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Cisplatin Mimics ARF Tumor Suppressor Regulation of RelA (p65) Nuclear Factor-B Transactivation

School of Life Sciences, Division of Gene Regulation and Expression, University of Dundee, Dundee, Scotland, United Kingdom

Requests for reprints: Neil D. Perkins, School of Life Sciences, Division of Gene Regulation and Expression, University of Dundee, MSI/WTB Complex, Dow Street, Dundee, DD1 5EH, Scotland, United Kingdom. Phone: 44-1382-345-606; Fax: 44-1382-348-072; E-mail: n.d.perkins{at}dundee.ac.uk.

	Abstract

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The RelA (p65) nuclear factor-B (NF-B) subunit can contribute towards tumor cell survival through inducing the expression of a variety of antiapoptotic genes. However, the NF-B response can show great diversity and is not always antiapoptotic. Here, we find that cisplatin, a DNA cross-linking agent and commonly used anticancer compound, does not affect RelA nuclear translocation but modulates its transcriptional activity. Similar to other genotoxic agents, such as daunorubicin and UV light, cisplatin treatment in the U-2 OS osteosarcoma cell line represses RelA activity and inhibits expression of the NF-B antiapoptotic target gene Bcl-x_L. The mechanism through which cisplatin achieves these effects is different to daunorubicin and UV light but shows great similarity to the RelA regulatory pathway induced by the ARF tumor suppressor: cisplatin regulation of RelA requires ATR/Chk1 activity, represses Bcl-x_L but not XIAP expression, and results in phosphorylation of RelA at Thr⁵⁰⁵. In contrast to these results, another chemotherapeutic drug etoposide activates NF-B and induces expression of these target genes. Thus, within a single tumor cell line, there is great heterogeneity in the NF-B response to different, commonly used chemotherapeutic drugs. These observations suggest that it might be possible to minimize the ability of RelA to inhibit cancer therapy by diagnostically predicting the type of chemotherapeutic drug most compatible with NF-B functionality in a tumor cell type. Moreover, our data indicate that at least with respect to RelA, cisplatin functions as an ARF mimic. Other drugs capable of mimicking this aspect of ARF function might therefore have therapeutic potential. (Cancer Res 2006; 66(2): 929-35)

	Introduction

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Aberrantly active nuclear factor-B (NF-B) is associated with diseases of an inflammatory origin, such as rheumatoid arthritis and inflammatory bowel disease, as well as cancer (1–4). Moreover, NF-B provides the link between chronic inflammation and tumor development, thought to cause up to 20% of human cancers (5–7). These effects result not only from NF-B's ability to control the expression of genes required for inflammation and the immune response but also from its function as an important regulator of apoptosis and cellular proliferation (8, 9). NF-B, and specifically the RelA (p65) subunit, is frequently considered an antiapoptotic protein due to the liver apoptosis and subsequent embryonic lethality found with rela null mice, resulting from increased sensitivity to tumor necrosis factor- (TNF-)–induced cell death (10). NF-B has now been found to promote resistance to apoptosis by a wide variety of agents, which in addition to natural molecules, such as TNF, include a number of chemotherapeutic drugs and ionizing radiation (9). Therefore, in addition to a role in tumorigenesis, NF-B is also thought to reduce the efficiency of cancer therapy (11). For these reasons, drugs targeting the NF-B pathway are being actively investigated and developed as both anticancer and anti-inflammatory agents (12–14).

The antiapoptotic function of NF-B results principally from its ability to transcriptionally induce the expression of antiapoptotic genes, such as cIAP1, cIAP2, XIAP, Blf/A1, and Bcl-x_L (9). However, in common with many other transcriptional regulators, NF-B subunits do not always target the same genes regardless of activating stimuli. For example, RelA is not always antiapoptotic, and in some circumstances, the RelA subunit can induce the expression of proapoptotic target genes, such as Fas, FasL, and death receptors DR4 and DR5 (9). Moreover, we have recently shown that under some circumstances, RelA can repress the expression of antiapoptotic genes. We observed that atypical inducers of NF-B activity, such as the chemotherapeutic agents daunorubicin and doxorubicin as well as UV-C light, resulted in RelA-dependent repression of Bcl-x_L, XIAP, and A20 gene expression (15). Daunorubicin and doxorubicin are structurally related topoisomerase II inhibitors and DNA interchelators, whereas UV-C treatment induces pyrimidine dimer cross-linking resulting in single-strand DNA breaks. These stimuli all induced RelA DNA binding, and chromatin immunoprecipitation analysis showed that RelA was promoter associated under these conditions. In contrast to those activators of RelA associated with increased expression of these genes, these atypical inducers resulted in the association of RelA with histone deacetylases (HDAC), which function as repressors of gene expression. Therefore, whether NF-B prevents or facilitates apoptosis is stimulus, cell type, and context dependent (9).

