Overexpression of survivin in primary ATL cells and sodium arsenite induces apoptosis by down-regulating survivin expression in ATL cell lines

doi:10.1182/blood-2005-08-3423

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Blood, 15 June 2006, Vol. 107, No. 12, pp. 4880-4887.
Prepublished online as a Blood First Edition Paper on February 23, 2006; DOI 10.1182/blood-2005-08-3423.

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NEOPLASIA
Overexpression of survivin in primary ATL cells and sodium arsenite induces apoptosis by down-regulating survivin expression in ATL cell lines
Xiao-Fang Che, Chun-Lei Zheng, Satsuki Owatari, Masato Mutoh, Takenari Gotanda, Hei-Cheul Jeung, Tatsuhiko Furukawa, Ryuji Ikeda, Masatatsu Yamamoto, Misako Haraguchi, Naomichi Arima, and Shin-ichi Akiyama
From the Department of Molecular Oncology, Graduate School of Medical & Dental Sciences, and Department of Hematology and Immunology, Kagoshima University Hospital, Center for Chronic Viral Diseases, Division of Host Response, Kagoshima University, Sakuragaoka, Japan; and Pharmaceutical Research Laboratories, Toray Industries, Kamakura-city, Kanagawa, Japan.

   Abstract

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Patients with acute- or lymphoma-type adult T-cell leukemia(ATL) have a poor outcome because of the intrinsic drug resistanceto chemotherapy. Protection from apoptosis is a common featureinvolved in multidrug-resistance of ATL. IAP (inhibitor of apoptosis)family proteins inhibit apoptosis induced by a variety of stimuli.In this study, we investigated the expression of IAP familymembers (survivin, cIAP1, cIAP2, and XIAP) in the primary leukemiccells from patients with ATL. We found that survivin was overexpressedin ATL, especially in acute-type ATL. Sodium arsenite was shownto down-regulate the expression of survivin at both the proteinand RNA levels in a time- and dose-dependent manner, thus inhibitingcell growth, inducing apoptosis, and enhancing the caspase-3activity in ATL cells. Nuclear factor- ${kappa}$ B (NF- ${kappa}$ B) enhances thetranscriptional activity of survivin. Sodium arsenite suppressedthe constitutive NF- ${kappa}$ B activation by preventing the I ${kappa}$ B- ${alpha}$ degradationand the nuclear translocation of NF- ${kappa}$ B. These findings suggestthat survivin is an important antiapoptotic molecule that confersdrug resistance on ATL cells. Sodium arsenite was shown to down-regulatethe expression of survivin through the NF- ${kappa}$ B pathway, thus inhibitingcell growth and promoting apoptosis of ATL cells.

   Introduction

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Adult T-cell leukemia (ATL) is an aggressive malignancy of CD4⁺T cells associated with human T-cell leukemia virus type 1 (HTLV-1)infection.¹ There is evidence suggesting that HTLV-1 viral Taxprotein activates the expression of a number of cellular genes,such as growth factors, growth factor receptors, and oncogenes,through the induction of transcription factors, such as nuclearfactor- ${kappa}$ B (NF- ${kappa}$ B),² cyclic adenosine monophosphate (cAMP) responseelement binding protein (CREB)/AP-1 transcription factor (ATF),³and serum response factor (SRF).⁴ However, the presence of taxgene expression has not yet been clearly established in freshlyisolated ATL cells; moreover, defective viruses, which cannotproduce Tax, have been observed in ATL cells, thus suggestingthat the tax gene is necessary for the initial stages of leukemogenesis,but it is not essential for the late stage of leukemia.⁵ Assuggested by the multistep model of tumorigenesis,⁶ mutationsof various genes are considered to contribute to leukemogenesis.
ATL is divided into 4 clinical subtypes: acute, lymphoma, chronic,and smoldering.⁷ Chronic- and smoldering-type ATLs have a mildclinical course and do not require treatment with intensivechemotherapy. Acute- and lymphoma-type ATLs require intensivechemotherapy, and the median survival period is less than 1year because of resistance to chemotherapy. Several mechanismsare involved in the multidrug resistance of ATL, including theoverexpression of P-glycoprotein (P-gp),⁸ multidrug resistanceprotein 1 (MRP1),⁹ and lung resistance-related protein (LRP).¹⁰Accumulating evidence suggests that the activation of NF- ${kappa}$ B isa critical process in the inhibition of apoptosis and resistanceto chemotherapy.¹¹
Survivin, cIAP1, cIAP2, and XIAP belong to the IAP (inhibitorof apoptosis) family, which is defined by 1 or more repeatsof a highly conserved 70–amino acid domain called thebaculovirus IAP repeat (BIR) located at the amino-terminus.IAP family proteins directly bind and inhibit certain caspasesand also inhibit apoptosis induced by a variety of stimuli.¹²Previous studies have revealed that several IAPs, such as survivin,NAIP, and XIAP, were overexpressed in acutel myeloid leukemia(AML).¹³ Survivin was overexpressed in chronic lymphocytic leukemia(CLL) and ATL.^14,15 The IAPs are probably involved in the drugresistance in leukemia. Survivin was also demonstrated to bean unfavorable prognostic factor in leukemia, oral squamouscell carcinoma, and bladder cancer.^16-19 Among the known IAPs,survivin was prominently and consistently expressed in ATL andthe expression level of the survivin mRNA has correlated witha shorter survival of the patients.¹⁵ However, the expressionof other IAP members such as IAP1, IAP2, and XIAP in ATL isstill uncertain. Ishitsuka and colleagues showed that arsenictrioxide (As₂O₃) has a therapeutic potential for the treatmentof ATL.²⁰ They suggested that As₂O₃ induced apoptosis of ATLcells by the destruction of the Bcl-2 protein and the enhancementof the Bak protein production.²¹
In the present study, we investigated the expression levelsof the members of the IAP family in primary ATL cells. We thusfound survivin to be overexpressed in ATL while sodium arseniteinhibited cell growth and apoptosis through the down-regulationof survivin.

