Irreversible JNK1-JUN inhibition by JNK-IN-8 sensitizes pancreatic cancer to 5-FU/FOLFOX chemotherapy
Matthew B. Lipner, Xianlu L. Peng, Chong Jin, Yi Xu, Yanzhe Gao, Michael P. East, Naim U. Rashid, Richard A. Moffitt, Silvia G. Herrera Loeza, Ashley B. Morrison, Brian T. Golitz, Cyrus Vaziri, Lee M. Graves, Gary L. Johnson, Jen Jen Yeh
Matthew B. Lipner, Xianlu L. Peng, Chong Jin, Yi Xu, Yanzhe Gao, Michael P. East, Naim U. Rashid, Richard A. Moffitt, Silvia G. Herrera Loeza, Ashley B. Morrison, Brian T. Golitz, Cyrus Vaziri, Lee M. Graves, Gary L. Johnson, Jen Jen Yeh
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Research Article Oncology Therapeutics

Irreversible JNK1-JUN inhibition by JNK-IN-8 sensitizes pancreatic cancer to 5-FU/FOLFOX chemotherapy

Abstract

Over 55,000 people in the United States are diagnosed with pancreatic ductal adenocarcinoma (PDAC) yearly, and fewer than 20% of these patients survive a year beyond diagnosis. Chemotherapies are considered or used in nearly every PDAC case, but there is limited understanding of the complex signaling responses underlying resistance to these common treatments. Here, we take an unbiased approach to study protein kinase network changes following chemotherapies in patient-derived xenograft (PDX) models of PDAC to facilitate design of rational drug combinations. Proteomics profiling following chemotherapy regimens reveals that activation of JNK-JUN signaling occurs after 5-fluorouracil plus leucovorin (5-FU + LEU) and FOLFOX (5-FU + LEU plus oxaliplatin [OX]), but not after OX alone or gemcitabine. Cell and tumor growth assays with the irreversible inhibitor JNK-IN-8 and genetic manipulations demonstrate that JNK and JUN each contribute to chemoresistance and cancer cell survival after FOLFOX. Active JNK1 and JUN are specifically implicated in these effects, and synergy with JNK-IN-8 is linked to FOLFOX-mediated JUN activation, cell cycle dysregulation, and DNA damage response. This study highlights the potential for JNK-IN-8 as a biological tool and potential combination therapy with FOLFOX in PDAC and reinforces the need to tailor treatment to functional characteristics of individual tumors.

Authors

Matthew B. Lipner, Xianlu L. Peng, Chong Jin, Yi Xu, Yanzhe Gao, Michael P. East, Naim U. Rashid, Richard A. Moffitt, Silvia G. Herrera Loeza, Ashley B. Morrison, Brian T. Golitz, Cyrus Vaziri, Lee M. Graves, Gary L. Johnson, Jen Jen Yeh

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Figure 1

5-FU and FOLFOX chemotherapy regimens induce druggable activation of JNK and JUN.

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5-FU and FOLFOX chemotherapy regimens induce druggable activation of JNK...
(A) MIB-MS performed on PDX tumors biopsied before and after treatment with individual chemotherapy regimens (5-FU, 8-day [8d] 100 mg/kg 5-FU + LEU in P108-T1 PDX tumors; OX, 8d 5 mg/kg in P108-T1 PDX tumors; GEM, 3d 80 mg/kg in P108-T1 PDX tumors) or FOLFOX compared with vehicle-treated PDX tumors (3d 100 mg/kg 5-FU + LEU and 5 mg/kg OX in P319-T1 PDX tumors). JNK1 (MAPK8) and JNK2 (MAPK9) are shaded red, and kinases known to activate JNK are shaded blue. Biological replicate values are indicated by cyan and yellow dots (n = 2). (B) RNA-seq expression of predicted JUN transcriptional target genes (MSigDB: CREBP1CJUN_01) in FOLFOX-treated and matched pretreatment biopsy tumors, with labeled genes with known roles in cancer signaling. (C) Representative immunoblots showing upregulation of p-JUN after indicated doses of FOLFOX in PDX-derived lines P411-T1 and P422-T1, as well as ATCC cell lines CFPAC-1 and MIA PaCa-2. Vertical line indicates noncontiguous samples that were treated and collected simultaneously and run on the same gels. KU80 used as loading control.