Phosphorylation of IκBα at Serine 32 by T-lymphokine-activated Killer Cell-originated Protein Kinase Is Essential for Chemoresistance against Doxorubicin in Cervical Cancer Cells*

Background: The regulatory mechanism of TOPK underlying cancer cell survival remains unknown. Results: TOPK directly interacts with and phosphorylates IκBα at Ser-32. Conclusion: TOPK is a critical mediator of cervical cancer chemoresistance in response to doxorubicin. Significance: This study provides new insight on role of TOPK in cervical cancer cell survival in response to doxorubicin. T-lymphokine-activated killer cell-originated protein kinase (TOPK) is known to be up-regulated in cancer cells and appears to contribute to cancer cell proliferation and survival. However, the molecular mechanism by which TOPK regulates cancer cell survival still remains elusive. Here we show that TOPK directly interacted with and phosphorylated IκBα at Ser-32, leading to p65 nuclear translocation and NF-κB activation. We also revealed that doxorubicin promoted the interaction between nonphosphorylated or phosphorylated TOPK and IκBα and that TOPK-mediated IκBα phosphorylation was enhanced in response to doxorubicin. Also, exogenously overexpressed TOPK augmented transcriptional activity driven by either NF-κB or inhibitor of apoptosis protein 2 (cIAP2) promoters. On the other hand, NF-κB activity including IκBα phosphorylation and p65 nuclear translocation, as well as cIAP2 gene expression, was markedly diminished in TOPK knockdown HeLa cervical cancer cells. Moreover, doxorubicin-mediated apoptosis was noticeably increased in TOPK knockdown HeLa cells, compared with control cells, which resulted from caspase-dependent signaling pathways. These results demonstrate that TOPK is a molecular target of doxorubicin and mediates doxorubicin chemoresistance of HeLa cells, suggesting a novel mechanism for TOPK barrier of doxorubicin-mediated cervical cancer cell apoptosis.


T-lymphokine-activated killer cell-originated protein kinase (TOPK) is known to be up-regulated in cancer cells and appears
to contribute to cancer cell proliferation and survival. However, the molecular mechanism by which TOPK regulates cancer cell survival still remains elusive. Here we show that TOPK directly interacted with and phosphorylated IB␣ at Ser-32, leading to p65 nuclear translocation and NF-B activation. We also revealed that doxorubicin promoted the interaction between nonphosphorylated or phosphorylated TOPK and IB␣ and that TOPK-mediated IB␣ phosphorylation was enhanced in response to doxorubicin. Also, exogenously overexpressed TOPK augmented transcriptional activity driven by either NF-B or inhibitor of apoptosis protein 2 (cIAP2) promoters. On the other hand, NF-B activity including IB␣ phosphorylation and p65 nuclear translocation, as well as cIAP2 gene expression, was markedly diminished in TOPK knockdown HeLa cervical cancer cells. Moreover, doxorubicin-mediated apoptosis was noticeably increased in TOPK knockdown HeLa cells, compared with control cells, which resulted from caspasedependent signaling pathways. These results demonstrate that TOPK is a molecular target of doxorubicin and mediates doxorubicin chemoresistance of HeLa cells, suggesting a novel mechanism for TOPK barrier of doxorubicin-mediated cervical cancer cell apoptosis.