   Patients, materials, and methods

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Patients
Between July 1999 and July 2003, we studied 38 patients withATL (Table 1) consisting of 18 men and 20 women with a medianage of 62 years (range, 21-87 years). According to previouslyreported diagnostic criteria,⁷ 23 of these patients had acute-typeATL, 12 had chronic-type ATL, and 3 had smoldering-type ATL.The performance status (PS) was based on the 5-grade scale ofthe World Health Organization. Seventeen patients had a PS of0; 8 patients had a PS of 1; 6 patients had a PS of 2; 3 patientshad a PS of 3; and 4 patients had a PS of 4. During this study,we treated patients with acute ATL with combination chemotherapyregimens such as a response-oriented multidrug protocol; a cyclophosphamide,DOX, vincristine, and prednisone protocol; or an LSG15 protocol.None of the patients with chronic and smoldering ATL requiredtreatment with intensive chemotherapy. Approval for this studywas obtained from the Kagoshima University institutional reviewboard. Informed consent was provided according to the Declarationof Helsinki.

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Table 1.. Patient characteristics

Reagents and antibodies
RPMI 1640 was purchased from Nissui Seiyaku (Tokyo, Japan).Fetal calf serum (FCS) was obtained from Equitech-Bio (Kerrville,TX). Sodium arsenite (NaAsO₂, AsIII) and Ac-DEVD-MCA (Ac-Asp-Glu-Val-Asp-MCA)were obtained from Wako Pure Chemical Industries (Osaka, Japan).MTT (3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium bromide)was obtained from Sigma Chemical (St Louis, MO).
Antibodies against NF- ${kappa}$ B (polyclonal antibody p65 and monoclonalantibody p50) and monoclonal antibodies against Bcl-2, PARP,and I ${kappa}$ B- ${alpha}$ were obtained from Santa Cruz Biotechnology (Santa Cruz,CA). A monoclonal antibody against ${alpha}$ -tubulin was from Oncogene(Boston, MA). A polyclonal antibody against survivin, MP001,was prepared in our laboratory. MRPm6, a monoclonal antibodyagainst MRP1, was purchased from Progen Biotechnick (Heidelberg,Germany).
Cell lines and cell cultures
The human ATL cell line MT2 is derived from normal human leucocytestransformed by the leukemic T cells of a patient with ATL; S1Tcomes from HTLV-1–infected CD4⁺ T cells with no Tax expressionthat are derived from a patient with ATL. The acute T-cell lymphomacell line Jurkat was used as a control. The cell lines weregrown in RPMI 1640 containing 10% FCS, 2 mM glutamine, and 100U/mL penicillin at 37°C in a 5% CO₂ humidified atmosphere.
cDNA synthesis
Peripheral blood mononuclear cells were separated by Ficoll-Conray(Immuno-Biological, Gunma, Japan) density gradient centrifugationand stored at –80°C until use for RNA or protein extraction.The total RNA from peripheral blood mononuclear cells and thecultured cells was isolated using TRIzol reagent (Invitrogen,Carlsbad, CA). RNA (1 µg) was reverse transcribed usinga first-strand cDNA synthesis kit (ReverTra Ace ${alpha}$ ; TOYOBO, Osaka,Japan).
Reverse transcription–PCR
The resulting first-strand cDNA (1 µL) was used for eachpolymerase chain reaction (PCR). The human survivin primerswere as follows: forward, 5'-GAT TTG AAT CGC GGG ACC CGT TG-3';and reverse, 5'-TCAAGA CAA AAC AGG AGC ACA GT-3'. The primersof $beta$ -actin for internal control were as follows: forward, 5'-CAGCTT CGG AAC AAG AGA CC-3'; and reverse, 5'-GTC CGA TGA TTC CTGCTG AT-3'.
The PCR amplification mixture was adjusted to a final volumeof 20 µL. Twenty-five cycles were performed at 94°Cfor 30 seconds for denaturation, 58°C for 30 seconds forannealing, and 72°C for 1 minute for extension. The PCRproducts were separated on 1% agarose gel and then were stainedwith ethidium bromide.
Real-time reverse transcription–PCR quantification
The resulting first-strand cDNA (1 µL) was assayed byreal-time reverse transcription (RT)–PCR (PRISM 7900HT;Applied Biosystems, Foster City, CA) according to a technicalbrochure of the company. The sets of primers and TaqMan probeswere designed with the primer design software Primer Expressversion 2.0 (Applied Biosystems). The primers and TaqMan probeswere as follows: The sequence of the forward primer for survivinmRNA was 5'-TTC AAG AAC TGG CCC TTC TTG-3', and that of thereverse primer was 5'-TGG CTC CCA GCC TTC CA-3'; the TaqManprobe was FAM-CCT GCA CCC CGG AGC GGA T-TAMRA. For XIAP mRNA,the forward primer was 5'-GCC TTA GAC AGG CCA TCT GAG A-3',and the reverse primer was 5'-TTC CTC GGG TAT ATG GTG TCT GAT-3';the TaqMan probe was FAM-TGC AGA CTA TCT TTT GAG AAC TGG GCAGGT-TAMRA. For cIAP1 mRNA, the forward primer was 5'-CAG ACACAT GCA GCT CGA ATG-3', and the reverse primer was 5'-AAG CCACCA TCA CAA CAA AAG-3'; the TaqMan probe was FAM-TGT TCC AGTTCA GCC TGA GCA GCT TG-TAMRA. The forward primer for GAPDH mRNAwas 5'-GAA GGT GAA GGT CGG AGT-3', and the reverse primer was5'-GAA GAT GGT GAT GGG ATT TC-3'; the TaqMan probe was FAM-CAAGCT TCC CGT TCT CAG CC-TAMRA. The conditions for the 1-stepRT-PCR were as follows: 2 minutes at 50°C and 10 minutesat 95°C, and then 40 cycles of amplification for TaqManUniversal PCR Master Mix (Roche, Branchburg, NJ) at 95°Cfor 15 seconds and annealing and extension at 60°C for 1minute. Human GAPDH was used for normalization. Quantificationof the target gene expression was done using the comparativecycle threshold method according to the instructions of themanufacturer (Applied Biosystems). All experiments were performedin triplicate for each data point. Each quantitation was performedwith the standard curve method.
