Nucleic Acids Research

Nucleic Acids Research Advance Access published online on November 29, 2008
Nucleic Acids Research, doi:10.1093/nar/gkn934

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© 2008 The Author(s)
This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/2.0/uk/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

Nucleic Acid Enzymes

Casein kinase I / phosphorylates topoisomerase II at serine-1106 and modulates DNA cleavage activity

Adrian G. Grozav¹, Kenichi Chikamori¹, Toshiyuki Kozuki¹, Dale R. Grabowski¹, Ronald M. Bukowski¹, Belinda Willard², Michael Kinter², Anni H. Andersen³, Ram Ganapathi¹ and Mahrukh K. Ganapathi^1,*

¹Clinical Pharmacology Program, Taussig Cancer Institute, ²Lerner Research Institute, Department of Cell Biology, Cleveland Clinic Foundation, Cleveland, OH 44195, USA and ³Department of Molecular Biology, Aarhus University, Aarhus, Denmark

*To whom correspondence should be addressed. Tel: +1 216 445 8416; Fax: +1 216 444 7115; Email: ganapam{at}ccf.org

Received September 12, 2008. Revised November 4, 2008. Accepted November 5, 2008.

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION FUNDING REFERENCES

 
We previously reported that phosphorylation of topoisomerase (topo) II at serine-1106 (Ser-1106) regulates enzyme activity and sensitivity to topo II-targeted drugs. In this study we demonstrate that phosphorylation of Ser-1106, which is flanked by acidic amino acids, is regulated in vivo by casein kinase (CK) I and/or CKI, but not by CKII. The CKI inhibitors, CKI-7 and IC261, reduced Ser-1106 phosphorylation and decreased formation of etoposide-stabilized topo II–DNA cleavable complex. In contrast, the CKII inhibitor, 5,6-dichlorobenzimidazole riboside, did not affect etoposide-stabilized topo II–DNA cleavable complex formation. Since, IC261 specifically targets the Ca²⁺-regulated isozymes, CKI and CKI, we examined the effect of down-regulating these enzymes on Ser-1106 phosphorylation. Down-regulation of these isozymes with targeted si-RNAs led to hypophosphorylation of the Ser-1106 containing peptide. However, si-RNA-mediated down-regulation of CKII and ' did not alter Ser-1106 phosphorylation. Furthermore, reduced phosphorylation of Ser-1106, observed in HRR25 (CKI/ homologous gene)-deleted Saccharomyces cerevisiae cells transformed with human topo II, was enhanced following expression of human CKI. Down-regulation of CKI and CKI also led to reduced formation of etoposide stabilized topo II–DNA cleavable complex. These results provide strong support for an essential role of CKI/ in phosphorylating Ser-1106 in human topo II and in regulating enzyme function.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION FUNDING REFERENCES

 
Type II DNA topoisomerases, topoisomerase II (topo II) and β, regulate DNA topology by creating transient double stranded DNA breaks (1–3). Although, both enzymes exhibit significant sequence homology and catalyze redundant catalytic reactions, they are involved in different cellular functions. This difference may in part be due to differential regulation of these enzymes. Several different mechanisms have been shown to regulate topo II activity, including transcriptional, translational, as well as post-translational mechanisms. The major post-translational mechanisms that modulate topo II activity are phosphorylation, interaction with other proteins and proteasome-mediated degradation (1–3).

Both topo II and topo IIβ are phosphorylated at several sites, primarily in the divergent C-terminal region (4–8). Whereas, little is known about site-specific phosphorylation of topo IIβ, several in vitro and in vivo studies have identified specific phosphorylation sites in topo II. Within the C-terminal region of topo II phosphorylation of threonine-1342, serine(Ser)-1376, Ser-1469 and Ser-1524 catalyzed by casein kinase (CK) II (6,9–14), and of Ser-1212, Ser-1246, Ser-1353, Ser-1360 and Ser-1392 catalyzed by a proline directed kinase has been observed (15). Recently, it has been reported that Polo-like kinase 1 phosphorylates topo II at Ser-1337 and Ser-1524 (16). In addition to the sites in the C-terminal region, phosphorylation of Ser-29 located in the ATP binding domain within the N-terminal region (17) and of Ser-1106 located within the catalytic core have also been reported (18). Whereas phosphorylation of Ser-29 is catalyzed by protein kinase C (17), the kinase responsible for phosphorylation of Ser-1106 has not yet been identified.

Since Ser-1106 is located in the catalytic domain of topo II and phosphorylation of this site enhances enzyme activity and sensitivity to topo II-targeted drugs in vivo (18), it is important to decipher the mechanism by which phosphorylation of Ser-1106 is regulated. The first step toward determining this mechanism would be to identify the kinase(s) that catalyzes phosphorylation at this site. Based on the acidic amino acid sequences that flank Ser-1106 at the amino- and carboxy-terminus, two potential kinases that could phosphorylate this site are CKI and CKII (19). Although CKII has been recognized as a major kinase phosphorylating topo II, the role of CKI in phosphorylating topo II has not been explored. Unlike CKII, which consists of a tetramer of two catalytic subunits, and/or ', and two regulatory β subunits (20–22), human CKI comprises of a superfamily of seven different isozymes that function as monomers (23,24). Structurally these isozymes, CKI, β, 1, 2, 3, and , are organized into three distinct regions – a short N-terminal region, a highly conserved kinase domain and a highly variable C-terminal domain, primarily involved in regulating enzyme function. The CKI and CKI isozymes are very similar in structure and exhibit 98% homology in the kinase domain and 50% homology in the C-terminal domain. Autophosphorylation of the C-terminal domain leads to inhibition of the enzyme, which can be relieved following dephosphorylation or proteolytic cleavage of this region, often via a Ca²⁺-dependent mechanism (25,26). Indeed, it has been suggested that dephosphorylation of CKI by the Ca²⁺/calmodulin-dependent phosphatase, calcineurin, enhances phosphorylation of DARP-32 by this isozyme (27,28).

