transformation of primary fibroblasts by the activated ras oncogene and related oncogenes. We have extended the JNK analysis to human tumor cells. JNK is commonly serum-inducible or constitutively active in a variety of human tumor cells. Specific inhibition blocks tumor cell growth. Moreover, stable expression of a dominant negative inhibitor, c-Jun (S63A, S73A), blocks DNA repair and greatly sensitizes human tumor lines (T98G glioblastoma, A549 lung, MCF-7 breast, and PC3 prostate carcinoma) to killing by cisplatin, up to 9.7-fold for PC3 cells. We hypothesize that during progression of cancer, the JNK pathway is commonly selected as greatly enhancing DNA repair and synthesis, thereby facilitating oncongenesis. To test this, highly specific antisense compounds complementary to the two isoform families JNK1 and JNK2 have been developed and characterized. Systemic antisense treatment of athymic mice bearing established PC3 xenografts inhibits growth by 79 percent, better than cisplatin (49 percent), and combined antisense treatment promotes complete regression in high frequency. Conversely, PC3 cells are 100 percent tumorigenic. To test the generality, eight additional prostate cell lines were found to proliferate in direct proportion to the serum-inducible level of JNK activity over a 9-fold range. Moreover antisense JNK2 but not antisense JNK1 nearly completely blocks the growth of all lines in proportion to the JNK activity strongly indicating that JNK2 is commonly required for serum-stimulated growth prostate carcinoma cells. It is proposed to test the hypothesis that JNK is oncogenic in prostate carcinoma. We will test whether JNK is required for proliferation of prostate carcinoma lines in vitro (Aim 1) and in vivo (Aim 2). The efficacy of antisense JNK will be tested critically in the TRAMP model (Aim 2). The mechanism of oncogenesis by JNK will be tested by determining whether predicted DNA synthesis genes are expressed in tumor cells (Aim 3) and prostate tumor specimens (Aim 4) using established cDNA arrays. Microarrays will be constructed that utilize 35,000 NIH/CGAP sequence verified cancer expression library obtained by cloning from laser capture microdissection human tumor specimens. These studies test a novel hypothesis and test the utility of new inhibitors for the treatment of prostate carcinoma.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA084107-05
Application #
6790645
Study Section
Metabolic Pathology Study Section (MEP)
Program Officer
Perry, Mary Ellen
Project Start
2000-07-31
Project End
2005-06-30
Budget Start
2004-09-15
Budget End
2005-06-30
Support Year
5
Fiscal Year
2004
Total Cost
$34,638
Indirect Cost

  Institution

Name
Sidney Kimmel Cancer Center
Department
Type
DUNS #
789644697
City
San Diego
State
CA
Country
United States
Zip Code
92121

  Publications

Baron, V; Adamson, E D; Calogero, A et al. (2006) The transcription factor Egr1 is a direct regulator of multiple tumor suppressors including TGFbeta1, PTEN, p53, and fibronectin. Cancer Gene Ther 13:115-24
Wang, Yipeng; Yu, Qiuju; Cho, Ann H et al. (2005) Survey of differentially methylated promoters in prostate cancer cell lines. Neoplasia 7:748-60
Wang, Yipeng; Hayakawa, Jun; Long, Fred et al. (2005) ""Promoter array"" studies identify cohorts of genes directly regulated by methylation, copy number change, or transcription factor binding in human cancer cells. Ann N Y Acad Sci 1058:162-85
Hayakawa, Jun; Mittal, Shalu; Wang, Yipeng et al. (2004) Identification of promoters bound by c-Jun/ATF2 during rapid large-scale gene activation following genotoxic stress. Mol Cell 16:521-35
Hayakawa, Jun; Depatie, Chantal; Ohmichi, Masahide et al. (2003) The activation of c-Jun NH2-terminal kinase (JNK) by DNA-damaging agents serves to promote drug resistance via activating transcription factor 2 (ATF2)-dependent enhanced DNA repair. J Biol Chem 278:20582-92
Yang, Yong-Min; Bost, Frederic; Charbono, Wilfried et al. (2003) C-Jun NH(2)-terminal kinase mediates proliferation and tumor growth of human prostate carcinoma. Clin Cancer Res 9:391-401
Baron, Veronique; De Gregorio, Giorgia; Krones-Herzig, Anja et al. (2003) Inhibition of Egr-1 expression reverses transformation of prostate cancer cells in vitro and in vivo. Oncogene 22:4194-204
Glinsky, Gennadi V; Krones-Herzig, Anja; Glinskii, Anna B et al. (2003) Microarray analysis of xenograft-derived cancer cell lines representing multiple experimental models of human prostate cancer. Mol Carcinog 37:209-21
Virolle, Thierry; Krones-Herzig, Anja; Baron, Veronique et al. (2003) Egr1 promotes growth and survival of prostate cancer cells. Identification of novel Egr1 target genes. J Biol Chem 278:11802-10
Adamson, Eileen D; Mercola, Dan (2002) Egr1 transcription factor: multiple roles in prostate tumor cell growth and survival. Tumour Biol 23:93-102