Protein extraction and Western blotting
After treatment with various concentrations of sodium arsenite,cells were harvested and lysed with RIPA buffer (50 mM Tris-HCl[pH 7.4], 150 mM NaCl, 1 mM EGTA, 1 mM EDTA, 20 mM NaF, 100mM Na₃VO₄, 0.5% Nonidet P-40 [NP-40], 1% Triton X-100, and 1mM PMSF). The lysates were passed through a 21-gauge needleto break up the cell aggregates, and were cleared by centrifugationat 14 000g for 15 minutes at 4°C; the supernatant (totalcell lysate) was immediately used or stored at –80°Cuntil use.
For the detection of NF- ${kappa}$ B, the cells were washed with ice-coldphosphate-buffered saline (PBS) and lysed in 400 µL lysisbuffer (buffer A, containing 10 mM HEPES [pH 7.9], 10 mM KCl,0.2 mM EDTA, 1 mM DTT, 0.5 mM PMSF, and 0.6% NP-40). The lysateswere centrifuged at 250g for 10 minutes. The supernatant wascollected as the cytosolic fraction. The pellets containingthe nuclei were washed in buffer A without NP-40 and then wereresuspended in 50 µL nuclear lysis buffer (buffer C, containing20 mM HEPES [pH 7.9], 0.4 M NaCl, 2 mM EDTA, 1 mM DTT, and 1mM PMSF), incubated for 30 minutes at 4°C, and centrifugedat 20 000g for 20 minutes. The supernatants were either usedas nuclear fractions immediately or stored at –80°Cuntil use. The protein concentration was determined by a Bio-Radprotein assay according to the manufacturer's protocol (Bio-RadLaboratories, Hercules, CA).
Lysates containing 100 µg of protein were subjected to12.5% or 9.4% SDS-polyacrylamide gel electrophoresis (SDS-PAGE),and then were transferred to Immobilon-P membrane (Millipore,Bedford, MA). The membrane was incubated with the primary antibody(dilution of 1:1000) overnight at 4°C and then with a peroxidase-linkedsecondary antibody (dilution of 1:2000) for 1 hour at room temperature,and proteins were visualized by enhanced chemiluminescence.
For detection of MRP1, 100 µg crude membranes preparedfrom Jurkat and S1T cells and 10 µg membrane vesiclesprepared from KB/MRP, which was used as a positive control,were subjected to 7.5% SDS-PAGE, and an m6 monoclonal antibodyagainst MRP1 was used for MRP1 detection. The density of thebands for MRP1 was quantified using a charge-coupled device(CCD) camera (Bio-Rad Laboratories-Segrate, Milan, Italy).
Cell survival by the MTT assay
MT2 (2 x 10⁴/mL), S1T, and Jurkat cells (1 x 10⁴/mL) were incubatedeither with or without various concentrations of sodium arsenitefor the indicated time in 96-well plates. Ten µL MTT solution(5 µg/mL) was added to each well and then the plates wereincubated for an additional 4 hours. The MTT formazan precipitatewas dissolved in 100 µL isopropanol containing 0.04 NHCl. The plates were shaken for 5 minutes and read immediatelyat 570 nm using a model 550 Micro Plate Reader (Bio-Rad, Hercules,CA).
For chemosensitivity in vitro, MT2, S1T, and Jurkat cells (1x 10⁴/mL) were incubated in culture medium with various concentrationsof indicated drugs at a final volume of 100 µL. After3 days, 10 µL MTT was added to each well and the plateswere incubated for an additional 4 hours. Optical density at570 nm (OD₅₇₀) was measured as described.
Apoptosis analysis by FACS
MT2, S1T, and Jurkat cells (1 x 10⁶) were treated with variousconcentrations of sodium arsenite for various periods. The cellswere harvested, washed once with PBS, suspended in 50 µLPBS, and mixed with 50 µL Coulter DNA-prep LRP (COULTER,Miami, FL), and then 1 mL Coulter DNA-prep Stain was added.The mixtures were then incubated for 15 minutes at room temperature.The sub-G₁ fraction was determined using a Coulter FACSCAN (BectonDickinson, San Jose, CA) as previously described.²²
Caspase-3 activity assay
Enzymatic reactions were carried out in the mixture containing50 µg cell lysate treated by various concentrations ofsodium arsenite, interleukin-1 $beta$ -converting enzyme (ICE)–likeenzyme assay buffer (100 mM HEPES [pH 7.5], 10% sucrose, and0.1% CHAPS), and 10 mM DTT. The reaction mixtures were incubatedat 30°C for 30 minutes. Next, the 50 µM syntheticfluorogenic substrate, Ac-DEVD-MCA (Ac-Asp-Glu-Val-Asp-MCA),was added and incubated at 30°C for another 60 minutes.The activity of caspase-3 was measured at an excitation wavelengthof 360 nm and an emission wavelength of 460 nm using a FP750microplate fluorescence reader (Jasco, Tokyo, Japan).
Statistical analysis
All statistical analyses were performed by the Statview 5.0software package for Windows (SAS Institute, Cary, NC). Forpatients with ATL, differences in the numerical data betweenthe 2 groups were evaluated using the Mann-Whitney U test. AP value of less than .05 was considered to be statisticallysignificant.
For the MTT assay, the fluorescence-activated cell-sorting (FACS)analysis, and the caspase-3 activity, the quantitative datawere expressed as the mean plus or minus standard deviation(SD). Statistical comparisons were performed using one-way analysisof variance (ANOVA) or the unpaired Student t test. Differenceswere regarded as significant when the probability values wereless than .01.

