Intracellular Location of Thymidylate Synthase and Its State of Phosphorylation*

(Received for publication, January 27, 1997)

William A. Samsonoff , James Reston , Mary McKee Dagger , Brigid O'Connor §, John Galivan , Gladys Maley and Frank Maley

From the Wadsworth Center, New York State Department of Health, Empire State Plaza, Albany, New York 12201-0509

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES


ABSTRACT

Thymidylate synthase (TS), an enzyme that is essential for DNA synthesis, was found to be associated mainly with the nucleolar region of H35 rat hepatoma cells, as determined both by immunogold electron microscopy and by autoradiography. In the latter case, the location of TS was established through the use of [6-3H]5-fluorodeoxyuridine, which forms a tight ternary complex of TS with 5-fluorodeoxyuridylate (FdUMP) and 5,10-methylenetetrahydrofolylpolyglutamate within the cell. However, with H35 cells containing 50-100-fold greater amounts of TS than unmodified H35 cells, the enzyme, although still in the nucleus, was located primarily in the cytoplasm as shown by autoradiography and immunohistochemistry. In addition, TS was also present in mitochondrial extracts of both cell lines, as determined by enzyme activity measurements and by ternary complex formation with [32P]FdUMP and 5,10-methylenetetrahydrofolate. Another unique observation is that the enzyme appears to be a phosphoprotein, similar to that found for other proteins associated with cell division and signal transduction. The significance of these findings relative to the role of TS in cell division remains to be determined, but suggest that this enzyme's contribution to the cell cycle may be more complex than believed previously.


INTRODUCTION

Thymidylate synthase (TS, EC 2.1.1.45)1 is a unique enzyme in nature by virtue of the fact that one of the substrates in the reaction, CH2H4PteGlu serves to reductively methylate the second substrate, dUMP, to yield dTMP and H2PteGlu. Because dTMP plays an essential role in the synthesis of DNA, the enzyme has been a chemotherapeutic target since its discovery about 40 years ago (1). The DNA sequences of some 30 different species of TS have been clarified (2) establishing it as one of the most phylogenetically conserved proteins known. X-ray crystal structures for the Lactobacillus casei (3), Escherichia coli (4, 5), and human TSs (6) have been utilized to define the mechanism by which the substrates interact with the enzyme to form product and the nature of the inhibition affected by substrate analogues, as well as to aid in the rational design of potential chemotherapeutic agents (7).

While much is known about the physical and enzymic properties of TS, less is known about how the enzyme is regulated within the cell, its structural location, and its potential interaction with other proteins. Recent studies indicate that this enzyme may be regulated at both the transcriptional (8) and translational levels of synthesis (9), while earlier studies suggested that TS forms multienzyme complexes involved in DNA synthesis both in T-even phage-infected E. coli (10, 11) and eukaryotic cells (12, 13). These findings are compounded further now by the enzyme's apparent association with the nucleolus of the cell and its state of phosphorylation, as will be described in this paper. In addition we will provide evidence that TS may be located also in the mitochondria of cells as has been described recently for a bifunctional dihydrofolate reductase·TS plant enzyme (14) and a dUTPase in HeLa cells (15).

Attempts to establish the intracellular location of TS have been inconclusive since depending on the technique and cells used, TS has been shown to be associated either with the nucleus (16, 17) or the cytoplasm (18, 19). Fluorescent antibody studies by us some 10 years ago using human TS antibody2 indicated that the enzyme was present mainly within the nucleus of the HeLa cell, but could not be confirmed with H35 hepatoma cells. More recently by using a similar technique with yeast the enzyme was shown to be localized to the nuclear periphery (20). To more clearly define the enzyme's location within a eukaryote, we will demonstrate, using immunogold electron microscopy and autoradiography, the nuclear and nucleolar presence of TS in a rat hepatoma (H35) cell line.


