(Received for publication, October 2, 1996, and in revised form, November 11, 1996)
From the Laboratory of Drug Discovery Research and
Development, Developmental Therapeutics Program, Division of Cancer
Treatment, Diagnosis and Centers, NCI, Frederick Cancer Research and
Development Center, Frederick, Maryland 21702 and the
§ Medicine Branch, Division of Clinical Sciences, NCI,
National Institutes of Health, Bethesda, Maryland 20892
Epothilones A and B, natural products with
minimal structural analogy to taxoids, have effects similar to those of
paclitaxel (Taxol®) in cultured cells and on microtubule
protein, but differ from paclitaxel in retaining activity in
multidrug-resistant cells. We examined interactions of the epothilones
with purified tubulin and additional cell lines, including a
paclitaxel-resistant ovarian carcinoma line with an altered
-tubulin. The epothilones, like paclitaxel, induced tubulin to form
microtubules at low temperatures and without GTP and/or
microtubule-associated proteins. The epothilones are competitive
inhibitors of the binding of [3H]paclitaxel to tubulin
polymers. The apparent Ki values for epothilones A
and B were 1.4 and 0.7 µM by Hanes analysis and 0.6 and
0.4 µM by Dixon analysis. In the paclitaxel-sensitive human cell lines we examined, epothilone B had greater
antiproliferative activity than epothilone A or paclitaxel, while
epothilone A was usually less active than paclitaxel. A
multidrug-resistant colon carcinoma line and the paclitaxel-resistant
ovarian line retained sensitivity to the epothilones. With
Potorous tridactylis kidney epithelial (PtK2)
cells examined by indirect immunofluorescence, microtubule bundles
appeared more rapidly following epothilone B treatment, and there were
different proportions of various mitotic aberrations following
treatment with different drugs.
Many facets of cellular growth depend on microtubules. They
provide support for organelles and membranes, resist compressive forces, provide tracks for intracellular vesicular transport and sorting, and form spindle fibers for chromosomal separation and segregation (1). Composed of the heterodimeric protein tubulin, microtubules are dynamic structures that undergo periods of slow growth
and rapid shortening both in vitro and in cells (2-4). Cellular functions of microtubules probably depend on this phenomenon. Jordan et al. (5) have shown that significant alterations of dynamic instability occur with a variety of antimitotic drugs that
interact with tubulin. An increasing number of such compounds, displaying great structural diversity, have become available, and the
most potent of these agents were initially isolated from natural
sources (6). Typically, such compounds inhibit tubulin polymerization,
and all lead to mitotic arrest. Ptx1
(Taxol®) and docetaxel (Taxotere®)
(structures in Fig. 1), however, stabilize microtubules (7, 8). These
complex diterpenes are currently being used to treat a variety of solid
tumors (9, 10).
Recently, three non-taxoid compounds have also been shown to stabilize microtubules. The macrolides EpA and EpB, from the bacterium Sorangium cellulosum (11), and the polyhydroxylated alkatetraene lactone Dcd (structures in Fig. 1), from the marine sponge Discodermia dissoluta (12), share with Ptx the ability to arrest cells in mitosis, cause formation of bundles of intracellular microtubules in non-mitotic cells, and induce the formation of hyperstable tubulin polymers.
Because the initial studies with the epothilones were performed with microtubule protein (11), we decided it was important to examine the interactions of these new drugs with purified tubulin and characterize the effects of MAPs and GTP on these interactions. We compared interactions between tubulin and Ptx with those between tubulin and the epothilones under a variety of conditions. Of particular interest to us was the nature of the binding site of the epothilones on microtubules because of the lack of structural similarity between the taxoids, Dcd, and the epothilones. Despite this dissimilarity, we observed a competitive pattern of inhibition by EpA and EpB on the binding of [3H]Ptx to polymer formed with purified tubulin. EpB was the most effective compound in inducing assembly of tubulin polymers, while the potency of EpA was similar to that of Ptx.
We also report initial studies on the antiproliferative effects of EpA and EpB in cultured cells. With Potorous tridactylis kidney epithelial (PtK2) cells, we confirmed the cellular reorganization of microtubules described by Bollag et al. (11). We found that EpB was more potent than Ptx and EpA, which tended to be less potent than Ptx, in inhibiting the growth of five human tumor cell lines. The epothilones retained their potency in cell lines resistant to Ptx.
EpA and EpB were isolated from S. cellulosum (11). The compounds were generously provided by Dr.