   Results

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
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Expression of mRNA for IAP proteins determined by real-time quantitative PCR or RT-PCR
ATL's drug resistance is one of the main obstacles to successfulchemotherapy. Kamihira et al¹⁵ reported that survivin was prominentlyand consistently expressed in ATL, thus correlating with theATL prognosis. However, the role of other IAP members such asIAP1, IAP2, and XIAP in the resistance of ATL to chemotherapyis uncertain. To quantitate the mRNA expression levels of theIAP family in ATL cells, real-time quantitative RT-PCR was performed.As shown in Figure 1A, the expression of the survivin gene wassignificantly higher (P < .01) in acute, chronic, and smolderingATL than that in healthy controls. The expression of the survivingene in acute ATL was higher than that in chronic and smolderingATL (P < .05). The expression of the survivin gene in PS3to PS4 ATL was higher than that in PS0 to PS2 ATL (P < .05).The mRNA levels of cIAP1 and XIAP (Figure 1B-C) did not differsubstantially among the subtypes of ATL and the healthy controls,and between PS0 to PS2 and PS3 to PS4 ATLs. The expression ofcIAP2 was also detected by RT-PCR, but the expression levelin ATL did not increase significantly more than that in thecontrol (data not shown). The patients' age, sex, and whiteblood cell (WBC) count of ATL were not correlated with the expressionof IAP proteins (data not shown). These results show that onlythe survivin gene was overexpressed in ATL, thereby showinga correlation with the PS of the patients.
Protein expression of survivin in ATL
We next examined the expression levels of survivin in ATL cellsfrom 17 patients by Western blotting (Figure 2A), and comparedwith the survivin mRNA levels in ATL cells of each patient.As shown in Figure 2B, the expression level of survivin mRNAwas significantly correlated with that of the protein (r = 0.516,P = .033). These results suggest that survivin alone is overexpressedamong the members of the IAP family in ATL, especially in acuteATL. The survivin expression level was correlated with the ATLprogression (Figure 1A).
Down-regulation of survivin by sodium arsenite in ATL cells
As₂O₃ was shown to have a therapeutic effect against acute promyelocyticleukemia (APL) and other types of haemotologic malignanciesby decreasing the expression of Bcl-2 and inducing apoptosis.It was recently reported that As₂O₃ combined with interferon ${alpha}$ (IFN- ${alpha}$ ) could also induce apoptosis in ATL cells. We thus investigatedwhether sodium arsenite can regulate the expression of survivinin ATL cells. MT2 (Tax-positive), S1T (Tax-negtive), and a T-celllymphoma cell line, Jurkat (as a control) cells were treatedwith 0, 2, and 5 µM sodium arsenite for 1, 2, and 3 days,and the expression of survivin and BCL-2 was detected by Westernblotting. ${alpha}$ -tubulin was used as a control for protein loading.The expression of survivin in MT2 and S1T cells dramaticallydecreased from 2 days after treatment with 2 and 5 µMsodium arsenite (Figure 3A). The relative density of survivincompared with the untreated controls is shown in Figure 3B.However, no clear down-regulation of survivin in Jurkat cellswas detected (Figure 3A-B). Sodium arsenite did not down-regulateBcl-2 expression in all 3 cell lines used in this study. TheRNA level of survivin was also decreased by sodium arsenitetreatment in S1T cells, but not in Jurkat cells (Figure 3C).These data suggest that survivin is a target of sodium arsenitein ATL cells. Sodium arsenite could both dose- and time-dependentlydown-regulate the survivin expression at the RNA and proteinlevels in ATL cells.