MATERIALS AND METHODS

Immunogold Treatment of Cells

The fixation of cells and the labeling procedures used for the localization of the TS antigen after first treating the cells with a purified anti-TS rabbit antibody then with an IgG secondary antibody (goat anti-rabbit antibody conjugated with 5 nm colloidal gold, Janssen Life Sciences, Piscataway, NJ) were essentially as described in the instructions provided by Janssen and by Hechemy et al. (21). The TS antigen was purified to homogeneity (22) and 1 mg injected as an emulsion with Freund's complete adjuvant several times along the midline region of a rabbit's spine. After 2 weeks antibody production was boosted with another 0.5 mg of TS in saline that was injected into the rabbit's hind legs intramuscularly and neck pad. After two more weeks 50 ml of blood was removed and allowed to clot. The TS antibody (IgG) was purified from the rabbit serum by CM-Affi-Gel blue chromatography (Bio-Rad) according to the manufacturer's instructions.

Quantitative Evaluation of Immunogold

Gold particles were counted on electron micrographs (final magnification × 45,000). Cell areas were determined by overlaying each micrograph with a calibrated lattice of known size, and underlying areas were determined for each cell compartment. The density of gold label is defined as the number of gold particles encountered per square micron of surface counted.

Electron Microscopy Autoradiography

H35S (FdUrd-sensitive) and H35R (FdUrd-resistant) cells (6 × 104 in 12 ml of Swim's medium containing 5% human serum 10% fetal bovine serum) were grown for 43 h in 100-mm plates in a CO2 incubator, after which 8 ml of medium was removed from each plate. Folinic acid was added to a final concentration of 100 µM to the remaining 4 ml, while [6-3H]FdUrd (22 Ci/mmol), DuPont NEN) was added to a final concentration of 0.26 µM. The plates were incubated for an additional 4 h, washed three times with media and incubated for 4 h with fresh Swim's media. At the end of this period, the cells were fixed with 2 ml of Trump's fixative for 15 min and washed two additional times with 5 ml of fixative. The plates were then incubated overnight at 40 °C and the cells gently scraped off the Petri dishes and centrifuged, followed by rinsing in 0.1 M sodium cacodylate buffer, pH 7.4. After a secondary fixation for 30 min at room temperature in a solution of 1% osmium tetroxide, 0.1 M cacodylate buffer, pH 7.4, the pellets were embedded in agar, dehydrated in a graded series of ethanol, and embedded in Epon/Oraldite. Sections of 0.1 µm were collected on carbon-coated grids, and autoradiographic emulsions were prepared essentially as described by Caro and van Tubergen (23). Grids were post-stained with uranyl acetate and Reynold's lead citrate (24) and examined in a Zeiss 910 transmission electron microscope at 100 kv.

Mitochondrial Isolation and Ternary Complex Formation

H35S and H35R cells were grown in Swim's medium to about 90% confluence in one to three roller bottles and harvested with 0.05% trypsin, 0.02% versene. The cells were added to an equal volume of Swim's medium and centrifuged for 5 min at 1000 rpm followed by washing with 20 ml of phosphate-buffered saline. The centrifuged cells were resuspended in 4 ml of isolation buffer (230 mM mannitol, 70 mM sucrose, 0.5 mM EGTA, 0.5% bovine serum albumin, and 10 mM Hepes, pH 7.4). The cells were then homogenized and centrifuged in a 15-ml plastic centrifuge tube at 1000 × g for 10 min at 4 °C using a Sorvall GLC-2B centrifuge. The supernatant fraction after transferring to another tube was recentrifuged at 20,000 × g in a Sorvall RC-2B centrifuge for 15 min. The pellet was resuspended in 5 ml of isolation buffer and recentrifuged. Alternatively, mitochondria were purified by isopycnic centrifugation as described by Rickwood et al. (25). In either case, the final mitochondrial pellet was suspended in 1 ml of STE (100 mM NaCl, 10 mM EDTA, 50 mM Tris-HCl, pH 7.4), and centrifuged in an Eppendorf centrifuge at 14,000 rpm for 10 min at 4 °C. The pellet was resuspended in 150 µl of STE and sonicated for 7 s in an ethanol/ice bath and centrifuged as above. Alternatively, the mitochondria were suspended in cold water and after lysis the membranous fraction was centrifuged, as above, in an Eppendorf centrifuge. Ternary complexes containing [32P]FdUMP were obtained by a slight modification of the procedure of Maley et al. (26) as follows: to 8 µl of H35R cell extract, mitochondrial supernatant fraction, or purified recombinant rat TS (27) was added 1 µl of 50 mM MgCl2, 3 µl of a 1.6 mM (R,S)-CH2H4PteGlu solution (26), 3 µl of 0.1 M cytidine 5'-monophosphate, and 5 µl of [32P]FdUMP (1.1 × 106 dpm). After incubating at room temperature for 30 min the reactions were stopped with an equal volume of SDS-loading buffer and boiled for 3 min. Half of the sample was subjected to 12.5% SDS-PAGE for 1 h at 180 volts. The gel was dried and exposed to Kodak X-Omat x-ray film for 15-60 min at room temperature.