In another work from our laboratory, we have discovered that the ARF tumor suppressor, although not an inducer of NF-B DNA binding, modulates RelA transcriptional activity. Indeed, similar to the results described above, we find that ARF expression results in repression of the antiapoptotic gene Bcl-x_L by RelA through induced association with HDAC1 (16). Furthermore, ARF sensitizes cells to TNF-induced cell death (16). However, the effect of ARF on RelA was in other ways distinct to that of daunorubicin/doxorubicin and UV-C. Significantly, ARF-induced repression of NF-B transcriptional activity requires the evolutionarily conserved Thr⁵⁰⁵ residue of RelA and the ATR/Chk1 kinase pathway (16, 17). We found that ARF modulates ATR/Chk1 activity, and that Chk1 phosphorylates Thr⁵⁰⁵ (17). In contrast, repression of transcription by RelA in response to daunorubicin/doxorubicin and UV-C does not require Thr⁵⁰⁵ or ATR/Chk1, despite the fact that these DNA-damaging agents also activate Chk1 (15, 16).

These findings led us to hypothesize that there may be multiple classes of "repressor" RelA, with distinct properties (18). Furthermore, they indicated that the function of NF-B in cancer, and RelA in particular, might be more complex than merely functioning as a tumor promoter (19). Indeed, NF-B might function more analogously to a tumor suppressor under some circumstances, particularly in the early stages of tumorigenesis before the function of the ARF/p53 pathway is lost (19). Our data also suggested that the response of NF-B to distinct cancer therapies might also vary, depending on the cell type and context. Although in the cell types we examined, daunorubicin/doxorubicin treatment resulted in a form of RelA that repressed transcription, we also observed that another topoisomerase II inhibitor (etoposide) induced the opposing form of NF-B, at least in a reporter gene assay (15). Therefore, DNA damage per se does not result in the transcriptional repressor form of RelA. Rather, these observations, together with the results from our ARF studies, indicated that there is great potential for heterogeneity in the NF-B response to cell stimuli. Given the role of NF-B in tumorigenesis and apoptosis, such differing responses could profoundly affect the effectiveness of cancer therapies, particularly if NF-B inhibitors come into common clinical usage. With this in mind, we have begun to extend our studies to investigate the precise mechanisms through which other chemotherapeutic agents affect NF-B–dependent transcription. In this report, we have investigated the effects of cisplatin on RelA function. Cisplatin is a DNA cross-linking agent used in the treatment of solid tumors of testes, ovaries, and the head and neck (20). It is also used in the treatment of osteosarcoma (21). Cisplatin generates DNA adducts but unlike daunorubicin, doxorubicin, or etoposide does not inhibit topoisomerase II. Here, we show that similar to daunorubicin, cisplatin induces repression of NF-B–dependent reporter gene and endogenous Bcl-x_L expression. Surprisingly, this repression is distinct to that seen with daunorubicin and UV-C. Rather, cisplatin mimics the effects we had previously seen with ARF. In particular, cisplatin modulation of RelA is ATR/Chk1 dependent and requires phosphorylation of RelA at Thr⁵⁰⁵.

	Materials and Methods

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Cells. U-2 OS osteosarcoma cells were obtained from the European Collection of Cell Cultures (Salisbury, United Kingdom) and were not grown beyond passage 35. NARF2 cells are a derivative of U-2 OS cells, which contain a stably integrated, isopropyl-L-thio-B-D-galactopyranoside (IPTG) inducible ARF expression plasmid and have been described previously (16, 22). HeLa 57A cells, which contain a chromosomally integrated NF-B luciferase reporter plasmid, were grown and analyzed as previously described (23).