Doxorubicin, anthracycline antibiotic, is known to function as a potent chemotherapeutic agent against solid tumors and malignant hematological diseases (1,2). Doxorubicin acts as DNA intercalating agent, causing dysfunction of DNA topoi-somerase II and double-stranded DNA break, and elicits its inhibitory activity on tumors (3). This doxorubicin-induced DNA damage leads to target cell death. In parallel, DNA damage results in NF-B activation to enhance transcription of NF-B-driven genes, which are involved in cell proliferation and survival (4). In an unstimulated state, NF-B is sequestered in the cytoplasm by binding to IB. In response to doxorubicin, IB kinases (IKKs) 3 complex comprised of IKK␣, IKK␤, and NEMO is activated, and phosphorylates IB, which is sequentially ubiquitinated and subjected to proteasomal degradation (5). NF-B is then released from IB, and activated NF-B enters into nucleus and induces target gene transcription. Previous studies show that doxorubicin-induced apoptosis is triggered by cascades of caspase activation (6,7). NF-B is shown to play an important role in maintaining resistance to doxorubicin-induced tumor cells apoptosis and to contribute to prevention of efficacy of cancer therapeutics (8,9). Indeed, inhibition of NF-B sensitizes tumor cells to apoptosis in response to doxorubicin (10,11).
T-LAK-cell-originated protein kinase (TOPK) is known to be a serine/threonine kinase that is highly expressed in various malignant cells such as Burkitt's lymphoma and hematopoietic neoplasms or in normal tissues including testis, kidney, lung, placenta, and embryonic tissues (12)(13)(14)(15)(16). It has been proposed that TOPK, MAPKK-like protein kinase, acts as an upstream kinase for p38 MAPK, phosphatase MKP1, and peroxiredoxin 1 (12,17,18). In addition, TOPK phosphorylates JNK1 in UVBmediated signaling or Ras-induced cell transformation and positively regulates ERK2 during tumorigenesis (19,20). The cyclin B1/Cdk1 binds and phosphorylates TOPK on residue Thr-9 during mitosis, leading to enhancement of cytokinesis through PRC1 phosphorylation (13,21). It was reported that TOPK associates with p53 and suppresses its transcriptional activity, resulting in reduction of p21 expression (22 ously, we showed that TOPK confers TRAIL resistance to cancer cells (23). These reports suggest a role for TOPK in cancer cell proliferation and survival. However, little is known about mechanisms regarding the role of TOPK in cancer cell survival against cancer chemotherapy drugs involving doxorubicin.
Here we reveal that TOPK is a novel target molecule in response to doxorubicin and that TOPK directly interacts with and phosphorylates IB␣ at Ser-32, leading to subsequent NF-B activation. We also demonstrate that depletion of endogenous TOPK abrogated doxorubicin-induced IB␣ phosphorylation or p65 nuclear translocation. We provide evidence that overexpressed TOPK up-regulated expression of cIAP2 gene, one of the NF-B-dependent antiapoptotic genes, and conferred resistance to doxorubicin-induced HeLa cervical cancer cell death.
Plasmids and Transfection-Plasmid V5-TOPK was constructed. Briefly, total RNA from HeLa cell was extracted, and cDNA was prepared using Superscript III reverse transcriptase (Invitrogen). Sequentially, PCR was performed with the cDNA using sense strand, 5Ј-CGCGGATCCCGATGGAAGGGATC-AGTAATTT-3Ј harboring the BamHI site and antisense strand 5Ј-CCGCTCGAGCGGGACATCTGTTTCCAGAG-CTT-3Ј harboring the XhoI site, and the PCR product cut with BamHI/XhoI was inserted into the BamHI/XhoI sites of pcDNA6/V5-His A (Invitrogen). The construct was verified by sequencing. Plasmids, cIAP2 promoter-driven luciferase reporter vectors, wild type, and NF-B mutants, were kindly provided by Dr. Hinrich Gronemeyer (24). GFP-p65/RelA construct was a kind gift from Dr. Warner C. Greene (25). NF-Bdependent luciferase vector and TOPK siRNA construct were as described previously (23). 293 or HeLa cells growing on a 100-mm dish was transfected with each 10 g of plasmids using Effectene according to the manufacturer's instructions. 24 h after transfection, the cells were lysed, and cell lysate was subjected to immunoblot or immunoprecipitation.
