From the Division of Nephrology-Hypertension and the
§ Program in Molecular Pathology, Department of Medicine,
University of California San Diego and Veterans Affairs Medical Center,
La Jolla, California 92161, and the
Jikei University School of
Medicine, Department of Biochemistry II, Minato-ku, Tokyo 105, Japan
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ABSTRACT |
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Polyamines are required for entry and progression of the cell cycle. As such, augmentation of polyamine levels is essential for cellular transformation. Polyamines are autoregulated through induction of antizyme, which represses both the rate-limiting polyamine biosynthetic enzyme ornithine decarboxylase and cellular polyamine transport. In the present study we demonstrate that agmatine, a metabolite of arginine via arginine decarboxylase (an arginine pathway distinct from that of the classical polyamines), also serves the dual regulatory functions of suppressing polyamine biosynthesis and cellular polyamine uptake through induction of antizyme. The capacity of agmatine to induce antizyme is demonstrated by: (a) an agmatine-dependent translational frameshift of antizyme mRNA to produce a full-length protein and (b) suppression of agmatine-dependent inhibitory activity by either anti-antizyme IgG or antizyme inhibitor. Furthermore, agmatine administration depletes intracellular polyamine levels to suppress cellular proliferation in a transformed cell line. This suppression is reversible with polyamine supplementation. We propose a novel regulatory pathway in which agmatine acts as an antiproliferative molecule and potential tumor suppressor by restricting the cellular polyamine supply required to support growth.
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INTRODUCTION |
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Polyamines (putrescine, spermidine, and spermine) are required for DNA replication, proliferation, and cell homeostasis (1-3). Ornithine decarboxylase (ODC)1 is the first rate-limiting enzyme of polyamine biosynthesis and one of the most highly regulated eukaryotic enzymes. Cellular polyamine transporters are stimulated by many of the same factors that induce ODC activity, and similarly, enhanced cellular polyamine uptake occurs both in normal but rapidly proliferating cells (4) and in tumor cell lines (5-8). Cells in vivo can acquire polyamines released into the circulation by other cells, dietary sources, and gut flora. Polyamines have been demonstrated to play an important role in the transformation process. Conversely, polyamine depletion results in growth arrest (9, 10).
Intracellular polyamine concentrations are autoregulated by the induction of the protein antizyme (11). Antizyme is the only known endogenous protein that binds to ODC, inhibiting activity and accelerating its degradation (12). In addition to inhibiting polyamine biosynthesis, antizyme has recently been shown to concurrently suppress polyamine transporter(s) (13, 14). Pharmacological inhibition of ODC activity, however, has been shown to result in compensatory cellular polyamine uptake (6). Beneficial therapeutic intervention must therefore address both polyamine transport as well as biosynthesis (for review see Ref. 15).
The metabolism of arginine to agmatine by ADC has only recently been demonstrated in mammals (16). As agmatine and polyamines are structurally analogous polycationic molecules derived from distinct arginine-dependent pathways (6), we speculated that the ADC metabolite agmatine may play a role in regulating intracellular polyamines. Herein we report concurrent suppression of both polyamine biosynthesis and transport by agmatine. This occurs primarily via induction of antizyme and results in attenuated proliferation in a transformed cell line.
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EXPERIMENTAL PROCEDURES |
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Materials-- All chemicals were purchased from Sigma unless otherwise stated. We were unable to detect impurities by HPLC analysis in agmatine purchased from Aldrich. Sigma agmatine was found to have 3-8% impurities.
Cells and Cell Cultures-- All cell lines were from American Type Culture Collection except MCT (mouse kidney proximal tubule) (17), Ras-3T3 (Ras transformed NIH-3T3 fibroblast) (18), mMC (mouse glomerular mesangial) (19), JS-1 (human Schwann tumor) (20), and ENDO (rat glomerular endothelial) (21). Cells were maintained in culture in Dulbecco's modified Eagle's medium (Life Technologies, Inc.) supplemented with 5% fetal calf serum (HyClone Laboratories). Experiments were performed when incubation of cell cultures in 10-cm dishes reached ~80-95% confluence, unless otherwise noted.
ODC Activity-- Cells were washed and resuspended in ODC reaction buffer (10 mM Tris, pH 7.4, 2.5 mM dithiothreitol, 0.3 mM pyridoxal-5-phosphate, 0.1 mM EDTA) and homogenized by polytron. The homogenate was centrifuged at 30,000 × g for 40 min, and the supernatant was assayed for ODC activity as described (22).
Transport Studies--
Cells were cultured (6-well plates) in
the absence or presence of 1 mM agmatine for the indicated
times (see Fig. 2). Cells were then washed three times with
phosphate-buffered saline prior to a 15-min incubation with 0.5 µCi
ml1 12.5 nM [3H]putrescine (NEN
Life Science Products) in Dulbecco's modified Eagle's medium. Five
cold washes of phosphate-buffered saline terminated the incorporation.
Cells were lysed with 1 N NaOH and counted in a
scintillation counter.
Antizyme Frameshifting-- Fusion antizyme mRNAs were used in a reticulocyte lysate assay as described previously (11). Frameshift efficiencies were calculated from the radioactivities of frameshift and termination bands with a BAS 2000 image analyzer.