Where indicated, endogenous NF-B activity was induced by 10 ng/mL TNF- (Sigma, Gillingham, United Kingdom), 1 µmol/L daunorubicin (Affiniti, Exeter, United Kingdom), 4 µg/mL cisplatin (Sigma), or 40 J/m² UV-C (254 nm) using a Stratalinker (Stratagene, Amsterdam, the Netherlands). Endogenous Chk1 activity was inhibited by prestimulation with 1 µmol/L Gö6976 (Calbiochem, Nottingham, United Kingdom).

Antibodies. All antibodies have been described previously (15, 17), except the new goat anti-RelA phospho-T505 antibody. This antibody used the same peptide immunogen as described previously (17) and was raised by Pacific Immunology Corp. (Ramona, CA) as part of a collaboration with Active Motif. This antibody was purified using both phospho-peptide and non–phospho-peptide affinity chromatography. Peptide ELISA confirmed that the resulting purified antibody specifically recognizes the phosphorylated T505 epitope.

Other experimental procedures. All reporter plasmid luciferase assays, chromatin immunoprecipitation assays, semiquantitative PCR, immunofluorescence microscopy, electrophoretic mobility shift assay (EMSA), Western blots, and immunoprecipitations were done as described previously (15–17). All antibodies, plasmids, PCR primers, and small interfering RNAs (siRNA) have been described and characterized before (15–17). Luciferase assays were done according to the manufacturer's instructions (Promega, Southampton, United Kingdom), and results were normalized for protein concentration with all experiments done a minimum of three times before calculating means and SD as shown in the figures.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

 
Cisplatin represses NF-B–dependent transcription. Treatment of human osteosarcoma U-2 OS cells with daunorubicin or doxorubicin results in active repression of transcription by the RelA subunit of NF-B (15). Here, we extend these observations to another chemotherapeutic drug, cisplatin, which, although a DNA-damaging agent, is chemically and mechanistically distinct to these other compounds. It was a surprise, therefore, when treatment of U-2 OS cells with cisplatin for 8 hours repressed the activity of an NF-B–responsive luciferase reporter plasmid to a magnitude similar to that seen with daunorubicin (Fig. 1A). In contrast, and as expected, TNF strongly induced NF-B activity. These effects were dependent upon the B elements present in this plasmid, suggesting a direct effect on NF-B (Fig. 1A). Cisplatin treatment also repressed the activity of a chromosomally integrated, 3x B luciferase reporter plasmid in HeLa 57A cells (Fig. 1B), which we have previously shown to be strongly activated by TNF (23).

View larger version (41K): [in this window] [in a new window]   Figure 1. Cisplatin represses NF-B–dependent transcription. A, TNF activates, whereas cisplatin and daunorubicin repress NF-B reporter plasmid activity. U-2 OS cells were transfected with 2 µg of 3x B concanavalin A luciferase NF-B reporter plasmid or a control lacking B sites as indicated. Cells were either unstimulated or stimulated for 8 hours with 10 ng/mL TNF, 4 µg/mL cisplatin, or 1 µmol/L daunorubicin, 36 hours after transfection. Fold activation or repression relative to levels seen in untreated controls. Normalized such that no change in luciferase activity has a value of 0. B, cisplatin represses NF-B activity in HeLa cells. HeLa 57A cells, which contain a chromosomally integrated 3x B reporter plasmid, were treated as in (A). C-D, cisplatin inhibits expression of Bcl-xL but not XIAP mRNA. RNA was prepared from U-2 OS cells treated with either 4 µg/mL cisplatin or 15 µmol/L etoposide for the indicated times (C), 1 µmol/L daunorubicin, or 40 J/m2 UV-C for 0 or 6 hours (D, right) or the U-2 OS cell derivative NARF2, where ARF was induced by 1 mmol/L IPTG for 0 or 24 hours (D, left). Semiquantitative PCR analysis was done using 5 ng total RNA, with primers specific to human XIAP, Bcl-xL, or a glyceraldehyde-3-phosphate dehydrogenase (GAPDH) control.