Labeling of H35 Cells with 32Pi and TS Isolation

H35R rat hepatoma cells were grown in Swim's medium as above on 60-mm tissue culture plates for 24 h prior to labeling. The cells, which were at 80% confluence at this time, were washed 3 × with 2 ml of phosphate-free Dulbecco's modified Eagle's medium (DMEM) and were then incubated with 2 ml of phosphate-free DMEM, at 37 °C in a CO2 incubator for 1 h. The media were replaced with 1.5 ml of phosphate-free DMEM containing 1% fetal bovine serum (1.5 ml/plate) and 120 µCi of 32Pi, which was incubated in a 37 °C CO2 incubator for 4 h. The plates were washed four times with 2 ml of phosphate-buffered saline and the cells lysed in 0.5 ml of a modified RIPA (50 mM Tris-HCl, pH 7.5, 150 mM NaCl, 0.1% SDS, 1% Triton X-100, 2 mM phenylmethanesulfonyl fluoride, 10 µg/ml aprotinin, 10 µg/ml leupeptin, 10 mM NaF, 0.1 mM Na3VO4) on ice with gentle rocking for 30 min. The lysates were transferred to 1.5-ml Eppendorf tubes, which were centrifuged at 14,000 rpm for 10 min at 4 °C in an Eppendorf 5415 centrifuge. The supernatant fractions were transferred to fresh Eppendorf tubes, to which were added 25 µl of protein A-Sepharose (10% slurry in modified RIPA), incubated for 1 h, and centrifuged for 10 min at 14,000 rpm at 4 °C. To the supernatant fractions transferred to fresh tubes was added 10 µl of rabbit anti-rat TS serum, and after incubation on ice for 1 h, 25 µl of protein A-Sepharose beads was added to each tube, which were shaken for 1 h. The beads were centrifuged and washed four times with 200 µl of modified RIPA, then resuspended in 20 µl of SDS-loading buffer containing 2-mercaptoethanol and boiled for 5 min. Each supernatant fraction (10 µl) was loaded onto a 12.5% SDS-PAGE gel, and after 1 h at 175 volts, the gel was stained with Coomassie Blue, followed by destaining and drying onto Whatman No. 3MM paper. The dried gel was exposed to Kodak X-Omat film for 1-3 days at -70 °C using an enhancing screen.