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Figure 1.. IAP family mRNA expression. A quantitative RT-PCR analysis for survivin (A), cIAP1 (B), and XIAP (C) is shown in patients with acute, chronic, and smoldering ATL and in a healthy control (left), low PS and high PS (right). Each mRNA expression level was normalized on the basis of the GAPDH mRNA expression and expressed relative to the mRNA level in a healthy control. Boxes correspond to the interquartile range. Lines in the boxes represent median values. The vertical lines represent the 10th and 90th percentiles, and the circles represent the outliers. Differences were analyzed by Mann-Whitney's U test.

Effects of sodium arsenite on cell proliferation
We next examined whether the growth inhibition of ATL cellsby sodium arsenite correlates with the suppression of survivinexpression. MT2, S1T, and Jurkat cells were treated with 0,0.5, 1, 2, 5, and 10 µM sodium arsenite for 5 to 7 days,and cell proliferation was measured by an MTT assay. As shownin Figure 4, the growth of MT2 and S1T cells was inhibited ata dose of 0.5 µM sodium arsenite (Figure 4A-B). However,no significant growth suppression was observed at a dose of2 µM sodium arsenite in Jurkat cells (Figure 4C).
The dose-response curves of sodium arsenite for S1T and MT2cells were compared with that for Jurkat cells. As shown inFigure 4D, MT2 and S1T cells were more sensitive to sodium arsenitethan Jurkat cells. IC₅₀ values (the concentrations of sodiumarsenite that inhibit 50% of cell growth) for MT2, S1T, andJurkat cells were 2.17 µM ± 0.33 µM, 1.99µM ± 0.03 µM, and 10.54 µM ±0.17 µM, respectively. These results suggest that theATL cell lines MT2 and S1T are sensitive to sodium arseniteeven at low concentrations, and the suppression of survivinexpression is, at least in part, involved in the growth inhibitionof the ATL cells.
Effects of sodium arsenite on apoptosis
To investigate whether the inhibition of cell proliferationwas due to enhanced apoptosis, the proportion of sub-G₁ fractionwas investigated in the presence of 0, 1, 2, 5, and 10 µMsodium arsenite for 1, 2, and 3 days. Sodium arsenite at 1 µMdid not increase the proportion of sub-G₁ fraction, but theproportion of sub-G₁ fraction both dose- and time-dependentlyincreased at 2, 5, and 10 µM in MT2 and S1T cells (Figure 5A-B).However, the increase in the proportion of the sub-G₁ fractionof Jurkat cells treated with the same concentrations of sodiumarsenite was less than that of the ATL cells (Figure 5C). Sub-G₁fraction in MT2 and S1T cells treated with various concentrationsof sodium arsenite for 3 days was significantly higher thanthat in Jurkat cells (P < .01) (Figure 5D). This result suggeststhat sodium arsenite inhibits the growth of ATL cells by inducingapoptosis.
Effects of sodium arsenite on caspases activation in ATL cells
Survivin was shown to bind directly with caspase-3 to inhibitthe caspase activity in human cells exposed to apoptotic stimuli.We investigated whether caspases-3 are activated in ATL cellsby treatment with sodium arsenite. As shown in Figure 6, thecaspases-3 activity increased in MT2 (Figure 6A) and S1T (Figure 6B)cells treated with 2 and 5 µM of sodium arsenite. Theincreased cleavage of PARP was also detected in MT2 and S1Tcells treated with sodium arsenite (Figure 3A). These resultsindicate that the down-regulation of survivin by sodium arsenitethus causes caspase-3–dependent cell death.

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Figure 2.. Protein expression of survivin in ATL. Whole-cell lysates (50 µg protein) from patients with ATL were separated by 12.5% SDS-PAGE and then transferred to a PVDF membrane. The transferred proteins were reacted with antibody against survivin (A) as described in "Patients, materials, and methods." *Concentrations of survivin protein and mRNA are expressed relative to the survivin protein and mRNA levels in control normal cells, which were assigned values of 1. (B) A comparison between the survivin mRNA level (y-axis) and the protein expression level (x-axis) in 17 patients with ATL. The survivin mRNA level correlated with the protein level (r = 0.516, P = .033).

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Figure 3.. The effects of sodium arsenite on the survivin expression in ATL cells. (A) MT2, S1T, and Jurkat cells were incubated in the presence of 2 or 5 µM arsenic trioxide for 24, 48, or 72 hours. Whole-cell lysates (100 µg protein) were prepared and separated by 12.5% SDS-PAGE and transferred to a PVDF membrane. The transferred proteins were reacted with the antibody against survivin, Bcl-2, or PARP as described in "Patients, materials, and methods." As an internal control, ${alpha}$ -tubulin expression was detected. (B) The quantification of the survivin levels in MT2, S1T, and Jurkat cells. The relative density of the bands for survivin obtained by a densitometric analysis and ${alpha}$ -tubulin was used to normalize the respective intensities. (C) S1T and Jurkat cells were treated with sodium arsenite at the indicated concentration and time. Total RNA was then subjected to RT-PCR using primers specific for the amplification of survivin. $beta$ -actin expression was examined as an internal control to ensure the RNA integrity and proper amplification.

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Figure 4.. Growth inhibition of MT2, S1T, and Jurkat cells by sodium arsenite. Proliferation of MT2 (A), S1T (B), and Jurkat (C) cells in the absence or presence of the indicated concentrations of sodium arsenite was assessed by MTT assay. (D) The sodium arsenite toxicity in MT2, S1T, and Jurkat cells was determined by an MTT assay. The points represent the means of triplicate determinations, while the bars show SD.