Cisplatin stimulation does not induce NF-B DNA binding or nuclear translocation. Analysis of NF-B DNA binding by EMSA revealed that cisplatin did not induce binding to the consensus HIV B site over an 8-hour time course of stimulation in U-2 OS cells (Fig. 2A). In contrast, the other DNA-damaging agents daunorubicin and etoposide both robustly induced NF-B DNA-binding in the same cells (Fig. 2A). Furthermore, immunofluorescence analysis confirmed that cisplatin, unlike UV-C–induced DNA damage, does not induce RelA nuclear localization; therefore, the failure to observe stimulation of DNA binding by EMSA does not reflect more subtle effects on NF-B's affinity for its binding site (Fig. 2B). This effect was again reminiscent of the effects we had previously seen with ARF. Here, ARF does not induce NF-B DNA binding but rather modulates the activity of the basal or induced NF-B already present in the nucleus (16). This effect of ARF was confirmed by immunofluorescence analysis (Fig. 2B). We had previously observed that ARF was capable of repressing the transcriptional activity of TNF-induced NF-B but did not affect TNF-induced NF-B DNA binding (16). To determine whether cisplatin could exert a similar dominant effect on TNF-induced NF-B, U-2 OS cells were treated with both stimuli. This experiment revealed that cisplatin does inhibit the transcriptional activity of TNF-induced NF-B, although not completely (Fig. 2C). Moreover, cisplatin does not inhibit TNF-induced NF-B DNA binding. In fact, a slight enhancement was typically observed (Fig. 2D). Supershift analysis also revealed that both the basal and induced levels of NF-B in U-2 OS cells consisted primarily of RelA containing complexes (Fig. 2D). It should be noted that in U-2 OS cells, the ARF promoter is methylated; thus, the cells are functionally ARF null (24). In addition, we have confirmed that cisplatin treatment does not induce ARF expression in these cells (data not shown).

View larger version (54K): [in this window] [in a new window]   Figure 2. Cisplatin and ARF do not induce NF-B DNA binding or RelA nuclear translocation. A, EMSA analysis using nuclear protein extracts from U-2 OS cells treated with either 4 µg/mL cisplatin (left) or 15 µmol/L etoposide (right) for the indicated times. A lane using 1 µmol/L daunorubicin-treated cells (3 hours) is also shown. EMSA analysis was done using a 32P-labeled consensus Ig/HIV B probe. B, immunofluorescence analysis of RelA nuclear localization following cisplatin treatment. U-2 OS were plated onto coverslips and fixed after 4 µg/mL cisplatin (4 hours) or 40 J/m2 UV-C (4 hours) treatment. Cells were stained with rabbit anti-RelA antibody (Santa Cruz Biotechnology, Santa Cruz, CA) or 4',6-diamidino-2-phenylindole (DAPI) to reveal DNA. In addition, NARF2 cells were treated with 1 mmol/L IPTG for 0 or 24 hours to induce ARF and similarly stained for RelA. Cells were analyzed, and images were acquired using a DeltaVision microscope. C, cisplatin treatment represses TNF-induced NF-B activity. U-2 OS cells were transfected as in Fig. 1A, except that some transfected cells were also treated with TNF (8 hours) and/or cisplatin (6 hours). D, cisplatin does not inhibit TNF-induced NF-B DNA binding. EMSA analysis was done as in (A), except that cells were treated with 10 ng/mL TNF for 30 minutes or cisplatin for 4 hours either alone or in combination. Where indicated, supershift analysis was done with a specific anti-RelA antibody.

View larger version (14K): [in this window] [in a new window]   Figure 3. Cisplatin does not affect RelA binding to the Bcl-xL promoter but does induce HDAC1 recruitment. Control or cisplatin-treated U-2 OS cells were harvested, and chromatin immunoprecipitation analysis was done with the indicated RelA, HDAC1, acetylated H3 (Lys9 and Lys14) or Gal4 control antibodies using primers to the Bcl-xL or glyceraldehyde-3-phosphate dehydrogenase (GAPDH) promoters.

View larger version (45K): [in this window] [in a new window]   Figure 4. Cisplatin repression of NF-B requires the ATR/Chk1 pathway. A, cisplatin represses the RelA transactivation domain in a Thr505-dependent manner. U-2 OS cells were transfected with 2 µg of Gal4 luciferase reporter plasmid together with expression plasmids encoding either the Gal4 RelA (TAD) or Gal4 RelA (TAD T505A) expression plasmids as indicated. Thirty-two hours after transfection, cells were either left untreated or stimulated for (16 hours) with 4 µg/mL cisplatin. Relative luciferase activity per microgram of protein. The RelA transactivation domain (TAD) used in this study encodes amino acids 428 to 551 of human RelA. B, cisplatin-mediated repression of NF-B activity requires ATR. U-2 OS cells were transfected as in Fig. 1A and treated with either 4 µg/mL cisplatin or 40 J/m2 UV-C for 0 or 8 hours. Cells also included 1 µg of kinase-dead ATR expression plasmid or a control plasmid as indicated. C, siRNAs targeting ATR and Chk1 abolish cisplatin-induced repression of Bcl-xL. PCR analysis of Bcl-xL expression was done following treatment of U-2 OS cells with the indicated siRNAs. Analysis of ATR, Chk1, and ATM expression, as well as the glyceraldehyde-3-phosphate dehydrogenase (GAPDH) control, is also included. D, cisplatin induces phosphorylation of Chk1. Whole-cell lysates were prepared from U-2 OS cells treated with 4 µg/mL cisplatin for the indicated times. Western blot analysis was done using the indicated Chk1 or phosphospecific Chk1 antibodies.