In Vitro Phosphorylation of Thymidylate Synthase

H35R cells were grown for 24 h as described above. The medium was removed, and the plates were rinsed with a buffer solution containing 0.25 M sucrose, 50 mM Tris-Cl, pH 7.4, and 5 mM MgSO4. The cells from six plates were scraped off with the above buffer, but containing 2 mM phenylmethanesulfonyl fluoride, 10 µg/ml aprotinin, 10 µg/ml leupeptin, 10 mM NaF, and 0.1 mM sodium vanadate, and sonicated for 10 s in an ethanol/ice bath. Aliquots of the sonicates (0.28 ml) were added to each Eppendorf tube with 20 µCi of [gamma -32P]ATP. The incubations, conducted at room temperature, were terminated at various times by the addition of 1 µmol of cold ATP, which so diluted the [gamma -32P]ATP to effectively end the measurable incorporation of labeled phosphate into the protein acceptors. The cellular debris was centrifuged for 10 min at 14,000 rpm in an Eppendorf centrifuge at 4 °C. The supernatant fractions were transferred to fresh Eppendorf tubes, where they were treated with 7 µl of rabbit anti-rat TS serum for 1 h on ice, followed by 15 µl of protein A-Sepharose (Pharmacia Biotech Inc.) for 1 h on ice.


RESULTS

Evidence for the Nuclear Presence of TS

Earlier studies by us using fluorescent guinea pig antibody to HeLa cell TS, as well as immunogold electron microscopy, strongly implicated the association of TS with the nucleus.2 However, attempts to repeat these studies by exposing H35S cells to rat TS fluorescent antibody were inconclusive, mainly due to the difference in membrane permeability of the two cell lines. Since we had available to us much larger quantities of rat TS (22) than HeLa TS for the preparation of antibody, we explored the use of immunogold secondary antibody (goat anti-rabbit IgG) fixation to rabbit anti-rat TS antibody following treatment of H35S cells with the latter.

Fig. 1A reveals that little or no gold particles could be detected when the cells were exposed to nonspecific IgG. In contrast, when the H35S cells were treated with purified anti-TS IgG, a major share of the immunogold particles were found to be localized to the nucleus (Fig. 1B) with most of the particles being associated with the nucleolus (Fig. 1C). The nuclear distribution of the particles could be partially blocked if the antibody was first treated with H35 TS, verifying the specificity of the reaction (Fig. 2). That the nuclear (nucleolar) association of the TS antibody was not a random event was verified by measuring a statistically significant number of immunogold particles in a large number of areas inside, as well as outside of the cell (Fig. 2). However, because of the uniqueness of these findings and the possibility that the results of Fig. 1 were a consequence of the technology employed and did not truly represent what was observed, a more direct approach was sought, that of autoradiography.


Fig. 1. Location of TS in H35 cells using immunogold labeled secondary antibody. H35S cells, fixed for electron microscopy, were treated with prebleed rabbit IgG (A); anti-TS IgG, with the boxed region encompassing the nucleolus (B), and the nucleolar region in B, enlarged about 2.5 times (C).
[View Larger Version of this Image (127K GIF file)]


Fig. 2. Distribution of TS-directed immunogold particles in H35S cells, which is typified by the results in Fig. 1. The density of gold particles in each cell compartment was determined as described under "Materials and Methods." A minimum of 20 cells was counted in each of five experiments, with the standard deviations given by the error bars.
[View Larger Version of this Image (28K GIF file)]

Nuclear-Nucleolar Location of TS via Autoradiography

To unambiguously confirm the immunogold results a biochemical approach was taken, that of exposing the cells to [6-3H]FdUrd and leucovorin, which in the case of the former compound will be converted to [6-3H]FdUMP once in the cell, while the latter is metabolized to 5,10-methylenetetrahydrofolylpolyglutamate. Both compounds then combine with TS to form a tight ternary complex, which is the basis, in most cases, of the chemotherapeutic response to fluorouracil or FdUrd (28). Although leucovorin was added to make certain the folate pool was not limiting, it was found in most instances that the concentration of this pool was adequate. After thorough washing of the cells to remove unbound [6-3H]FdUrd, it was hoped that the location of the TS complex within the cell would be revealed on autoradiography. As shown in Fig. 3A, most of the labeled ternary complex resided in the nucleus of the H35S cells and, similar to the immunogold electron micrographs of Fig. 1, appears to be localized primarily to the nucleolar region. Since the possibility existed that the nucleolar presence of the label was due to the breakdown of FdUrd to fluorouracil and its subsequent incorporation into nucleolar RNA, this experiment was repeated in the presence of a 100-fold excess of unlabeled uracil or deoxyuridine. No dilution of the radioactivity was apparent, indicating that incorporation into RNA was not the source of the label within the cell (data not shown). In addition, SDS-PAGE of H35S and H35R cells treated as described in Fig. 3, followed by autoradiography, revealed that all of the radioactivity was associated with the FdUMP·TS ternary complex with none of the label at the origin, which would be indicative of RNA (data not presented).