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Figure 5.. Effects of sodium arsenite on the proportion of sub-G₁ fraction of MT2, S1T, and Jurkat cells. MT2, S1T, and Jurkat cells were treated with 0, 1, 2, 5, or 10 µM sodium arsenite for 1, 2, or 3 days. The cells were then stained by propidium iodide (PI) and analyzed by flow cytometry. The proportion of sub-G₁ fraction of MT2 (A) and S1T (B) was higher than that of Jurkat cells (C) under the indicated concentrations of sodium arsenite and the indicated time. Each column and bar represents the mean ± SD of 3 independent experiments. (D) The sub-G₁ fraction of MT2, S1T, and Jurkat cells treated with sodium arsenite for 3 days was compared. Each column and bar represents the mean ± SD of 3 independent experiments. *P < .01.

Decreased expression of survivin through the surpression of NF- ${kappa}$ B activity by sodium arsenite
NF- ${kappa}$ B is known to be constitutively activated in ATL. Eithera Tax-dependent or Tax-independent mechanism of activation ofthe NF- ${kappa}$ B pathway is crucial for the proliferation of malignantcells, protection from apoptosis, and drug resistance in ATL.Tax regulates the expression of survivin through NF- ${kappa}$ B pathway,and the combination of As₂O₃ and IFN- ${alpha}$ decreases the activationof NF- ${kappa}$ B in ATL cells. We therefore investigated the levels ofnuclear p50 and p65 in ATL cells treated with sodium arsenite.As shown in Figure 7A, sodium arsenite increased the level ofI ${kappa}$ B- ${alpha}$ in MT2 cells. p50 and p65 in the nucleus of MT2 cells wasdecreased by sodium arsenite in a dose- and time-dependent manner.Cytosolic and nuclear survivin decreased in accordance withthe decrease of nuclear p50 and p65. Although no significantdecrease of p50 was seen in the nuclei of S1T cells, p65 inthe nuclei dose-dependently decreased by sodium arsenite (Figure 7B).These results suggest that sodium arsenite suppress the expressionof survivin by preventing I ${kappa}$ B- ${alpha}$ degradation and the translocationof NF- ${kappa}$ B into the nuclei.
Expression of MRP1 and the resistance to sodium arsenite in Jurkat cells
To elucidate the molecular basis for the difference in sensitivityto sodium arsenite between Jurkat and S1T cells, we examinedthe expression levels of MRP1 in these cells. MRP1 is involvedin arsenite resistance and supposed to transport arsenite conjugatedwith glutathione. As shown in Figure 8A, MRP1 was expressedin both Jurkat and S1T cells, but the expression level of MRP1in Jurkat cells was about 3-fold higher than that in S1T cells.The higher molecular weight of MRP1 in S1T cells might be causedby a variation in glycosylation of MRP1 in the cells.

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Figure 6.. The activities of caspase-3 in MT2 and S1T cells in the absence or presence of sodium arsenite. The caspase-3 activity was measured in the cell lysates using the specific substrate Ac-DEVD-MCA. The data are expressed in arbitrary units. Each value represents the mean of 3 independent experiments. Bars indicate SD. *P < .01.

As shown in Figure 8B, Jurkat cells were about 4-fold more resistantto sodium arsenite than S1T cells (IC₅₀ values of S1T and Jurkatcells for sodium arsenite were 1.99 µM ± 0.03 µMand 9.73 µM ± 0.71 µM, respectively). Aninhibitor of MRP1, AG-A alone had no cytotoxic effect at 30µM and decreased the IC₅₀ value of Jurkat cells for sodiumarsenite to 4.03 µM ± 0.04 µM. A specificinhibitor of MRP1, MK571 at 30 µM completely abolishedthe difference in sensitivity to sodium arsenite between the2 cell lines. These findings suggest that the difference insensitivity to sodium arsenite between Jurkat and S1T cellsis attributed to the different expression levels of MRP1 inthese cells.

   Discussion

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Patients with acute- or lymphoma-type ATL have a poor outcome,with a median survival of about 6 months for acute-type and10 months for lymphoma-type; the expected 4-year survival isonly about 5%. Combination chemotherapy regimens, especiallythose for the treatment of aggressive non-Hodgkin lymphoma oracute lymphoblastic leukemia, have little effect on ATL. Thepoor outcome might be due to multidrug resistance in ATL cells.Overexpression of P-gp, MRP-1, and LRP tend to be common featuresof the malignant cells, and they confer intrinsic and acquireddrug resistance on the cells. Another important mechanism ofthe resistance to apoptosis-inducing anticancer agents is thefailure to activate apoptosis. Members of the IAP family arealso overexpressed in many tumors and leukemia, and they alsoinhibit apoptosis. In order to find out the specific targetfor ATL therapy, we investigated the expression levels of themembers of the IAP family, the survivin gene, IAP1, IAP2, andXIAP, in ATL cells from patients using real-time PCR or RT-PCR.Among them, survivin alone was overexpressed in ATL, especiallyin acute-type ATL. The expression level of survivin in poorPS was higher than that in good PS.