In Vitro Kinase Assay-In vitro kinase assay was performed with active or inactive TOPK and GST-IB␣ protein. Briefly, the reactions containing 100 M were done at 30°C for 30 min. The samples were subjected to 10% SDS-PAGE and visualized by immunoblot. For TOPK immunoprecipitation kinase assay, 293 cells were transfected with V5-TOPK construct, treated with doxorubicin, and lysed. Cell lysate was immunoprecipitated with V5 antibody. The precipitates were reacted with GST-IB␣ and analyzed with immunoblot using phospho-IB␣ (Ser-32) antibody.
Immunoblot and Immunoprecipitation-For immunoblot analysis, 20 g of each total cell lysate was resolved by SDS-PAGE, probed using each respective antibody, and detected with SuperSignal West Pico chemiluminescent substrate (Pierce) and x-ray film. For immunoprecipitation, 500 g of total cell lysate was mixed with specific antibody and then protein agarose beads at 4°C for 2 h using rocker. The beads were washed, subjected to 10% SDS-PAGE, and then subjected to immunoblot.
GST Pulldown Assay-To investigate the interaction of TOPK and IB␣, GST pulldown assay was performed with GST-IB␣. 293 cells were expressed with V5-TOPK construct, harvested 24 h after transfection, and lysed. 500 g of total cell lysate was incubated with 2 g of GST-IB␣ protein coupled to glutathione-Sepharose 4B at 4°C for 2 h. The beads were washed with lysis buffer, boiled with sample buffer, separated on 10% SDS-PAGE, and then analyzed with immunoblot using V5 antibody.
Luciferase Assay-For luciferase assay, CHO-K1 cells growing on 6-well plates were transfected with each 1 g of NF-B promoter or cIAP2 promoter-luciferase reporter construct, plus 0.5 g of the pRL-SV40 gene using 4 l of Effectene reagent. 24 h after transfection, the cells were treated with doxorubicin for 24 h, harvested, and then lysed. Firefly and Renilla luciferase activities were measured using cell lysate.
GFP-RelA Localization-Control siRNA cells or HeLa-TOPK siRNA cells were seeded on cover glass in 6-well plates and transfected with 0.5 g of GFP-RelA construct. The cells were stimulated with doxorubicin for 6 h. The cells were observed under a fluorescent microscope to determine expression and localization of GFP-RelA.
Terminal Deoxynucleotidyl TUNEL Assay-TUNEL assay was performed using the DeadEnd fluorometric TUNEL sys-tem (Promega) according to the manufacturer's instruction. Control siRNA cells or HeLa-TOPK siRNA cells were treated with doxorubicin for 24 h, fixed with 4% methanol-free formaldehyde, and permeabilized with Triton X-100. Terminal deoxynucleotidyltransferase and nucleotide mixture including fluorescein-dUTP were used for labeling DNA breaks. After incubation, the cells were washed and mounted. The cells were observed and analyzed under a fluorescence microscope.
Statistical Analysis-The results are shown as the means Ϯ S.D. for at least three independent experiments in duplicate. Significant differences were evaluated by Student's t test. Each cell lysate (500 g) was immunoprecipitated (IP) with TOPK antibody (1 g) and followed by immunoblotting (IB) using phosphoserine/ threonine (p-Ser/Thr) antibody. Phosphorylation of the indicated proteins was detected with the respective phospho-specific antibodies. B, 293 cells grown on 100-mm dishes were transfected with each 10 g of empty vector or V5-TOPK construct. At 24 h after transfection, the cells were treated with doxorubicin (1 M) for each indicated time. Each cell lysate (500 g) was subjected to immunoprecipitation using IB␣ antibody (1 g) and then analyzed by immunoblot using V5 antibody. Expression of V5-TOPK was verified. C, each 10 g of empty vector or V5-TOPK construct was expressed in 293 cells, and the GST pulldown experiment was done using cell lysate (500 g) and GST-IB␣ (2 g) coupled to glutathione-Sepharose beads. The beads were subjected to 10% SDS-PAGE and then probed with V5 antibody. D, HeLa cells were treated with 1 M of doxorubicin for the indicated times. Immunoprecipitation was done with IB␣ antibody (Sepharose bead conjugate), followed by immunoblot using TOPK or IB␣ antibody. E, each 10 g of V5-TOPK construct was expressed in 293 cells. The cells were treated with doxorubicin (1 M) for each indicated time. Each cell lysate (500 g) was immunoprecipitated using IB␣ antibody (Sepharose bead conjugate) and then probed with phospho-TOPK (Thr-9) antibody.