Antizyme Antibody and Antizyme Inhibitor Assays-- MCT cells were incubated with 5 mM agmatine and 1 mM aminoguanidine for 24 h. Aminoguanidine was used to inhibit serum diamine oxidase, an enzyme that metabolizes agmatine. Preparation of ODC, anti-antizyme antibody, and antizyme inhibitor methodology were as described previously (23).
Proliferation Assays--
15,000 (see Fig. 4A) or
5000 (see Fig. 4D) MCT cells/well on a 96-well plate were
incubated in the absence or presence of 1 mM agmatine and
0.05 mM putrescine for 24 or 48 h as indicated in the
figures. [3H]Thymidine (1 µCi/well) was added 16 h
prior to harvesting in an automated multiwell harvester and scintillation counting. Cell counting (see Fig. 4B) was
performed by plating 50,000 MCT cells/well of a 24-well plate in the
absence or presence of agmatine (concentrations indicated in the figure
legend). Cells were collected and counted in a hemocytometer using
trypan blue exclusion to identify viable cells.
Conversion of Agmatine to Polyamines-- MCT cells (10-cm plate) were incubated with [3H]agmatine (10 µCi/10 ml Dulbecco's modified Eagle's medium + 5% fetal calf serum; American Radiolabeled Chemicals Inc.) for a 2-h incubation period. Cells were washed, collected, scraped, lysed, and prepared for HPLC as described below.
Determination of Intracellular Polyamine Levels-- Cellular extracts were deproteinated prior to derivatization (AccQ-Fluor kit, Waters Corp.) and HPLC elution on a C18 reverse phase column (ODS Hypersil 3 µm). The HPLC flow rate was 0.5 ml/min, and the elution gradient was as follows: 5% A 0-3 min, 7% A 3-10 min, 7-30% a 10-30 min, and 30-50% A 30-35 min. Buffer A was supplied in the AccQ-Fluor kit, and buffer B was HPLC grade acetonitrile. Polyamines were detected by fluorescence as per AccQ-Fluor kit instructions (see Fig. 4C) or radioactivity assessed for [3H]agmatine conversion (not shown).
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RESULTS |
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Agmatine Suppresses ODC Activity-- Because the kidney is a principal site of ADC activity, we performed these experiments in a mouse kidney proximal tubule cell line, MCT (17). This transformed cell line demonstrates elevated constitutive ODC activity and diminished ADC activity compared with freshly isolated proximal tubule cells.2 These aspects make the MCT cell line an appropriate model system for observing the effects of agmatine supplementation on ODC activity and intracellular polyamine levels. Exogenous agmatine administration to MCT cells for 18 h resulted in a concentration-dependent suppression of ODC activity (Fig. 1A). Agmatine was not toxic at these or higher concentrations as determined by trypan blue exclusion. Agmatine purchased from either Aldrich or Sigma yielded comparable results. The effects on ODC activity were evident following a 30-min lag period (Fig. 1B). Because agmatine is distributed by the plasma and can be concentrated in tissues (34), we examined whether its effects are cell type-specific. Fig. 1C demonstrates the efficacy of exogenous agmatine administration for 18 h in suppressing ODC activity in multiple immortalized or transformed cell lines.
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Agmatine Suppresses Polyamine Transport-- The rapid polyamine transport observed in MCT cells as determined by [3H]putrescine uptake is indicative of active polyamine transporters (Fig. 2, 0 h of agmatine preincubation). To determine whether agmatine affects polyamine transporters, cells were preincubated in the presence of agmatine and then shifted to agmatine-free medium containing [3H]putrescine. Extracellular agmatine was removed during the labeled uptake period of this experiment to demonstrate suppression of transporters and avoid potential competitive effects of agmatine with [3H]putrescine (Fig. 2).
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Induction of Antizyme by Agmatine-- Polyamines autoregulate their intracellular concentrations through the induction of antizyme, which suppresses both polyamine biosynthesis and transport. It has been demonstrated that polyamine induction of antizyme is not primarily a transcriptional event but rather occurs by a distinct mechanism of programmed ribosomal frameshifting (11). We utilized a rabbit reticulocyte lysate assay to examine whether agmatine can directly induce a +1 translational frameshift of antizyme mRNA in vitro. These results are depicted in Fig. 3A. The frameshift efficiency, and therefore the effectiveness of producing full-length, functional antizyme by 4 mM agmatine, was comparable with that of 4 mM putrescine and 0.5 mM spermidine. These concentrations of the canonical polyamines represent at or near maximal effective concentrations for this assay as previously established (11). We have found that the effect of agmatine on frameshift efficiencies was dose-dependent (not shown). We next examined whether antizyme induction is required for the effect of agmatine on ODC. Purified ODC enzymatic activity was markedly inhibited in the presence of agmatine-treated (MCT) cell extracts. The ODC inhibitory activity of agmatine-treated cell extracts was precipitated with the anti-antizyme antibody but not with control IgG (Fig. 3B). Furthermore, addition of highly purified antizyme inhibitor (24) also attenuated the inhibitory effect of the cell extracts (Fig. 3B). Together, these results demonstrate that agmatine is capable of inducing antizyme.