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Figure 7.. The effect of sodium arsenite on the levels of I ${kappa}$ B- ${alpha}$ , NF- ${kappa}$ B, and survivin in nuclear and cytosolic fraction from MT2 and S1T cells. (A) MT2 cells were treated with sodium arsenite at the indicated concentrations; nuclear and cytosolic fractions were prepared at the indicated time. Nuclear protein (50 µg) was subjected to Western blotting using the antibody against p50, p65, or survivin. Cytoplasmic fraction (100 µg of protein) was subjected to Western blotting using the specific antibody against I ${kappa}$ B- ${alpha}$ or survivin. ${alpha}$ -tubulin expression was used as a loading control. NE indicates nuclear extract; CE, cytoplasmic extract. *Nonspecific band. (B) p50 and p65 in the nucleus and cytoplasmic survivin in S1T cells treated with sodium arsenite in the indicated concentration, and time was measured by Western blot as in panel A.

Survivin is broadly expressed in embryonic and fetal organs,²³but it becomes undetectable in most terminally differentiatednormal tissues.²⁴ Survivin was overexpressed in the majorityof human tumor types. In gene-profiling studies, survivin wasidentified as the fourth "transcriptome" expressed in the mostcommon human cancers, but not in normal tissues.²⁵ Retrospectivetrial studies suggest that the expression level of the survivingene contributes to the clinical outcome of tumors, includingan abbreviated overall survival, increased rates of recurrences,resistance to therapy, and reduced apoptotic index.²⁶ Recentstudies using real-time PCR showed that high expression levelsof survivin mRNA were a risk factor for prognosis of ATL inthe clinical setting.¹⁵ These results are consistent with ourresults in this study.
There are some reports regarding the relationship between survivinexpression and sensitivity to anticancer agents. Forced overexpressionof survivin increased the resistance to paclitaxel in prostatecancer cell lines. The inhibition of survivin sensitizes prostatecancer cells to paclitaxel-induced apoptosis through caspase-dependantmechanism in vitro and in vivo.²⁷ Down-regulation of survivinexpression with ribozyme or small interfering RNA (siRNA) increasedsensitivity to topotecan and adriamycin in JR8 melanoma cellline and HL-60/ADR cells.^28,29 We have knocked down survivinin KB-3-1 cells using siRNA and found that the cells with thedecreased level of survivin were more sensitive to doxorubicin,etoposide, and sodium arsenite than were the control KB-3-1cells (data not shown). Survivin is an attractive therapeutictarget in cancer for its differential expression in tumors versusnormal tissues, and for its role in maintaining cancer-cellviability.²⁵ A survivin-based therapy would be effective inremoving the general cell-viability machinery exploited by cancercells and it is also expected to have less side effects sincesurvivin is not detected in most normal tissues. Targeting survivinwith antisense oligonucleotides,²⁶ ribozymes,²⁸ or expressionof dominant-negative mutants³⁰ resulted in caspase-dependentcell death and suppression of tumor growth in vivo. However,it remains difficult to apply these approaches to ATL therapyso far. In this study, we found, for the first time, that trivalentarsenite, sodium arsenite, could down-regulate the expressionof survivin at RNA and protein level in ATL cells. Sodium arsenitemay provide a new avenue to suppressing survivin, which is anattractive target for treatment of patients with ATL.

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Figure 8.. Expression of MRP1 and the resistance to sodium arsenite in Jurkat cells. (A) Crude membranes (100 µg protein) were prepared and separated by 7.5% SDS-PAGE and transferred to a PVDF membrane. The transferred proteins were reacted with an antibody against MRP1 as described in "Patients, materials, and methods." KB/MRP membrane vesicles (10 µg) were used as a positive control. (B) Jurkat and S1T cells were incubated with the indicated concentrations of drugs for 72 hours, and cell viability was determined by the MTT assay. The points represent the means of triplicate determinations, and the bars show SD.