Michael Goetz of Merck Research Laboratories. Ptx and
[3H]Ptx (19-23 mCi/mmol) were obtained from the Drug
Synthesis and Chemistry Branch, NCI (Rockville, MD). Drugs were
dissolved in dimethyl sulfoxide, and control samples contained
equivalent amounts of solvent. Heat-treated MAPs and
electrophoretically homogeneous tubulin were prepared from bovine brain
(13). Tubulin was freed from unbound nucleotide by gel-filtration
chromatography, reconcentrated, and dialyzed against 0.1 M
Mes (pH 6.9) as described elsewhere (8). The tubulin was centrifuged to
remove aggregated protein and stored in liquid nitrogen in 0.2-ml
aliquots. Human Burkitt lymphoma CA46 cells were a gift from Dr. P. O'Connor, NCI (Bethesda, MD); P. tridactylis kidney
epithelial (PtK2) cells were from the American Type Culture
Collection. The human ovarian carcinoma line 1A9 (14) was used to
generate a Ptx-resistant line, 1A9 (PTX22), by incubating the cells
with increasing concentrations of Ptx in the presence of
verapamil.2 The human colon carcinoma line
SW620 and its subline SW620AD-300, which overexpresses P-glycoprotein,
were described elsewhere (15). Culture media and FCS were from Life
Technologies, Inc., Permanox and glass slides from Nunc, murine
monoclonal anti--tubulin antibody and GTP from
Sigma, and Texas Red-conjugated goat-anti-mouse IgG and ProLong antifade fluorescent mounting media from Molecular Probes.
GTP and ddGTP (from Pharmacia) were repurified by anion exchange
chromatography on DEAE-cellulose.
Cells were grown in 5-ml suspension cultures at 37°C in a humidified 5% CO2 atmosphere in RPMI medium supplemented to 2 mM glutamine, 12% FCS, 10 µg/ml gentamicin sulfate, 1% (v/v) dimethyl sulfoxide, and varying drug concentrations. The initial inoculum was 105 cells/ml. For determination of IC50 values, cells were grown for 72 h and counted in a Coulter counter. The IC50 drug concentration inhibited increase in cell number by 50%.
Inhibition of Carcinoma Cell GrowthCells were continually incubated in RPMI medium containing 10% FCS, 12 µg/ml gentamicin sulfate, and 2 mM glutamine. The medium for the Ptx-resistant ovarian line also contained 5 µg/ml verapamil (to inhibit expression of P-glycoprotein) and 15 ng/ml Ptx. Prior to drug treatment, the Ptx-resistant ovarian cells were removed from Ptx-containing media for 5-7 days. Drug effects were determined in 96-well microtiter plates, with cells fixed and stained for protein (16).
Indirect ImmunofluorescenceConfluent monolayers of
PtK2 cells, grown on 25-cm2 plates, were
suspended by incubation with 7 ml/plate of 0.05% trypsin and 0.53 mM EDTA in Hank's balanced salt solution. Suspended cells were diluted 1:40 with MEM containing 1 mM sodium pyruvate,
0.1 mM nonessential amino acids, 10% FCS, 2 mM
glutamine, and 10 µg/ml gentamicin sulfate and allowed to attach and
grow for 24 h at 37°C in a humid 5% CO2 atmosphere
on sterile, eight-well Permanox or glass cell-culture slides (300 µl/well, 103 cells/well). Medium was removed and attached
cells were incubated in supplemented MEM containing 10 µM
drug at 37°C. After various incubation times, medium was removed, and
cells were rinsed with PBS at 37°C. Attached cells were fixed in
20°C methanol for 10 min, rinsed three times with PBS, and
incubated in PBS containing 0.1% Triton X-100 and 10% FCS for 30 min
at room temperature to block nonspecific antibody binding sites. The
blocking buffer was removed, and the cells were incubated for 1 h
at 37°C with antibody to
-tubulin (200 µl/well, 1:200 dilution
in blocking buffer). Cells were washed three times with PBS and
incubated for 45 min with Texas Red-conjugated goat anti-mouse IgG (150 µl/well, 1:50 dilution in PBS). Following removal of the secondary antibody by two washes with PBS, diaminopropidium iodide (2 µg/ml) dissolved in PBS was added to stain DNA. Slides were wet-mounted in
ProLong according to the manufacturer's procedures. Cells were examined with a Nikon Optiphot-2 epifluorescence microscope and photographs taken with Kodak T-MAX 100 film.
Polymerization was followed turbidimetrically at 350 nm in Gilford model 250 spectrophotometers equipped with electronic temperature controllers. Base-line levels were established with the reaction mixtures, containing all components except drug, held at 0°C. Drug was added and mixed into the reaction mixture, and the reaction was followed as indicated at 0°C. Temperature settings were changed as indicated, rising in the reaction mixtures at 0.5°C/s and falling at 0.1°C/s.