Doxorubicin Activates TOPK and Promotes
stimuli. Doxorubicin commonly used in cancer treatment is known to induce genotoxic stress and p53 activation (26). However, the molecular targets of doxorubicin are poorly characterized. We have explored whether doxorubicin can affect TOPK activity or expression. To investigate whether doxorubicin might affect TOPK activity, we first treated human cervical HeLa cancer cells with doxorubicin in time-dependent manner.
The results showed that doxorubicin strongly induced phosphorylation of Ser/Thr residues on TOPK, indicating the efficacy of doxorubicin on catalytic activity of TOPK (Fig. 1A). TOPK expression was slightly affected by doxorubicin treatment. We next examined the change of phosphorylation level of IB␣ or AKT that is involved in cancer cell survival. Phosphorylation level of IB␣ or AKT was augmented at 1 or 2 h after doxorubicin treatment. These results suggest that TOPK might be one of the molecular targets of doxorubicin and that doxorubicin-induced TOPK activity might be implicated in IB␣ phosphorylation. We next hypothesized that TOPK could associate with and regulate IB␣ phosphorylation status. To examine the possibility for binding of TOPK to IB␣, we transfected V5-TOPK into HEK293 cells, left them in the absence or presence of doxorubicin, and then performed immunoprecipitation experiments. We discovered that TOPK directly bound to IB␣ in vivo, and doxorubicin markedly enhanced the binding capacity (Fig. 1B). To further verify that TOPK interacts with IB␣ in vitro, GST pulldown assays were also carried out. GST-IB␣ coupled to glutathione-Sepharose beads was incubated with cell lysate expressing V5-TOPK construct. The results indicated that TOPK bound to IB␣ in vitro, proving a direct interaction between TOPK and IB␣ (Fig. 1C). Furthermore, we verified that endogenous TOPK associated with IB␣, and the interaction was significantly potentiated by doxorubicin treatment (Fig. 1D). To ensure that phosphorylated TOPK is indeed active form of TOPK, we also explored whether phosphorylated TOPK interacts with IB␣. The phosphorylated TOPK at Thr-9 was shown to bind to IB␣ (Fig. 1E). The binding was markedly increased in response to doxorubicin. Collectively, these findings demonstrated that TOPK interacts with IB␣ and that doxorubicin induces TOPK phosphorylation and promotes association of phosphorylated TOPK with IB␣, probably affecting IB␣ phosphorylation. TOPK Directly Phosphorylates IB␣, and Doxorubicin Enhances Its Kinase Activity-We next examined whether TOPK could phosphorylates IB␣. The active form of TOPK, a constitutively phosphorylated TOPK at Thr-9, was employed for kinase assay. Kinase assay using active TOPK and GST-IB␣ was performed in vitro. The results revealed that active TOPK phosphorylated residue Ser-32 on IB␣ in dose-dependent manner ( Fig. 2A). As expected, inactive TOPK did not exert the kinase activity against IB␣ (Fig. 2B). We also investigated whether doxorubicin affects TOPK-induced IB␣ phosphorylation in vivo. V5-TOPK construct was expressed in HEK293 cells, followed by immunoprecipitation kinase assay. We confirmed that doxorubicin strongly induces TOPK-mediated phosphorylation of IB␣ (Ser-32) in a time-dependent manner (Fig. 2C). These results suggest that TOPK associates with and directly phosphorylates IB␣ to elicit NF-B activity.