Fig. 3. Location of [6-3H]FdUMP·TS·CH2H4PteGlu ternary complex in H35S cells (A) and H35R cells (B). The procedure employed is described under "Materials and Methods."
[View Larger Version of this Image (73K GIF file)]

In an attempt to increase the immunogold particles and labeled ternary complexes within the cell, an FdUrd-resistant cell line (H35R) that contained 50-100-fold greater levels of TS than the FdUrd-sensitive line (H35S) (22) was employed. In contrast to the findings with the H35S cell line (Fig. 3A), the H35R cells revealed that although some radioactivity was in the nucleus, most of the ternary complex was spread throughout the cytoplasm (Fig. 3B). It is of interest to note that the morphology of the two cell lines differed in that the H35R cells are larger than the H35S cells. It should be emphasized though that the level of TS found in dividing cells in culture and in tissues, both normal and neoplastic, is more like that found in H35S than H35R, that is quite low. As in the case of the immunogold studies, these findings were reproduced in numerous autoradiographs where it was possible to easily distinguish between H35S and H35R cells.

Mitochondrial Presence of Thymidylate Synthase

As a consequence of recent findings suggesting the presence of TS in plant mitochondria as a dihydrofolate reductase·TS bifunctional complex (14) and the presence of a dUTPase in rat liver mitochondria, we extensively purified mitochondria from H35S and H35R cells by the same procedure used for dUTPase (15) and found considerable TS activity in the latter relative to the former using a sensitive tritium release assay (29). To confirm the assay, we incubated mitochondrial extracts with [32P] FdUMP and CH2H4PteGlu, and as shown in Fig. 4, mitochondria do indeed contain TS as evidenced by their ability to form a ternary complex. To demonstrate that the enzyme was not associated with the mitochondrial membranes, lysis of the mitochondria in water followed by centrifugation to remove the membranous fraction revealed TS to be present mainly in the supernatant fraction. As in the case of the dUTPase (15), TS appears to be imported, since evidence for a sequence in mitochondrial DNA, which hybridizes to the rat TS cDNA could not be detected, although it is possible that the mitochondrial TS sequence, if it does exist, is sufficiently different from the genomic DNA that it does not hybridize to mitochondrial TS DNA. However, based on the high degree of evolutionary homology of the various TSs described to date (2), this would appear to be unlikely.


Fig. 4. Ternary complex formation as evidence for the presence of TS in rat liver mitochondria following SDS-PAGE and autoradiography. Lane 1, H35R cell extract; lane 2, mitochondrial supernatant fraction after sonation of mitochondria isolated from H35R cells; lane 3, purified recombinant rat TS. The formation of the [32P] FdUMP ternary complexes is described under "Materials and Methods."
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Evidence That Thymidylate Synthase Is Phosphorylated

In view of the fact that many proteins, in particularly those associated with the regulation of cell division are phosphorylated (30), we examined this possibility for TS. H35R cells were incubated with 32Pi, and the TS present within the cells was extracted with antibody specific for rat TS using protein A. As shown in the SDS-PAGE autoradiogram (Fig. 5), the TS extracted from the cells was labeled with 32Pi (Fig. 5, lane 2), but no label was present in this region when nonspecific serum was used (Fig. 5, lane 1). In the presence of increasing amounts of okadaic acid, an inhibitor of phosphoserine/phosphothreonine phosphatases, the amount of label associated with TS appeared to increase (Fig. 5, lanes 3 and 4), while the addition of staurosporine, a protein kinase inhibitor, blocked TS labeling completely (Fig. 5, lane 5).