Our earlier studies demonstrating a Ca²⁺-dependent mechanism in regulating phosphorylation of Ser-1106 and in modulating sensitivity to topo II-targeted drugs (18) suggested that the kinase responsible for phosphorylating this site may be CKI and/or CKI, rather than CKII. In this study we examined the role of CKI/ and CKII in phosphorylating Ser-1106 by attenuating the activity of these kinases with specific inhibitors or with targeted si-RNAs. Our results demonstrated that CKI/, but not CKII, catalyzes the in vivo phosphorylation of Ser-1106 and regulates topo II–DNA cleavage activity.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION FUNDING REFERENCES

 
Reagents
CKI-7 was obtained from Seikagaku Kogyo, Tokyo. IC261 was kindly provided by ICOS Corp., Bothell, WA and 5,6-dichlorobenzimidazole riboside (DRB) was purchased from Calbiochem, La Jolla, CA, USA. Etoposide was purchased from Sigma-Aldrich, St Louis, MO, USA. Stock solutions of these compounds were made in dimethyl sulfoxide and stored at –20^°C. The rabbit polyclonal antibody to topo II was a gift from Dr Ian Hickson, ICRF, Oxford, UK. Mouse monoclonal antibodies to CKI and CKI were obtained from ICOS Corp., Bothell, WA (generous gift from Dr Anthony DiMaggio) and BD Biosciences, San Jose, CA, USA respectively. Goat polyclonal antibodies to CKII and CKII' were obtained from Santa Cruz Biotechnology, Santa Cruz, CA, USA.

Cell culture
HL-60 cells were maintained in RPMI 1640 supplemented with 10% fetal bovine serum and 2 mM glutamine at 37^°C in a humidified atmosphere of 5% CO₂ and 95% air. HCT-116 cells, obtained from Dr Bert Vogelstein, Johns Hopkins University, Baltimore, MD, were maintained in McCoy's 5A medium supplemented with 10% fetal bovine serum and 2 mM glutamine at 37^°C in a humidified atmosphere of 5% CO₂ and 95% air. Cells were treated with CKI-7 (200 µM), IC261 (10 µM) or DRB (40 µM) for 3 h. When the combination of CKI or CKII inhibitor and etoposide was employed, cells were pretreated with CKI-7, IC261 or DRB for 3 h. Following this treatment, cells were washed, resuspended in inhibitor-free medium and incubated for an additional hour in etoposide.

Transfection with targeted si-RNAs
A 21-nucleotide duplex si-RNA (si-CKI/) with the sequence sense: 5'-CUGGGGAAGAAGGGCAACCdTdT-3' and antisense: 5'-GGUUGCCCUUCUUCCCCAGdTdT-3', purchased from Qiagen, Valencia, CA, USA was used to target identical regions in CKI and CKI (29). In addition the On-Target plus SMART pool si-RNA anti-CSNKID human (si-CKI) and On-Target plus SMART pool si-RNA anti-CSNKIE human (si-CKI) were purchased from Dharmacon, Lafayette, CO. For targeting CKII RNA the siGENOM SMART pool CSNK2A1 (Dharmacon, Lafayette, CO) was employed. The CKII' si-RNA (sense: 5'-CAGUCUGAGGAGCCGCGAGdTdT-3', antisense: 5'-CGGCUCCUCAGACUGdTdT-3'), previously described (30) was synthesized by MWG Biotech, Ebersberg, Germany. The control si-RNA (5'-GCUCAGAUCAAUACGGAGAdT dT-3') was purchased from Dharmacon, Lafayette, CO. HCT-116 cells were incubated in serum-free McCoy's medium for 6–10 h with the si-RNA (100 nM) in the presence of Lipofectamine 2000 (Invitrogen Life Technology, Carlsbad, CA) as described by the manufacturer. When the combination of si-CKI and si-CKI was employed, the concentration of each si-RNA was reduced to 75 nM. Following the initial incubation, cells were washed and cultured in McCoy's medium containing 10% fetal bovine serum and 2 mM L-glutamine for 24 h. At the end of the incubation period, cells were harvested for preparing cell lysates. When cells were transfected with si-CKI/ about 50–70% of the cells that readily detached upon washing were used for preparing lysates for 2D-phosphopeptide maps of topo II, since both CKI and CKI were maximally down-regulated in this population.

Transformation of Sachharomyces cerevisiae W303 cells
The wild-type (WT) S. cerevisiae W303 strain (ura3-1, trp1-1, leu 2-3, 112, his3-11, 15 can1-100, ade2-1) and 7D, an HRR25 isolate isogenic to W303 (31) kindly provided by Dr Anthony DeMaggio (ICOS, Corp., Bothell, WA) were transformed with human topo II cDNA cloned in the pHT212 vector using the Yeastmaker lithium acetate transformation system (Clontech, Palo Alto, CA). Control transformations were carried out with the pHT212 plasmid (LEU2). Cells transformed with the pHT212 plasmid or pHT212 plasmid with the human topo II insert were selected on plates lacking leucine (18). The HRR25 isolate expressing human topo II was transfomed with the human CKI cDNA, (kindly provided by Dr Jeff Kuret, Ohio State University, Columbus, OH), which was inserted in MluI and XbaI restriction sites of the modified pRS316 plasmid, YEpRS316. The YEpRS316 plasmid was constructed by insertion of the ScaI fragment from pYEpWOB6 which contains the 2 µm origin. Control transformations were carried out with the YEpRS316 plasmid (LEU2 and URA3). The transformed cells were selected on plates lacking leucine and uracil.