TOPK Positively Regulates NF-B-driven Transcriptional Activity and cIAP2 Gene Expression in Response to Doxorubicin-
Doxorubicin has been reported to induce NF-B activation in apoptosis process (27). We asked whether TOPK can be involved in doxorubicin-induced NF-B-responsive transcriptional activity. CHO-K1 cells were transfected with NF-B promoter-driven luciferase reporter construct without or with the V5-TOPK construct and then left in absence or presence of doxorubicin. As expected, NF-B promoter-driven transcriptional activity was augmented by doxorubicin treatment (Fig.  3A). Also, expression of TOPK alone increased the transcriptional activity in dose-dependent manner. Moreover, doxorubicin-induced NF-B activity was markedly increased by TOPK expression. We next employed the promoter of the cIAP2 gene, one of NF-B responsive genes, which is linked to luciferase reporter gene. Using promoters of wild type or NF-B cis-element mutant types of cIAP2, transcriptional activities were assessed. As shown in Fig. 3B, TOPK expression resulted in an increase of cIAP2 promoter-driven luciferase activity induced by doxorubicin, whereas the activity was greatly reduced in cIAP2 promoters having a mutation on NF-B cis-element. It appeared that cIAP2 promoter (Ϫ39 mut) having a mutation of a NF-B site (Ϫ39) elicited a little differential responsiveness compared with another cIAP2 promoter (ϩ102 mut), indicating site-specific selectivity of NF-B response. We have previously established HeLa-TOPK siRNA knockdown cell lines (23). Using a reverse transcription-PCR experiment, we next investigated whether TOPK affects expression of cIAP2 gene in response to doxorubicin. Doxorubicin strongly induced expression of cIAP2 gene in control cells (Fig. 3C). In contrast, the doxorubicin-induced cIAP2 gene expression was dramatically diminished in TOPK siRNA cells. As expected, doxorubicin treatment also increased the expression of TOPK gene. Taken together, these findings demonstrate that TOPK up-regulates NF-B activity and cIAP2 expression in response to doxorubicin, implying the role of TOPK in doxorubicin-mediated apoptotic signaling.
Depletion of TOPK Abolishes Doxorubicin-mediated IB␣ Phosphorylation and p65 Nuclear Translocation-Doxorubicin has been suggested to induce IB phosphorylation and p65 nuclear translocation (28). To clarify the effect of TOPK on doxorubicin-mediated IB␣ degradation or phosphorylation, we employed HeLa-TOPK siRNA knockdown cell lines. As expected, the phosphorylation level of IB␣ in HeLa cells expressing control siRNA was markedly augmented in response to doxorubicin treatment, whereas the level was little changed in TOPK siRNA cells (Fig. 4A). We also determined the effect of wedelolactone, the irreversible inhibitor of IKK␣ and IKK␤, on doxorubicin-induced IB␣ phosphorylation. Wedelolactone little affected the doxorubicin-induced IB␣ phosphorylation. These data imply that TOPK-mediated IB␣ phosphorylation in response to doxorubicin might be independent on IKKs. In response to various stimuli including doxorubicin, p65/RelA nuclear translocation is essential for NF-B activation. The cells were transfected with GFP-RelA construct, treated with doxorubicin, and then analyzed by fluorescence microscopy. In control siRNA cells, RelA was shown to be successfully translocated to the nucleus in response to doxorubicin (Fig. 4B). In contrast, RelA failed to displace from the cytoplasm to the nucleus in TOPK siRNA cells by doxorubicin. Also, the level of RelA protein in the cytoplasm or nucleus was assessed. Nuclear RelA was markedly increased in response to doxorubicin in control siRNA cells (Fig. 4C), whereas the nuclear RelA was a little increased in TOPK siRNA cells. On the other hand, the basal level of nuclear RelA in the absence of doxorubicin is decreased in TOPK siRNA cells, compared with control siRNA cells, suggesting TOPK-mediated basal regulation of nuclear p65 expression. Collectively, these findings propose that TOPK mediates IB␣ phosphorylation and subsequent RelA nuclear translocation in Luciferase activity was evaluated. *, p Ͻ 0.01; **, p Ͻ 0.05. C, total RNAs were prepared from HeLa-TOPK siRNA or control siRNA cells stimulated with doxorubicin (1 M). RT-PCR was sequentially performed using SuperScript III reverse transcriptase and each primer for cIAP2 or GAPDH genes. PCR products were resolved on a 1.5% agarose gel and analyzed using GelDoc (Bio-Rad).