Fig. 5. In situ labeling of TS with 32Pi. The results represented in each lane are as follows: lane 1, cell extracts to which was added nonspecific rabbit serum prior to protein A beads; lane 2, the same as lane 1 but containing serum from a rabbit immunized to rat TS; lane 3, same as lane 2, but the cells were incubated with 40 nM okadaic acid for 2 h; lane 4, same as lane 2, but the cells were incubated with 100 nM okadaic acid; lane 5, same as lane 2, but the cells were incubated with 2 nM staurosporine. The procedure employed for the immunoaffinity isolation of H35 TS is described under "Materials and Methods."
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Phosphorylation of Thymidylate Synthase in Vitro

To verify the results in Fig. 5, we determined if the apparent phosphorylation of TS that was occurring in situ could be measured in cellular extracts. It is apparent from the results in Fig. 6 that a kinase is present in the extracts that transferred 32P from [gamma -32P]ATP to a specific site on the TS present in the extracts. For the purpose of measuring potential kinase activity, we used H35R cells rather than H35S cells, since a much greater quantity of TS is present in extracts from these cells, which did not require the addition of TS as a substrate. To reduce the background and to basically terminate the transfer of 32P, a large excess of cold ATP was added at the indicated times in Fig. 6, which appeared to have the desired effect of ending measurable incorporation of radioactivity into protein. It is clear from the results in Fig. 6 that the transfer is time-dependent. Preliminary results indicate that at least one serine in the enzyme is phosphorylated.


Fig. 6. In vitro labeling of TS in cell extracts with [gamma 32P]ATP. The times at which the reactions were quenched by the addition of a great excess of cold ATP are as follows: 0 min (lane 1), 5 min (lane 2), 20 min (lane 3), 60 min (lane 4), 90 min (lane 5) and 150 min (lane 6). The methodology employed is described under "Materials and Methods."
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DISCUSSION

Numerous proteins, particularly those associated with cell division, have been found in the past decade to be associated with the nucleus. Even before these more recent developments, TS was reported to be present in the nucleus of eukaryotic cells as part of a "replitase" complex consisting of enzymes involved mainly in providing substrates for DNA synthesis (17), although the cytoplasmic location of TS has also been reported (18, 19). We have shown in this paper by both immunogold labeling and autoradiography that not only is TS associated with the nucleus of H35S cells, it is located predominantly in the nucleolus. It was hoped that cells selected for their resistance to FdUrd (H35R), as a result of a 50-100-fold increase in TS, would show an even greater nuclear content of TS. However, much to our surprise, when these cells were examined by autoradiography to locate TS by means of ternary complex formation, most of the TS was found in the cytoplasm, although some was still in the nucleus. It should be emphasized that the presence of such high concentrations of TS in H35R cells is not encountered normally, since TS, even in actively dividing cells, can be detected only by a sensitive tritium release assay (29), whereas the enzyme can be measured easily in H35R cell extracts using a spectrophotometric assay (26). This massive level of TS in the cytoplasm of H35R cells is also associated with an altered morphology in that these cells appear to be considerably larger than the H35S cells. It is not known at this time whether the morphologic differences are associated with an apparent impaired transport of TS to the nucleus. Even so, it is not obvious how TS is directed to the nucleus, since it does not possess a typical nuclear localization signal (31), although there are three sites in the protein sequence of human, mouse, and rat TS (27) with three to four basic residues within a seven- to eight-amino acid peptide sequence that could serve this purpose. Alternatively, the enzyme might be chaperoned into the nucleus by a protein similar to that described recently for the Id family of helix-loop-helix proteins (32). It is of interest to note that dUTPase, like TS, although associated with the nucleus, does not contain a characteristic nuclear localization signal either (15, 33).