Metabolic labeling with [³²P] orthophosphoric acid
Log phase cultures of HL-60 or HCT-116 cells were incubated in phosphate-free RPMI-1640 supplemented with 10% dialyzed fetal bovine serum and 2 mM glutamine for 1 h at 37^°C. Cells were then labeled with carrier-free [³²P] orthophosphoric acid (MP Biomedicals, Irvine, CA) for an additional 3 h. During the labeling period, the CKI or CKII inhibitor was added for experiments involving these treatments. Yeast cells were labeled as previously described (18). Briefly, cells cultured overnight at 30°C with shaking (250 rpm) in synthetic dropout liquid medium lacking leucine were incubated in YPDA without phosphate medium, for 3 h with shaking, to a cell density corresponding to 0.6 units (A600). Following centrifugation, cells were resuspended into 20 ml of YPDA medium without phosphate containing 5 mCi of [³²P]-orthophosphoric acid and incubated at 30°C for 1 h with shaking.

Preparation of cell lysates, immunoprecipitation and western blotting
Lysates of HL-60 and HCT-116 cells were prepared in radioimmunoprecipitation assay (RIPA) buffer as described earlier (18). Topo II protein immunoprecipitated from the cell lysate was subjected to SDS–polyacrylamide gel electrophoresis (SDS–PAGE) and transferred to nitrocellulose membrane (18). The membrane was stained with Gelcode Blue staining reagent (Pierce Chemical Co., Rockford, IL) to visualize the topo II band, which was excised and processed for proteolysis with cyanogen bromide (CNBr) or trypsin (18). For determination of down-regulation of CKI and CKI, western blot analysis was carried out on cell lysates (20–40 µg) prepared from si-RNA transfected cells that were harvested just prior to labeling with [³²P]-orthophosphoric acid (32). Cell lysate of S. cerevisiae cells were prepared in Y-PER lysis buffer after freezing the cell pellet in liquid nitrogen and human topo II present in the lysate was purified by Ni²⁺-nitrilotriacetic acid essentially as described earlier (18). Purified topo II was subjected to SDS–PAGE, transferred to nitrocellulose membrane and the stained topo II band was processed for phosphopetide mapping.

Phosphopeptide mapping of ³²P-labeled topo II
The 170 kDa ³²P-labeled topo II band visualized by staining with Gelcode Blue staining reagent on the nitrocellulose membrane was excised and digested with trypsin essentially as described earlier (18). Following extensive washing of the membrane in water, topo II was proteolytically cleaved with 5 µg of trypsin-TPCK treated (Worthington Biochemical, Freehold, NJ) or with 2 µg of trypsin Gold® (Promega Inc., Madison, WI) in 1% ammonium bicarbonate, pH 8.3 at 37^°C for 14–16 h. In initial experiments involving treatment with CKI inhibitors, proteolytic digestion with TPCK-treated trypsin consistently led to generation of two Ser-1106 containing peptides due to partial proteolysis (Figure 1B), whereas in subsequent experiments trypsinization with highly purified trypsin Gold® consistently led to generation of a single Ser-1106 containing peptide. The tryptic peptides released in the ammonium bicarbonate solution were transferred to fresh microcentrifuge tube and the membrane piece was washed with 100 µl of 20% acetonitrile. The pooled eluate and washings were then concentrated by evaporation in a Savant Speed-Vac, washed three times with water and the peptides solubilized in pH 1.9 buffer (88% formic acid/glacial acetic acid/deionized water, 1:3.1:36, v/v). The peptides were then separated on thin layer cellulose plates by electrophoresis with pH 1.9 buffer in the horizontal dimension and chromatography in the vertical dimension (33). In initial experiments the phospho-chromatography buffer contained n-butanol/pyridine/acetic acid/deionized water (5/3.3/1/4, v/v). To improve migration of the Ser-1106-peptide an isobutyric acid buffer (isobutyric acid/n-butanol/pyridine/acetic acid/deionized water) (32.9/1/2.5/1.5/14.7, v/v), which resolves extremely hydrophilic phosphopeptides, was used.

View larger version (46K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 1. CKI inhibitors, CKI-7 and IC261, decrease phosphorylation of the topo II peptides containing Ser-1106. HL-60 cells were labeled with [32P] orthophosphoric acid for 3 h at 37°C in the absence or presence of CKI inhibitors, CKI-7 (200 µM) or IC261 (10 µM). Lysates of these cells were immunoprecipitated with topo II-specific antibodies. The immunoprecipitated protein was subjected to SDS–PAGE and transferred to nitrocellulose membrane. Two-thirds of the topo II band was cleaved with CNBr and one-third of the band was proteolysed with trypsin. (A) CNBr fragments of topo II from cells treated in the absence or presence of CKI-7 or IC261 were separated by SDS–PAGE. (B) Phosphopeptide maps of tryptic digests of topo II from cells treated in the absence (Control) or presence of CKI-7 or IC261. The phosphochromatography buffer, n-butanol/pyridine/acetic acid/deionized water (5/3.3/1/4, v/v), was used for resolving peptides in the second dimension. Arrows indicate the position of Ser-1106 containing peptides.