View larger version (45K): [in this window] [in a new window]   Figure 5. Cisplatin induces Thr505 phosphorylation of RelA. A, cisplatin induces Thr505 phosphorylation. Whole-cell lysates were prepared from NARF2 cells either treated with IPTG to induce ARF for 24 hours or nuclear protein extracts were prepared from U-2 OS cells stimulated with 4 µg/mL cisplatin (4 hours), 1 µmol/L daunorubicin (4 hours), or 40 J/m2 UV-C (4 hours) or left untreated. Phosphorylated RelA was then immunopreciptated by incubating 100 µg of lysate with purified rabbit phospho-RelA T505A antibody. The immunoprecipitate was resolved by SDS-PAGE before Western blotting with an anti-RelA antibody (Santa Cruz Biotechnology). B, experiment was done as in (A), except that whole-cell lysates from U-2 OS cells were used in combination with the goat phospho-RelA T505A antibody and anti-RelA antibody (Santa Cruz Biotechnology). Both antibodies were used to either immunoprecipitate or Western blot RelA as indicated. C, cisplatin induced Thr505 phosphorylation is prevented by the Chk1 inhibitor Gö6976. Experiment was done as in (A), except that indicated cells were incubated with 1 µmol/L Gö6976 for 30 minutes before the addition of cisplatin and the preparation of whole-cell lysates. The same result is also seen with the goat phospho-RelA T505 antibody (data not shown).

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

Another implication of our studies concerns the ATR/Chk1 checkpoint kinase pathway. That this pathway seems able to modulate RelA function only in response to certain inducers implies that scaffold or adaptor proteins must exist to target Chk1 to RelA only under certain circumstances. Exactly why this occurs with ARF and cisplatin but not UV-C, daunorubicin/doxorubicin, and etoposide is unclear, but similar adaptor proteins, such as BRCA1 tumor suppressor, are known to target ATR to a subset of its substrates (35). The identity of such Chk1 adaptor proteins will be of great interest. It could be expected that this protein or proteins might also target Chk1 to substrates other than RelA. Moreover, if a consequence of the ARF/cisplatin induced Chk1 adaptor is to neutralize the oncogenic and antiapoptotic functions of RelA, it could well be a tumor suppressor in its own right. Furthermore, it is possible that its presence or deletion in a tumor might act as a diagnostic indicator for NF-B function, as described above.

Although we have focused on Thr⁵⁰⁵ phosphorylation of RelA because this is a modification with proven functional effects (16, 17), it is probable that this is not the only post-translational effect induced by cisplatin treatment. For example, a recent report implied that dephosphorylation of RelA at Thr⁴³⁵ by protein phosphatase 4 in response to cisplatin increases RelA transcriptional activity (36). Thr⁴³⁵ is also located in the RelA transactivation domain and shows some evolutionary conservation. The relative contribution of phosphorylations at 435 and 505 to RelA activity is currently under investigation, but the absence of a Thr⁴³⁵ phosphospecific antibody prevented analysis in this study.

This report adds cisplatin to a group of cancer drugs that have diverse effects on NF-B function. We propose that proapoptotic and antiapoptotic signals converge on RelA in response to a variety of stimuli, and that particular combinations of signals trigger distinct gene expression profiles (18, 30). This complexity of the NF-B response poses challenges to future therapy based on its activity. Nonetheless, it remains highly likely that compounds targeting the NF-B pathway, such as inhibitors of IB kinase, will prove clinically useful in cancer treatment. For example, this will almost certainly be the case where tumors have an inflammatory origin or where the expression of tumor suppressors, such as ARF, has been lost. However, an increased understanding of the mechanisms regulating diverse NF-B function in response to different treatments might help therapies be targeted more effectively. Furthermore, these studies could suggest alternative drug development pathways. Our demonstration that cisplatin essentially mimics the ability of ARF to regulate RelA activity suggests that it should be possible to develop other compounds targeting the same pathway but possibly with increased specificity and reduced toxicity. That a well-known and widely used chemotherapeutic drug seems to have the same mechanism of action on RelA as an important tumor suppressor, underlines the likely clinical importance of this pathway. It will be of interest therefore to determine how widely it becomes activated in response to other therapies and in other biological contexts.