Other properties that dUTPase and TS share relate to their presence in mitochondria and their state of phosphorylation. It is possible that the mitochondrial location of TS is due to the nonspecific adherence of TS to the surface of the mitochondria, but the extensive washing procedure employed would appear to mitigate against this possibility, as well as our recent finding that the enzyme can be released on hypotonic lysis of the mitochondria.3 Preliminary results reveal that the H35 TS is labeled on a serine, as has been found also for dUTPase (33). Because of these common properties of TS and dUTPase, it would not be unreasonable to assume that the two enzymes reside in the same regions of the cell, possibly in the proposed replitase complex (12). As shown in Fig. 6, extracts of H35 cells contain a kinase (5) that phosphorylates TS. More recently, to test TS's susceptibility to phosphorylation, we have found such kinases as protein kinase C and calmodulin kinase to phosphorylate recombinant rat TS quite well, and with a fair degree of specificity, as several other proteins including E. coli TS, were not phosphorylated.3

A function for the phosphorylation of TS, if any, is not known, although based on similar studies, it has been shown that phosphorylation can affect the stability, the activity, and even the location of a protein (34). As shown recently in the case of MADR2, its nuclear accumulation and signaling depend on it being phosphorylated (35). This does not appear to be an isolated case as more and more instances are being reported on the influence of protein phosphorylation on the cellular location of various proteins (34, 36, 37), particularly those associated with cell division. It is interesting to note that only the nuclear form of dUTPase is also phosphorylated (33). Whether a similar case can be made for TS remains to be determined. In a similar vein, questions can be raised regarding the function of TS in the nucleus of the cell and even more so the purpose of its nucleolar presence. Since TS has been shown to interact with its own mRNA to regulate its translation (9), as well as that of c-myc RNA (38), it is possible that what is observed in the autoradiographic patterns (Fig. 3A) is an association of TS with its mRNA or pre-mRNA or possibly its association with a replitase complex (17). As far as the mitochondrial location of TS, mitochondrial DNA must be maintained, and since TS is involved in providing a substrate for the synthesis and repair of DNA, this could very well be its function. In any event it would appear from the data presented here that the functional role of TS may be more complex than merely serving as a provider of dTMP. A preliminary account of these findings has been presented (39).


FOOTNOTES

*   This work was supported in part by Grants CA44355 (to F. M.) and CA25933 (to J. G.) from the National Cancer Institute (United States Public Health Service/Health and Human Services) and Grant MCB-9316321 (to G. M.) from the National Science Foundation.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.
Dagger    Present address: Dept. of Neurology, Massachusetts General Hospital, Charlestown, MA 02129.
§   Present address: Boston University School of Medicine, Boston Medical Center, P. O. Box 311, Boston, MA 02118.
   To whom correspondence should be addressed: Wadsworth Center, New York State Dept. of Health, Empire State Plaza, P. O. Box 509, Albany, NY 12201-0509. Tel.: 518-474-4184; Fax: 518-473-2900; E-mail: maley{at}wadsworth.org.
1   The abbreviations used are: TS, thymidylate synthase; dUMP, 2'-deoxyuridine 5'-monophosphate; FdUMP, 5-fluoro-2'-deoxyuridine 5'-monophosphate; dTMP, 2'-deoxythymidine 5'-monophosphate; FdUrd, 5-fluoro-2'-deoxyuridine; CH2H4PteGlu, 5,10-methylene tetrahydrofolate; H2PteGlu, dihydrofolate; dUTPase, deoxyuridine triphosphatase; PAGE, polyacrylamide gel electrophoresis; DMEM, Dulbecco's modified Eagle's medium; RIPA, radioimmune precipitation buffer.
2   W. A. Samsonoff, G. Maley, and F. Maley, unpublished observations.
3   J. Reston and F. Maley, unpublished data.

ACKNOWLEDGEMENTS

We express our appreciation to Judith Valentino for her excellent assistance in preparing this manuscript and to Zenia Nimec for her assistance in some of these experiments. We also thank Dr. Carmen Mannella of our institution for his helpful suggestions on the lysis of mitochondria.


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