TOPK in Chemoresistance to Doxorubicin-mediated Apoptosis
FEBRUARY 1, 2013 • VOLUME 288 • NUMBER 5 response to doxorubicin, as well as regulation of basal expression of nuclear p65. TOPK Confers Resistance to Doxorubicin-induced HeLa Cancer Cell Apoptosis-We next asked that TOPK might contribute to HeLa cervical cancer cell chemoresistance in response to doxorubicin. Therefore, we explored the effect of knocking down TOPK on doxorubicin-induced cell death. The doxorubicin-induced apoptosis rate in control siRNA cells was reduced ϳ29%, compared with the rate in HeLa-TOPK siRNA cells (Fig. 5A). To examine whether endogenous TOPK affected doxorubicin-mediated caspases activation leading to PARP cleavage, activation of caspase 3 or caspase 8, as well as PARP were examined in TOPK siRNA or control siRNA cells. Cleaved forms of caspase 3 or caspase 8 were more increased by doxorubicin treatment in TOPK siRNA cells than control siRNA cells (Fig. 5B). Also, cleaved forms of PARP were more increased in TOPK siRNA cells. These results demonstrate that endogenous TOPK alleviates doxorubicin-induced caspase 8 and caspase 3 activation, leading to PARP inactivation, suggesting the role of TOPK in doxorubicin-induced HeLa cancer cells apoptosis. To ensure that doxorubicin-induced apoptosis in HeLa-TOPK siRNA cells is mediated via caspase activation pathway, two inhibitors, general caspase inhibitor Z-VAD-FMK, and caspase 8 inhibitor Z-IETD-FMK, were employed. As expected, cleaved forms of PARP were decreased in the presence of each inhibitor, together with doxorubicin (Fig. 5C). These data show that doxorubicin-induced apoptosis in TOPK siRNA cells is mediated via caspase activation pathway. On the other hand, MAPK signaling pathways including ERK, p38, and JNK have been suggested to be implicated in doxorubicin-induced cancer cells apoptosis (29,30). Therefore, we next asked whether MAPK pathways are involved in doxorubicin-induced apoptosis in HeLa-TOPK siRNA cells. Using specific inhibitors, such as MEK1/2 inhibitor U0126, p38 MAPK inhibitor SB202190, and JNK inhibitor SP600125, the effect of doxorubicin on PARP cleavage in TOPK siRNA cells was determined. Treatment of SP600125, but not U0126 and SB202190, blocked doxorubicin-induced PARP cleavage (Fig. 5D). These results indicate that JNK might play an important role in doxorubicininduced HeLa cells, especially TOPK-depleted cell killing.