	Acknowledgments

 
Grant support: Royal Society University Fellowship (N.D. Perkins), 4-year Wellcome Trust Ph.D. studentship (K.J. Campbell), Active Motif (K.J. Campbell), and Cancer Research UK programme grant C1443/A5435 (S. Rocha).

The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

We thank all members of the NDP laboratory and the Division of Gene Regulation and Expression at the University of Dundee for their help and assistance and Prof. Philip Cohen for his support.

	Footnotes

 
Note: J. Witty is currently at the Faculty of Life Sciences, The University of Manchester, Michael Smith Building, Oxford Road, Manchester, M13 9PT, United Kingdom.

Received 6/27/05. Revised 11/ 2/05. Accepted 11/ 9/05.

	References

Top Abstract Introduction Materials and Methods Results Discussion References

 

1. Baldwin AS. The transcription factor NF-B and human disease. J Clin Invest 2001;107:3–6.[CrossRef][Medline]
2. Lin A, Karin M. NF-B in cancer: a marked target. Semin Cancer Biol 2003;13:107–14.[CrossRef][Medline]
3. Hayden MS, Ghosh S. Signaling to NF-B. Genes Dev 2004;18:2195–224.[Abstract/Free Full Text]
4. Perkins ND. The Rel/NF-B family: friend and foe. Trends Biochem Sci 2000;25:434–40.[CrossRef][Medline]
5. Greten FR, Eckmann L, Greten TF, et al. IKKß links inflammation and tumorigenesis in a mouse model of colitis-associated cancer. Cell 2004;118:285–96.[CrossRef][Medline]
6. Pikarsky E, Porat RM, Stein I, et al. NF-B functions as a tumour promoter in inflammation-associated cancer. Nature 2004;431:461–6.[CrossRef][Medline]
7. Luo JL, Maeda S, Hsu LC, Yagita H, Karin M. Inhibition of NF-B in cancer cells converts inflammation-induced tumor growth mediated by TNF to TRAIL-mediated tumor regression. Cancer Cell 2004;6:297–305.[CrossRef][Medline]
8. Pahl HL. Activators and target genes of Rel/NF-B transcription factors. Oncogene 1999;18:6853–66.[CrossRef][Medline]
9. Kucharczak J, Simmons MJ, Fan YJ, Gelinas C. To be, or not to be: NF-B is the answer—role of Rel/NF-B in the regulation of apoptosis. Oncogene 2003;22:8961–82.[CrossRef][Medline]
10. Beg AA, Baltimore D. An Essential role for NF-B in preventing TNF--induced cell death. Science 1996;274:782–4.[Abstract/Free Full Text]
11. Baldwin AS. Control of oncogenesis and cancer therapy resistance by the transcription factor NF-B. J Clin Invest 2001;107:241–6.[CrossRef][Medline]
12. Karin M, Yamamoto Y, Wang QM. The IKK NF-B system: a treasure trove for drug development. Nat Rev Drug Discov 2004;3:17–26.[CrossRef][Medline]
13. Haefner B. NF-B: arresting a major culprit in cancer. Drug Discov Today 2002;7:653–63.[CrossRef][Medline]
14. Darnell JE. Transcription factors as targets for cancer therapy. Nat Rev Cancer 2002;2:740–9.[CrossRef][Medline]
15. Campbell KJ, Rocha S, Perkins ND. Active repression of antiapoptotic gene expression by ReIA(p65) NF-B. Mol Cell 2004;13:853–65.[CrossRef][Medline]
16. Rocha S, Campbell KJ, Perkins ND. p53- and Mdm2-independent repression of NF-B transactivation by the ARF tumor suppressor. Mol Cell 2003;12:15–25.[CrossRef][Medline]
17. Rocha S, Garrett MD, Campbell KJ, Schumm K, Perkins ND. Regulation of NF-B and p53 through activation of ATR and Chk1 by the ARF tumour suppressor. EMBO J 2005;24:1157–69.[CrossRef][Medline]