As₂O₃ is very effective in the treatment of APL, which carriesthe t(15;17) translocation involving the RAR- ${alpha}$ and PML genes.³¹As₂O₃ could also induce apoptosis in breast cancer, esophagealcarcinoma, multiple myeloma, and ATL.^32-35 It has recently beenshown that As₂O₃ synergizes with IFN- ${alpha}$ to induce cell-cycle arrestand apoptosis in cells infected with HTLV-1, and in the adultT-cell leukemia and lymphoma cells.³⁶ Our study showed thatsodium arsenite alone could suppress the growth and induce apoptosisin ATL cells. Sodium arsenite suppressed the growth of ATL cellsat low concentrations and induced apoptosis of ATL cells ata relatively high concentration (2 µM), at which the expressionof survivin was down-regulated.
Survivin plays an important role in the suppression of mitochondria-dependentapoptosis by either directly or indirectly inhibiting the activityof caspases. Complexes between survivin and caspase-9,³⁷ caspase-3,or caspase-7³⁸ have been demonstrated. Survivin has also beenshown to be associated with Smac/DIABLO,³⁹ a proapoptotic proteinthat is released from mitochondria and it prevents the inhibitoryeffect of IAPs on caspase activation. Moreover, apoptosis inducedby dominant-negative survivin mutants have the characteristicsof mitochondria-dependent apoptosis with cytochrome c releaseand caspase-3 activation.⁴⁰ These findings suggest that survivinprotects apoptosis by interacting with Smac/DIABLO and caspase-9.In the present study, caspase-3 was activated by sodium arsenite.It is probable that sodium arsenite induced mitochondria-dependentapoptosis by decreasing the expression level of survivin inATL cells.
NF- ${kappa}$ B is known to be constitutively activated in ATL. The Tax-dependentor Tax-independent activation of the NF- ${kappa}$ B pathway is crucialfor proliferation, protection from apoptosis, and drug resistancein adult T-cell leukemia and lymphoma. The most common p50-RelA(p65) dimer, "specifically" known as NF- ${kappa}$ B, is more abundantand controls the expression of more genes than any other heterodimersor homodimers. NF- ${kappa}$ B exists as an inactive cytoplasmic complex,predominantly made up of p50-p65, and bound to I ${kappa}$ B- ${alpha}$ , an inhibitoryprotein of the NF- ${kappa}$ B. Recently, El-Sabban et al⁴¹ showed thatIFN- ${alpha}$ /As₂O₃ treatment significantly, and As₂O₃ alone slightlydecreased the expression of the viral transactivator proteinTax and repressed the activation of NF- ${kappa}$ B pathway. As₂O₃ inducedapoptosis of HL-60 cells by repressing the constitutive activationof NF- ${kappa}$ B.⁴² Moreover, Tax induced survivin expression throughNF- ${kappa}$ B pathway.⁴³ p50 and RelB were bound to the NF- ${kappa}$ B bindingsite in the survivin promoter between –354 and –345.⁴³Tax transactivated the survivin promoter through this NF- ${kappa}$ B bindingsite. Our results showed that the level of p65 and p50 in nucleiwas decreased, while the level of cytoplasmic I ${kappa}$ B- ${alpha}$ was increasedby treatment with sodium arsenite in Tax-expressing MT2 cells.This was consistent with the studies of El-Sabban et al⁴¹ andKawakami et al.⁴³ The NF- ${kappa}$ B activity in the cells that were notinfected with HTLV-1 was also repressed by As₂O₃.⁴² In accordancewith this report, we found that sodium arsenite down-regulatedthe expression of survivin through the inhibition of NF- ${kappa}$ B pathwayin S1T cells that did not expess Tax. Sodium arsenite mightsuppress the NF- ${kappa}$ B activity by repressing the p65 translocationto nuclei, but not through Tax.
Sodium arsenite down-regulated the expression of survivin, butnot of Bcl-2. Since there are a number of genes besides survivinand Bcl-2 that are up-regulated by NF- ${kappa}$ B and involved in facilitatingtumor cell survival,^44,45 further study is needed to elucidatewhether the down-regulation of these genes is also involvedin apoptosis and decreased cell growth of ATL cells caused bysodium arsenite.
In this study, the concentration of sodium arsenite requiredto inhibit the growth of ATL cells in vitro was more than 0.5µM and the concentration required to induce apoptosiswas more than 2 µM. These concentrations appear to bebeneficial and safe for clinical use in patients with ATL. Theplasma arsenic rapidly reached a mean maximum serum level of6.85 µM (range, 5.54-7.30 µM) at 4 hours after intravenousinjection of 10 mg As₂O₃.⁴⁶ A recent phase 2 trial in 7 patientswith a relapsed or refractory ATL has shown that the combinationof IFN- ${alpha}$ and As₂O₃ is a hopeful therapy for ATL.⁴⁷ These preliminaryresults highlight that the treatment of ATL with As₂O₃ and IFN- ${alpha}$ is feasible and has a clear antileukemic effect, even in patientswith refractory disease. Further study is needed to clarifywhether the combination of arsenite and IFN- ${alpha}$ can down-regulatesurvivin more effectively, and whether arsenite can enhancethe sensitivity of ATL cells to conventional anticancer agents.
T-cell leukemia Jurkat cells, which were used as a control,were more resistant to sodium arsenite than ATL cells. MRP1is a member of the ATP binding cassette (ABC) superfamily oftransport proteins and is involved in arsenite resistance. Wehave previously demonstrated the clinical significance of MRP1expression and that high MRP1 expression correlated with shortsurvival in patients with acute-type and lymphoma-type ATL.⁹The expression level of MRP1 in Jurkat cells was about 3-foldhigher than that in S1T cells, and MK571, a specific inhibitorof MRP1, abolished the difference in sensitivity to sodium arsenitebetween the 2 cell lines. Since MRP1 transported inorganic arsenicas a tri–glutathione (GSH) conjugate,⁴⁸ we examined theGSH level in the cells and found that the level of GSH in Jurkatcells was similar to that in S1T cells (data not shown). Thesefindings suggested that MRP1, at least in part, might be responsiblefor the decreased sensitivity to sodium arsenite of Jurkat cells.
In this study, we proved for the first time that arsenite coulddown-regulate survivin by repressing NF- ${kappa}$ B activation in ATLcells regardless of the Tax expression. Our findings providea rational basis for the new therapy for ATL using arsenite.

   Acknowledgements

We thank Ms Etsuko Sudou for excellent technical assistanceand Ms Hiromi Kakura for valuable secretarial assistance.

   Footnotes

Submitted August 29, 2005; accepted February 3, 2006.
Prepublished online as Blood First Edition Paper, February 23,2006; DOI 10.1182/blood-2005-08-3423.

Supported by a grant-in-aid from the Ministry of Education,Culture, Sports, Science and Technology, and grants from theJapan-China Medical Association.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

Reprints: Shin-ichi Akiyama, Department of Molecular Oncology, Graduate School of Medical & Dental Sciences, Kagoshima University, 8-35-1, Sakuragaoka, Kagoshima 890-8520, Japan; e-mail: akiyamas{at}m3.kufm.kagoshima-u.ac.jp.

   References

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

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  Copyright © 2006 by American Society of Hematology         Online ISSN: 1528-0020





	Copyright © 2006 by American Society of Hematology Online ISSN: 1528-0020