 
Liquid chromatography–tandem mass spectrometry (LC–MS)
LC–MS was carried out on tryptic digests of stained topo II protein band excised from SDS–polyacrylamide gels. In-gel trypsin digestion was carried out as described earlier (34). Briefly, following washing/destaining in two aliquots of 50% ethanol/5% acetic acid (v/v), reduction with dithiothreitol and alkylation with iodoacetamide, the excised gel pieces were dried in a Speed-vac and incubated with 30 µl of 20 ng/µl trypsin in 50 mM ammonium bicarbonate on ice for 10 min. Any excess trypsin solution was then removed and 20 µl of 50 mM ammonium bicarbonate was added. Following overnight digestion at room temperature, the peptides were extracted from polyacrylamide pieces in two 30 µl aliquots of 50% acetonitrile/5% formic acid (v/v). These extracts were combined and evaporated to 5 µl and then reconstituted in 1% acetic acid to a total volume of 25 µl for LC–MS analysis. The tryptic peptides in the extract (2 µl/injection) were separated by reversed-phase LC in a 10 cm x 50 µm (i.d.) Phenomenex Jupiter 10 µm C18 self-packed capillary column using a linear gradient of 2–70% acetonitrile containing 0.05 M acetic acid in 50 min at a constant flow rate of 0.2 µl/min. The effluent was analyzed using a Finnigan LCQ-Deca ion trap mass spectrometry system equipped with a Protana microelectrospray ion source (ThermoFisher, San Jose, CA) operated at 2.5 kV. Data interpretation was performed with the programs TurboSequest and Mascot. All matching spectra were verified by manual interpretation.

Selected reaction monitoring (SRM) mode was used to compare the extent of Ser-1106 phosphorylation in control scrambled si-RNA and si-CKI/ treated HCT-116 cells. The SRM experiment consisted of a 5-scan event analysis in which one scan event was a standard MS scan and the other four were different SRM descriptors directed to various sets of control or Ser-1106 containing peptides, both unphosphorylated and phosphorylated. To verify peptide recovery from the digestion procedure and the mass spectrometry response, one ion of the trypsin autolysis peptide VATVSLPR at m/z 422 (+2) and one ion of the unmodified topo II native peptide EVTFVPGLYK at m/z 577 (+2) were monitored. These two descriptors served as controls. In addition, the ion transition m/z 484 m/z 435 (+2) characteristic for phosphate loss from phosphorylated Ser-29 contained in RLpS²⁹VER peptide in topo II was monitored to confirm general phosphorylation of every sample. To determine the status of Ser-1106 phosphorylation, the peptide VPDEEENEES¹¹⁰⁶DNEKETEK containing phosphorylated Ser-1106 as doubly charged (m/z 1116) or triply charged (m/z 744) ion and their corresponding unphosphorylated peptide ions were monitored.

DNA cleavable complex formation
The effect of etoposide on forming a stable topo II–DNA cleavable complex was determined by measuring the amount of precipitated protein–DNA complex and by evaluating depletion of topo II not complexed with DNA (band depletion). For measuring precipitated protein–DNA complex, cells were labeled for 24 h with 0.02–0.04 µCi/ml of [¹⁴C]-thymidine, specific activity 53 mCi/mmol (Amersham, Arlington Heights, IL). For measuring DNA cleavable complex in cells down-regulated for CKI plus CKI, cells were treated for 6 h with scrambled si-RNA or si-CKI plus si-CKI prior to labeling. Cells were then trypsinized, treated with etoposide for 1 h and the precipitated protein–DNA complex was assayed as previously described (35). For the band depletion experiment cells were treated similarly without the addition of [¹⁴C]-thymidine. Cell lysates were prepared in 2-fold concentrated LDS-sample buffer (Invitrogen Life Technology, Carlsbad, CA, USA). The lysates were incubated at 70^°C for 10 min, sonicated and centrifuged at 12 000 x g. An aliquot (10–15 µl) of the lysate was subjected to western blot analysis. The membranes were probed with antibodies to topo II and topo I (internal control), which does not form a stabilized DNA cleavable complex with the topo II-targeted drug, etoposide. Down-regulation of CKI and CKI was also determined by western blotting with antibodies specific for CKI and CKI.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION FUNDING REFERENCES

 
Inhibitors of CKI and CKI (CKI-7 and IC261) lead to hypophosphorylation of the CNBr and tryptic topo II peptides containing Ser-1106 and reduce formation of etoposide stabilized topo II–DNA cleavable complex
The presence of acidic amino-acid residues N-terminal to Ser-1106 and the Ca²⁺-dependency of phosphorylation of this site (18) suggested that phosphorylation of Ser-1106 may be regulated by protein kinase CKI and/or CKI. Therefore we first examined whether two CKI inhibitors, CKI-7 and IC261, specific for CKI and CKI (36), altered phosphorylation of Ser-1106 containing peptides. Treatment of HL-60 cells with CKI-7 or IC261 led to hypophosphorylation of the CNBr (peptide 34) and tryptic phosphopeptides that were previously shown to harbor Ser-1106 (Figures 1A and 1B, respectively). Comparison of the intensity of spots corresponding to the peptides containing Ser-1106 (normalized to two other peptides) revealed that CKI-7 and IC-261 led to comparable decreases (20–40% and 25–30%, respectively) in phosphorylation of Ser-1106 as compared to untreated control cells. To determine whether decreased phosphorylation observed in the presence of CKI-7 or IC261 compromises the functional activity of topo II, we examined the effect of CKI-7 and IC261 on formation of etoposide stabilized topo II–DNA cleavable complex. Pre-treatment of HL-60 cells with 200 µM CKI-7 or 10 µM IC261 for 3 h prior to treatment with 5 µM etoposide for 1 h led to a significant (P < 0.05) decrease in the formation of etoposide-stabilized DNA cleavable complex (Figure 2). We also examined the effect of the CKII specific inhibitor, DRB, on formation of etoposide stabilized topo II–DNA cleavable complex. Pretreatment with 40 µM DRB did not alter etoposide stabilized topo II–DNA cleavable complex formation (Figure 2). These results suggest a role for CKI/ in regulating the functional activity of topo II via phosphorylation at Ser-1106.