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Agmatine Administration Suppresses Proliferation-- Intracellular polyamines are maintained in reserve, allowing passage through several cell cycles before polyamine depletion limits further cell division (25). [3H]Thymidine incorporation in MCT cells exhibited no change between untreated and agmatine-treated cells by 24 h (Fig. 4A). However, by 48 h agmatine-treated cells demonstrated a dramatic inhibition in the rate of DNA synthesis relative to control (Fig. 4A). Decreased cellular proliferation in agmatine-treated cells, as verified by cell counting, was maintained throughout a 10-day experiment (Fig. 4B).
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DISCUSSION |
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Polyamines are required components for both protein and nucleic acid synthesis, and polyamine biosynthesis is regulated throughout the course of the cell cycle (26, 27). Antizyme, through its ability to suppress both the polyamine biosynthetic enzyme ODC and polyamine transporters, is an effective endogenous mechanism for limiting intracellular polyamine levels. This unique, two-pronged negative feedback system of antizyme was thought to be exclusively induced by cellular polyamine accumulation. In this study we demonstrate induction of antizyme by an arginine-dependent pathway distinct from that of polyamine biosynthesis, with resultant suppression of polyamine biosynthesis and transport (Fig. 5).
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Inhibition of polyamine biosynthesis and transport by agmatine resulted in suppression of proliferation in a transformed cell line (Fig. 4, A and B). Recent studies have suggested a correlation of agmatine binding to imidazoline (I2) receptors with the selective inhibition of proliferation of cultured primary vascular smooth muscle cells (28). In our studies, inhibition of ODC activity was demonstrated in membrane-free preparations, which could not be attributed to a receptor-dependent mechanism. Agmatine exerted its maximum effects on proliferation at 1 mM (Fig. 4B). The capacity of agmatine to frameshift antizyme mRNA to produce a full-length protein was also observed at 1 mM. Although maximum frameshift efficiencies were at 4 mM (Fig. 3A), 1 mM may be sufficient to block ODC and polyamine transport causing maximal growth inhibition. Differences between the effect of agmatine in the frameshift and proliferation assays may also reflect differing concentrations of agmatine in the medium and in the cells. We are currently investigating how agmatine is transported and accumulated within the cell. Although we cannot entirely exclude potential nonantizyme-mediated effects by agmatine, antizyme is required for suppression of ODC activity (Fig. 3B). Furthermore, effects on proliferation were shown to be reversed if putrescine was administered concurrently with agmatine (Fig. 4D), thus supporting the premise of cellular polyamine limitation as the inhibitory mechanism. Although this latter result may initially appear inconsistent with the findings of concurrent agmatine inhibition of polyamine transport, it should be noted that inhibition of cellular uptake was neither complete nor immediate, requiring at least 2 h for maximum effect (Fig. 2), allowing cellular putrescine to accumulate in these cells over this period. Our results also demonstrate that agmatine, at doses causing cellular polyamine depletion, does not act as a precursor of the canonical polyamines in terms of supporting cell proliferation (Fig. 4). The findings of this study corroborate earlier studies reaffirming the necessity of polyamines in maintaining a transformed state.
When ODC activity is induced in tissues such as liver and kidney following a hyperplastic or hypertrophic stimulus, there is a concurrent reduction in ADC activity.3 We observed similar reciprocal changes in the transformed proximal tubule cell line, MCT, compared with freshly isolated proximal tubule cells.3 Such correlations suggest a physiologic role for ADC metabolites in the control of cellular proliferation and as potential tumor suppressors. ADC activity could also serve to divert arginine from arginase, thereby limiting substrate for ODC and effectively compounding the effects of agmatine. Targeted gene disruption of ADC would be an important step in further understanding the functional importance of this pathway.
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ACKNOWLEDGEMENTS |
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We thank Drs. E. G. Neilson (MCT and mMC), H. Holthofer (ENDO), A. Mizisin (JS-1), and F. C. White and M. Kamps (Ras-3T3) for kindly donating cell lines.
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FOOTNOTES |
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* This work was supported by National Institutes of Health Grants DK42155, DK28602, HL48108, and T32HL07261, funds from the Medical Research Service Veterans Affairs Central Office, and grants-in-aid from the Ministry of Education, Science and Culture in Japan.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
¶ To whom correspondence should be addressed: UCSD/VAMC, mail code 9111 H, Div. Nephrology-Hypertension, 3350 La Jolla Village Dr., San Diego, CA 92161. Tel.: 619-552-7528; Fax: 619-552-7549; E-mail: jsatriano{at}ucsd.edu.
** National Kidney Foundation Fellow.
Clinical Investigator of Medical Research Service, V.A. Central
Office.
1 The abbreviations used are: ODC, ornithine decarboxylase; ADC, arginine decarboxylase; HPLC, high pressure liquid chromatography.
2 J. Satriano, unpublished observation.
3 J. Satriano, V. Vallon, D. Schwartz, C. J. Kelly, and R. C. Blantz, manuscript in preparation.
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REFERENCES |
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