18. Campbell KJ, Perkins ND. Reprogramming RelA. Cell Cycle 2004;3:869–72.[Medline]
19. Perkins ND. NF-B: tumor promoter or suppressor? Trends Cell Biol 2004;14:64–9.[CrossRef][Medline]
20. Siddik ZH. Cisplatin: mode of cytotoxic action and molecular basis of resistance. Oncogene 2003;22:7265–79.[CrossRef][Medline]
21. Souhami RL, Craft AW, Van der Eijken JW, et al. Randomised trial of two regimens of chemotherapy in operable osteosarcoma: a study of the European Osteosarcoma Intergroup. Lancet 1997;350:911–7.[CrossRef][Medline]
22. Stott FJ, Bates S, James MC, et al. The alternative product from the human CDKN2A locus, p14(ARF), participates in a regulatory feedback loop with p53 and MDM2. EMBO J 1998;17:5001–14.[CrossRef][Medline]
23. Anderson LA, Perkins ND. Regulation of RelA (p65) function by the large subunit of replication factor C. Mol Cell Biol 2003;23:721–32.[Abstract/Free Full Text]
24. Park YB, Park MJ, Kimura K, Shimizu K, Lee SH, Yokota J. Alterations in the INK4a/ARF locus and their effects on the growth of human osteosarcoma cell lines. Cancer Genet Cytogenet 2002;133:105–11.[CrossRef][Medline]
25. Yazlovitskaya EM, Persons DL. Inhibition of cisplatin-induced ATR activity and enhanced sensitivity to cisplatin. Anticancer Res 2003;23:2275–9.[Medline]
26. Zhao H, Piwnica-Worms H. ATR-mediated checkpoint pathways regulate phosphorylation and activation of human Chk1. Mol Cell Biol 2001;21:4129–39.[Abstract/Free Full Text]
27. Kohn EA, Yoo CJ, Eastman A. The protein kinase c inhibitor Go6976 is a potent inhibitor of DNA damage-induced S and G(2) cell cycle checkpoints. Cancer Res 2003;63:31–5.[Abstract/Free Full Text]
28. Kawabe T. G₂ checkpoint abrogators as anticancer drugs. Mol Cancer Ther 2004;3:513–9.[Abstract/Free Full Text]
29. Ishimi Y, Komamura-Kohno Y, Kwon HJ, Yamada K, Nakanishi M. Identification of MCM4 as a target of the DNA replication block checkpoint system. J Biol Chem 2003;278:24644–50.[Abstract/Free Full Text]
30. Campbell KJ, Perkins ND. Post-translational modification of RelA(p65) NF-B. Biochem Soc Trans 2004;32:1087–9.[CrossRef][Medline]
31. Piret B, Piette J. Topoisomerase poisons activate the transcription factor NF-B in ACH-2 and CEM cells. Nucleic Acids Res 1996;24:4242–8.[Abstract/Free Full Text]
32. Nie Z, Mei Y, Ford M, et al. Oxidative stress increases A1 adenosine receptor expression by activating nuclear factor B. Mol Pharmacol 1998;53:663–9.[Abstract/Free Full Text]
33. Kim JS, Lee JM, Chwae YJ, et al. Cisplatin-induced apoptosis in Hep3B cells: mitochondria-dependent and -independent pathways. Biochem Pharmacol 2004;67:1459–68.[CrossRef][Medline]
34. Mabuchi S, Ohmichi M, Nishio Y, et al. Inhibition of NFB increases the efficacy of cisplatin in in vitro and in vivo ovarian cancer models. J Biol Chem 2004;279:23477–85.[Abstract/Free Full Text]
35. Foray N, Marot D, Gabriel A, et al. A subset of ATM- and ATR-dependent phosphorylation events requires the BRCA1 protein. EMBO J 2003;22:2860–71.[CrossRef][Medline]
36. Yeh PY, Yeh KH, Chuang SE, Song YC, Cheng AL. Suppression of MEK/ERK signaling pathway enhances cisplatin-induced NF-B activation by protein phosphatase 4-mediated NF-B p65 Thr dephosphorylation. J Biol Chem 2004;279:26143–8.[Abstract/Free Full Text]

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