View larger version (11K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 2. The CKI inhibitors, CKI-7 and IC261, but not the CKII inhibitor, DRB, decrease formation of etoposide-stabilized topo II–DNA cleavable complex. HL60 cells labeled overnight with 14C-thymidine were pre-incubated in the absence or presence of CKI-7 (200 µM), IC261 (10 µM) or DRB (40 µM) for 3 h at 37°C. Cells were then washed, resuspended in inhibitor-free medium and incubated for an additional hour in etoposide (5 µM). Control, labeled cells were incubated in the presence of medium alone. The labeled DNA was precipitated with SDS–KCl as described in Materials and methods section and the dpm in the precipitate was determined by liquid scintillation counting. DNA cleavable complex formation in the etoposide or inhibitor etoposide treatment was determined by calculating the ratio of dpm in treated cells to control cells. *Significantly (P < 0.05) lower than treatment with etoposide alone.

 
Down-regulation of CKI and/or CKI with targeted si-RNA decreases phosphorylation of the tryptic peptide containing Ser-1106
To confirm the role of CKI and/or CKI in phosphorylating Ser-1106 we down-regulated these two enzymes with three different sets of si-RNAs. These included si-CKI/—which targeted the nucleotide sequence (412–430) that is identical in the CKI and CKI coding region; si-CKI—which is a smart pool targeted to the CKI isozyme; and si-CKI—which is a smart pool targeted to the CKI isozyme. The si-CKI and si-CKI were used individually to down-regulate the specific isozyme or used in combination to simultaneously down-regulate both isozymes. Since, HL-60 cells are difficult to transfect we used the colon carcinoma cell line, HCT-116, for transfection of the si-RNAs. This cell line was chosen because it can be readily transfected and the phosphopeptide map of topo II in HCT-116 cells is similar to that in HL-60 cells (data not shown). Transfection of the three si-RNAs in HCT-116 cells led to significant down-regulation (60–80%) of the targeted isozyme; si-CKI/ and the combination of si-CKI and si-CKI led to down-regulation of both CKI and CKI, whereas si-CKI or si-CKI when used individually, down-regulated only the targeted enzyme CKI or CKI, respectively (Figures 3A, 5A and 8A). When both CKI and CKI were down-regulated a slight increase in the G₂ + M phase of the cell cycle was observed (data not shown).

View larger version (48K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 3. Phosphorylation of the topo II peptide containing Ser-1106 is reduced in HCT-116 cells transfected with si-CKI/, but not in nocadazole treated cells arrested in the G2+M phase of the cell cycle. HCT-116 cells were transfected with scrambled si-RNA or si-CKI/ as described in Materials and methods section, or treated for 16 h in the absence or presence of 200 nM nocadazole. For cells transfected with scrambled si-RNA or si-CKI/ a small aliquot was lysed in RIPA buffer and subjected to western blot analysis to determine down-regulation of CKI and CK1 (A). The remaining transfected cells (B), and cells treated in the absence or presence of nocadazole (C) were labeled with [32P] orthophosphoric acid for 3 h. At the end of the incubation, cells were lysed in RIPA buffer and cell lysates were immunoprecipitated with topo II-specific antibodies. The immunoprecipitated topo II protein was subjected to SDS–PAGE and transferred to nitrocellulose membrane. The topo II band was excised, proteolysed with trypsin and the labeled tryptic peptides analyzed by 2D-phosphopeptide mapping. The isobutyric acid buffer (isobutyric acid/n-butanol/pyridine/acetic acid/deionized water) (32.9/1/2.5/1.5/14.7, v/v) was used for resolving the peptides in the second dimension. The arrow indicates the position of Ser-1106 containing peptide.

 
The down-regulation of CKI and CKI in HCT-116 cells transfected with si-CKI/ resulted in significantly decreased (75%) phosphorylation of the tryptic Ser-1106 containing phosphopeptide, as compared to cells transfected with the control scrambled si-RNA (Figure 3B). This was not due to an increase in the G₂ + M population observed in cells transfected with si-CKI/, since phosphorylation at Ser-1106 was not affected when cells were blocked in mitosis following treatment with nocadazole (Figure 3C). Comparison of phosphorylation of Ser-1106 in topo II present in cells transfected with scrambled si-RNA or si-CKI/ by LC-MS (Figure 4) revealed findings that were similar to those obtained by 2D-phosphopeptide mapping. Although both phosphorylated and unphosphorylated Ser-1106 was detected in control cells transfected with scrambled si-RNA, only unphosphorylated Ser-1106 was detected in cells transfected with si-CKI/. Down-regulation of only one isozyme, CKI or CKI (Figure 5A), also led to hypophosphorylation of the Ser-1106 containing peptide (Figures 5B and 5C, respectively), albeit to a lesser extent than that observed when both CKI and CKI were down-regulated (Figure 3B). In cells treated with si-CKI, phosphorylation of Ser-1106 was 25–40% less than that observed in cells treated with scrambled si-RNA, whereas in cells treated with si-CKI phosphorylation of Ser-1106 was 40–65% less than that observed in cells treated with scrambled si-RNA. Differential hypophosphorylation of Ser-1106 in si-CKI and si-CKI transfected cells could be due to differences in the effectiveness of the two isozymes in phosphorylating this site or due to differential down-regulation of CKI (60%) and CKI (80%).