DISCUSSION
It has been suggested that some stimuli including TPA or UVB positively regulate TOPK activity (12,17,19). However, information about signaling pathways or stimuli triggering TOPK activation is still lacking. In this study, we uncovered that doxorubicin, one of the anticancer drugs, could phosphorylate serine or threonine residues on TOPK and increases TOPK mRNA level, indicating the effect of doxorubicin on TOPK catalytic activity and TOPK gene expression. Although the action mechanism of doxorubicin in cancer cell apoptosis is known, the molecular targets of doxorubicin are poorly identified. We demonstrate here that TOPK functions as a novel target molecule of doxorubicin, implying a critical role for TOPK in doxorubicin-induced cervical cancer cell death. Some molecules, such as p38 MAPK, JNK, phosphatase MKP1, and peroxiredoxin 1, have been proposed to act as downstream substrates for TOPK (12,(17)(18)(19). However, evidence for downstream targets of TOPK still remains elusive. We identified that TOPK directly binds to IB␣ and phosphorylates serine-32 residue on IB␣ in response to doxorubicin leading to NF-B activation. These data define TOPK as an upstream kinase of IB␣ regu- lating NF-B activity with a possible role in doxorubicin-mediated cervical cancer cell apoptosis. It has been suggested that NF-B contributes to chemoresistance to anticancer drugs and is triggered by genotoxic agents including doxorubicin, which limits the chemotherapeutics-mediated anticancer effects (31). Also, NF-B activation is known to result in induction of survival factors, Bcl-2 or IAPs (32). Therapeutic approaches to overcome NF-B-mediated chemoresistance are closely implicated in induction of IB overexpression or IB stabilization via proteasome inhibition preventing IB degradation (33,34). In this study, endogenously overexpressed TOPK was shown to increase doxorubicin-mediated NF-B-driven transcriptional activity in HeLa cervical cancer cells. The findings that TOPK activates NF-B in response to doxorubicin revealed the role of TOPK as a critical mediator in cervical cancer cell survival. A previous report proposed that NF-B activity induced by ultraviolet radiation or chemotherapeutic agent-induced DNA damage might promote U2OS osteosarcoma cell death, associated with interaction of p65 and histone deacetylases (35). A recent study also showed that doxorubicin increased transcription of the cIAP2 gene, an antiapoptotic gene, but repressed expression of Bcl-xL, XIAP, Bcl-2, or survivin gene in U2OS osteosarcoma cells and that NF-B inhibition prevented doxorubicin-mediated transcription of cIAP2, leading to enhanced cell death (27). Agreeing with this result, we indicated that expression of cIAP2 gene is increased in HeLa cervical cancer cells by doxorubicin treatment, but TOPK depletion abolishes this augmentation via NF-B inhibition. These findings suggest that doxorubicin-mediated increment of cIAP2 gene transcripts might be dependent on endogenous TOPK expression and that the reduction of cIAP2 via NF-B inhibition promotes cervical cancer cell death. It has been proposed that some MAPKs or their related signaling pathways are implicated in chemotherapeutics-mediated apoptosis (36 -38). JNK activity is especially closely involved in apoptosis in response to chemotherapeutic agents involving doxorubicin (7,30,39), which results in release of mitochondrial cytochrome c and second mitochondria-derived activator of caspase to cytoplasm, leading to caspase activation. Procaspase-9 is recruited and activated with subsequent activation of the downstream effector caspase-3 and PARP (40). Inhibition of JNK, but not ERK and p38 MAPK, markedly prevents doxorubicin-mediated apoptosis of TOPK-depleted HeLa cervical cancer cells. This finding suggests that JNK activity is essential for apoptosis to doxorubicin in cervical cancer cell lacking endogenous TOPK. Therefore, an approach to efficient doxorubicin-mediated chemotherapy for cervical cancers might include in part JNK activation, as well as blockage of TOPK expression or activity. Taken together, this study demonstrates that doxorubicin activates TOPK interaction with IB␣ and promotes its kinase activity against IB␣ at Ser-32, leading to NF-B activation. Also, we provide evidence that TOPK augments expression of cIAP2, acting as a key survival mediator in doxorubicinmediated apoptotic pathway, conferring resistance to doxorubicin-induced HeLa cervical cancer cell death. We here suggest that TOPK is a critical mediator of cervical cancer chemoresistance in response to doxorubicin. Therefore, approaches to inhibit TOPK through blocking its expression or its kinase activity via development of pharmacologic inhibitor might be valuable for further investigation involving mechanistic research to overcome cervical cancer chemoresistance and enhance chemosensitization.