View larger version (28K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 4. Peptides containing phosphorylated Ser-1106 are not detected by LC-MS analysis of topo II from si-CKI/ transfected HCT-116 cells. HCT-116 cells were transfected with scrambled si-RNA or si-CKI/. Topo II protein present in these cells was purified by immunoprecipitation and SDS–PAGE. The stained topo II band in the gel was digested with trypsin and the peptides were analyzed by LC–MS as described in Materials and methods section. (A) Total ion chromatograms (upper panel) and trypsin autolysis marker at m/z 422 (lower panel) of topo II tryptic digests from cells transfected with scrambled si-RNA or si-CKI/. (B) SRM chromatograms for the doubly charged peptide ion containing phosphorylated Ser-1106 at m/z 1116 (upper panel) and CID spectrum of doubly charged peptide ion (lower panel) containing phosphorylated Ser-1106 in topo II, detected only in samples treated with scrambled si-RNA. (C) SRM chromatograms for the triply charged peptide ion containing phosphorylated Ser-1106 at m/z 744 (upper panel) and characteristic H3PO4 neutral loss for the m/z 744 (+3) phosphorylated peptide (middle panel). CID spectrum of triply charged peptide ion (lower panel) containing phosphorylated Ser-1106 in topo II was detected only in samples treated with scrambled si-RNA. Characteristic loss of H3PO4 is seen in both CID spectra. Detected b (N-terminal) and y (C-terminal) fragment ions are labeled in the spectra.

 

View larger version (42K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 5. Down-regulation of CKI or CK1 with targeted si-RNAs in HCT-116 cells decreases phosphorylation of the topo II peptide containing Ser-1106. HCT-116 cells were transfected with scrambled si-RNA, si-CKI or si-CKI as described in Materials and methods section. A small aliquot of the cells was lysed in RIPA buffer and subjected to western blot analysis to determine down-regulation of CKI and CKI (A). The remaining cells were labeled with [32P] orthophosphoric acid for 3 h, lysed in RIPA buffer and the cell lysates were immunoprecipitated with topo II-specific antibodies. The immunoprecipitated topo II protein was subjected to SDS–PAGE and transferred to nitrocellulose membrane. The stained topo II band was excised, proteolysed with trypsin and the labeled tryptic peptides analyzed by 2D-phosphopeptide mapping (B, C). The isobutyric acid buffer (isobutyric acid/n-butanol/pyridine/acetic acid/deionized water) (32.9/1/2.5/1.5/14.7, v/v) was used for resolving the peptides in the second dimension. The arrow indicates the position of Ser-1106 containing peptide.

 
To confirm that phosphorylation of Ser-1106 in vivo does not involve CKII we examined the effect of transfecting HCT-116 cells with si-RNAs to CKII and CKII' on phosphorylation of Ser-1106. Results of this experiment revealed that transfectants, in which CKII and CKII' were significantly down-regulated (Figure 6A), did not exhibit altered phosphorylation of Ser-1106 although phosphorylation of other tryptic peptides previously reported to be substrates for casein kinase II (6) was reduced (Figure 6B).

View larger version (60K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 6. Down-regulation of CKII and ' with targeted si-RNAs does not alter phosphorylation of the topo II peptide containing Ser-1106. An aliquot of HCT-116 cells transfected with scrambled si-RNA or si-CKII plus si-CKII', as described in Materials and methods section, were lysed in RIPA buffer and subjected to western blot analysis to determine down-regulation of CKII and CKII' (A). The remaining cells were labeled with [32P] orthophosphoric acid for 3 h. Cell lysates prepared in RIPA buffer were immunoprecipitated with topo II-specific antibodies, subjected to SDS–PAGE and transferred to nitrocellulose membrane. The stained topo II band was excised, proteolysed with trypsin and the labeled tryptic peptides analyzed by 2D-phosphopeptide mapping (B). The isobutyric acid buffer (isobutyric acid/n-butanol/pyridine/acetic acid/deionized water) (32.9/1/2.5/1.5/14.7, v/v) was used for resolving the peptides in the second dimension. The arrow indicates the position of Ser-1106 containing peptide.

 
Phosphorylation of Ser-1106 in human topo II expressed in HRR25 S. cerevisae cells is reduced, but can be enhanced following transformation of the cells with human CKI
Since human topo II expressed in S. cerevisiae cells is phosphorylated at Ser-1106 (18) and the S. cerevisiae gene, HRR25 is homologous to CKI and CKI (37), we compared phosphorylation of Ser-1106 in WT or HRR25 cells transformed with human topo II. As shown in Figure 7A, phosphorylation of the tryptic Ser-1106 peptide was significantly reduced in HRR25 cells. Transformation of the HRR25 cells expressing human topo II with human CKI enhanced phosphorylation at Ser-1106 (Figure 7B). This finding provides further support for the role of CKI/, in particular the CKI isozyme, in regulating phosphorylation at Ser-1106 in topo II.

View larger version (64K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 7. Phosphorylation of Ser-1106 in human topo II expressing HRR25 S. cerevisae cells is reduced, but can be enhanced following transformation of the cells with human CKI. WT W303 cells or HRR25 isolate isogenic to W303 cells transformed with human topo II (A), or topo II expressing HRR25 W303 cells transformed with vector control or human CKI cDNA (B) were labeled with [32P] orthophosphoric acid for 1 h as described in Materials and methods section. Topo II from cell lysates prepared in Y-PER lysis buffer was purified by Ni2+-nitrilotriacetic acid or immunoprecipitated with topo II antibody. Purified topo II was subjected to SDS–PAGE and transferred to nitrocellulose membrane. The stained topo II band was excised, proteolysed with trypsin and the labeled tryptic peptides analyzed by 2D-phosphopeptide mapping. The phosphochromatography buffer, n-butanol/pyridine/acetic acid/deionized water (5/3.3/1/4, v/v), was used for separating the peptides in the second dimension (A) and the isobutyric acid buffer (isobutyric acid/n-butanol/pyridine/acetic acid/deionized water) (32.9/1/2.5/1.5/14.7, v/v) was used for resolving the peptides in the second dimension (B). The arrow indicates the position of Ser-1106 containing peptide.

 

View larger version (22K): [in this window] [in a new window] [Download PowerPoint slide]   Figure 8. Down-regulation of CKI and CKI in HCT-116 cells leads to reduced topo II–DNA cleavage activity. HCT-116 cells were treated with scrambled si-CKI (75 nM) plus si-CKI (75 nM) as described in Materials and methods section and subsequently treated with etoposide for 1 h. An aliquot of the cell lysate was used to determine down regulation of CKI and CKI (A). Cells labeled with [14C] thymidine were lysed and precipitated with SDS–KCl. The dpm present in the precipitate was determined by liquid scintillation counting (B). *Significantly (P < 0.01) lower than scrambled si-RNA-treated cells. Band depletion of topo II not present in the etoposide–stabilized DNA complex was determined by western blotting of lysates prepared in 2-fold concentrated LDS-sample buffer (C). The amount of topo II was normalized with topo I, which does not form a stable complex with the topo II-targeted drug, etoposide.

 
Reduced phosphorylation of Ser-1106 in HCT-116 cells transfected with si-CKI plus si-CKI leads to decreased formation of etoposide stabilized topo II–DNA cleavable complex
We previously demonstrated a functional role for Ser-1106 phosphorylation in topo II, based on the observation that mutation of Ser-1106 to alanine in human topo II led to decreased topo II function in vitro and in vivo in JN394 yeast cells transformed with human topo II (18). In this study we examined whether topo II function is affected when phosphorylation at Ser-1106 is altered by down-regulating the kinase(s), CKI and/or CKI, involved in phosphorylating this residue. Down-regulation of CKI and CKI by si-CKI plus si-CKI (Figure 8A) led to a significant (P < 0.01) decrease in SDS–KCl precipitable ¹⁴C-thymidine labeled etoposide stabilized topo II–DNA cleavable complex (Figure 8B). Since, formation of a stable topo II–DNA cleavable complex in the presence of etoposide leads to depletion of topo II not complexed with DNA, we also determined the amount of topo II in lysates of control or etoposide-treated HCT-116 cells that were transiently transfected with scrambled si-RNA or si-CKI plus si-CKI. In cells transfected with si-CKI plus si-CKI depletion of topo II following treatment with etoposide was less (40–50%) than that observed in cells transfected with scrambled si-RNA (Figure 8C). This finding corroborates the previous data demonstrating decreased formation of the etoposide stabilized topo II–DNA cleavable complex in cells transfected with si-CKI plus si-CKI. These results indicate that CKI and/or CKI are involved in regulating topo II function via phosphorylation at Ser-1106.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION FUNDING REFERENCES

 
In the present study we identify CKI and/or CKI as upstream kinase(s) regulating in vivo phosphorylation of topo II at Ser-1106 and thereby modulating the DNA cleavage activity of the enzyme. The role of CKI and/or CKI in phosphorylating Ser-1106 is based on several lines of experimental evidence. In vivo phosphorylation of the tryptic peptide that contains Ser-1106 is decreased when CKI and/or CKI are inhibited by the CKI inhibitors, CKI-7 and IC261 (specific for CKI/), or when CKI and CKI are down-regulated by targeted si-RNAs. Similarly, in human topo II expressing HRR25 (CKI and CKI homologous gene) deleted S. cerevisiae cells, the tryptic peptide containing Ser-1106 is also hypophosphorylated, and phosphorylation at this site can be enhanced following transformation of these cells with human CKI. The decrease in phosphorylation of the Ser-1106 tryptic peptide is indeed due to reduced phosphorylation at this site, since our earlier studies indicated that in vivo phosphorylation of this tryptic peptide was not observed when Ser-1106 in topo II was mutated to alanine (18). Furthermore, LC–MS analysis of phosphorylated Ser-1106 in topo II obtained from HCT-116 cells treated with scrambled si-RNA or si-CKI/ revealed the presence of phosphorylated Ser-1106 only in scrambled si-RNA treated cells.

The decrease in phosphorylation at Ser-1106 observed in cells exhibiting reduced kinase activity of CKI and CKI correlates with a decrease in topo II function. Inhibition of the CKI activity in cells treated with CKI inhibitors, CKI-7 or IC-261 leads to reduced formation of topo II–drug DNA complex in vivo. Similarly, when CKI and CKI are down-regulated by targeted si-RNAs, formation of the etoposide stabilized topo II–DNA cleavable complex is reduced. These results indicate that the phosphorylation at Ser-1106 catalyzed by CKI and/or CKI enhances the in vivo DNA cleavage activity of topo II.

Several different kinases, including CKII, protein kinase C, proline directed kinases e.g. cdc2 and Polo-like kinase 1 have been reported to phosphorylate topo II (6,9–17). However, this is the first report demonstrating CKI as a physiologically relevant kinase that modulates phosphorylation and activity of topo II. Our data demonstrating decreased phosphorylation of several peptides (excluding the Ser-1106 containing peptide) following down-regulation of CKII and CKII' with targeted si-RNAs provides evidence that CKII is also capable of phosphorylating topo II in vivo. However, phosphorylation at CKII sites does not significantly affect sensitivity to topoII-targeted drugs, since treatment of HL-60 cells with the CKII inhibitor, DRB, did not significantly alter formation of topo II-drug–DNA complex in vivo. Since our study did not evaluate the effect of reduced phosphorylation at CKII sites on other functions of topo II, the functional role of phosphorylations at CKII sites remains unclear. It is possible that phosphorylation at CKII sites, most of which map to regions in the C-terminal domain, along with other phosphorylations within this region regulate accessibility of the catalytic site to its substrate. This mechanism would be analogous to that described for regulation of the activity of CKI and CKI, wherein dephosphorylation of the C-terminal region activates the enzyme.

Our previous data demonstrating Ca²⁺-dependent phosphorylation of Ser-1106 (18), provides further support for the role of CKI and/or CKI (Ca²⁺-regulatable enzymes), but not CKII, as physiologic kinases that modulate Ser-1106 phosphorylation. Although, the catalytic activity of CKI and CKI does not require Ca²⁺, these enzymes can be regulated via Ca²⁺-dependent dephosphorylation or proteolysis (25,26). In neostriatal neurons, the metabotrophic glutamate receptors activate CKI by dephosphorylating the inhibitory C-terminal autophosphorylation sites by the Ca²⁺-dependent phosphatase, calcineurin (38). The activated CKI then leads to phosphorylation of Ser-137 of DARPP-32. A scenario similar to that described in neostriatal muscles, could explain how phosphorylation of Ser-1106 is regulated by Ca²⁺. Dephosphorylation by calcineurin and subsequent activation of CKI and/or CKI could result in phosphorylation of Ser-1106. Alternatively, a Ca²⁺-dependent protease, e.g. calpain, which is activated by calcium influx in neurons (27,39), could remove the inhibitory domain in CKI or CKI and lead to activation of these kinases.

CKI isozymes are involved in regulating several different cellular processes (40). The CKI and CKI isozymes have been shown to modulate the development process because of their role in the wnt signaling pathway. In addition, these isozymes play a role in circadian rhythm, cell division, apoptosis and neurodegenerative diseases. CKI and CKI phosphorylate p53, tubulin and microtubule-associated proteins to regulate cell growth, chromosome segregation and stress response at the spindle apparatus and the mitotic centrosome. The identification of topo II, which is also involved in regulating DNA replication and cell division, chromosome segregation and DNA repair, as another nuclear substrate of CKI and/or CKI in this study, suggests that these CKI isozymes may be essential for regulating various aspects of DNA metabolism. In this regard, topo II could function as part of a protein complex that comprises of transcription factors, nuclear regulatory proteins and kinases (including CKI and/or CKI)/phosphatases that regulate phosphorylation/dephosphorylation of components of the complex. Thus, it would be important to determine whether CKI or CKI is capable of associating with topo II.

In summary our results demonstrate that CKI and/or CKI are physiologically relevant kinase(s) that are involved in regulating site-specific phosphorylation at Ser-1106 and modulating the function of topo II. Since Ser-1106 phosphorylation regulates sensitivity of cells to topo II-targeted drugs and expression of CKI and/or CKI can be altered in cancer cells, one potential mechanism by which tumor cells develop resistance to topo II-targeted drugs could involve decrease in expression or activation of CKI and/or CKI. The correlation of Ser-1106 hypophosphorylation with etoposide resistance was not only observed in cell culture model systems but was also seen in blast cells isolated from patients with acute myelogenous leukemia. Comparison of Ser-1106 phosphorylation with etoposide induced apoptosis revealed that reduced phosphorylation at Ser-1106 was associated with decreased apoptosis (data not shown). Thus, it might be possible to identify sensitivity of tumors to topo II-targeting drugs by characterizing phosphorylation at Ser-1106 or by determining the expression level or activity of CKI and CKI in tumor samples.

	FUNDING

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION FUNDING REFERENCES

 
This work was supported by United States Public Health Service (grant numbers RO1 CA 74939, RO1 CA 117928). Funding for open access charge: National Institutes of Health.

Conflict of interest statement. None declared

	Footnotes

 
Present addresses: Kenichi Chikamori, NHO Sanyo Hospital, 685 Higashi-Kiwa, Ube, Yamaguchi 755-0241, Japan Michael Kinter, Free Radical Biology and Aging Research Program, MS 21, Oklahoma Medical Research Foundation, 825 N.E. 13th Street, Oklahoma City, OK 73104, USA

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