Inhibition of [3H]Ptx Binding to PolymerFor all binding studies, tubulin polymer was preformed in the absence of drugs for 30 min at 37°C in reaction mixtures containing 2 µM tubulin, 20 µM ddGTP, and 0.75 M monosodium glutamate (2 M stock solution adjusted to pH 6.6 with HCl). This condition induced nearly complete assembly of tubulin into polymer (data not presented; cf. Refs. 17-19). Mixtures of EpA or EpB with [3H]Ptx in varying concentrations were added to preformed polymer and incubated for 30 min at 37°C. Bound [3H]Ptx was separated from free [3H]Ptx by centrifugation of the reaction mixtures at 14,000 rpm in an Eppendorf microcentrifuge for 20 min at room temperature. Greater than 90% of added protein sedimented under these conditions even in the absence of drug. Protein and radiolabel in both supernatants and pellets (dissolved in 0.1 M NaOH overnight and neutralized with 0.1 M HCl) were quantitated by the Lowry procedure and liquid scintillation counting. Data from at least three independent experiments were combined for data analysis.
Electron MicroscopyDuring polymerization reactions 10 µl aliquots were removed at various times and placed on 200-mesh carbon-coated, Formvar-treated, copper grids. Samples were stained with several drops of 0.5% uranyl acetate and examined in a Zeiss model 10CA electron microscope.
Table I summarizes inhibitory effects of EpA, EpB, and Ptx on the growth of five human tumor cell lines. In all cases EpB was more potent than Ptx or EpA. Burkitt cells treated with EpA or EpB accumulated in mitotic arrest (data not presented; cf. Ref. 11). We confirmed the observation of Bollag et al. (11) that the epothilones were not P-glycoprotein substrates. The MDR colon carcinoma line SW620AD-300, with over a 1000-fold increased resistance to Ptx relative to its parental line, had sensitivity to EpA and EpB similar to that of the parental line.
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The ovarian carcinoma cells were evaluated because of the
characterization of the biochemical properties of tubulins derived from
the parental line and from a Ptx-resistant line2 that
strongly indicate that resistance was caused by an altered -tubulin.
It is therefore notable that the parental and Ptx-resistant lines had
nearly equal sensitivity to both EpA and EpB while retaining significant resistance to several potent taxoids we have examined, including docetaxel and
2-debenzoyl-2-meta-azidobenzoylpaclitaxel.3
PtK2 cells were used to evaluate the effects of EpA, EpB, and Ptx on intracellular microtubules. IC50 values, determined by counting both adherent and detached cells, were 40, 44, and 120 nM for EpA, EpB, and Ptx, respectively. We confirmed the findings of Bollag et al. (11) that EpA and EpB, like Ptx, enhance intracellular microtubule assembly.
Fig. 2 illustrates the effects of these drugs on
cellular microtubules at 2, 6, and 24 h. Panels A-C
show control cells; D-F, cells treated with Ptx;
G-I, with EpB; and J-L, with EpA. All three
drugs caused microtubules to become more bundled and to develop
multiple regions of nucleation (arrows in Fig. 2,
E, G, and K) in interphase cells
(those with nuclei). Bundling of microtubules at 2 h was more
extensive following EpB treatment than treatment with the other drugs.
After 24 h (Fig. 2, F, I, and L),
microtubules were found almost exclusively in large bundles. Each drug
examined produced similar cellular changes overall, but a few
morphological differences were noted, especially in mitotic cells.
A variety of mitotic aberrations were observed as early as 2 h and were maximal at 6 h (Table II). With 10 µM drug, normal spindles were never observed, and microtubule organization in mitotic cells (those with condensed chromosomes and no apparent nuclear membrane) was distinct from that in interphase cells. This suggests that, despite the high stability of microtubules formed in biochemical systems with these drugs (see below), substantial microtubule turnover occurs in cells (cf. Refs. 5 and 20).
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Most mitotic cells could be placed in one of three categories (Table II). Each subtype was observed following treatment with all three drugs, but relative proportions varied. Ptx produced more punctate-stained spindle aberrations (Fig. 2, D and E, arrowheads), probably representing multiple microtubule organizing centers or spindle poles. Short filaments resembling astral microtubules were attached to the multiple spindle poles, and these are listed as "aster spindles" in Table II. Astral microtubules appeared to be longer in epothilone-treated cells than in Ptx-treated cells. With EpB most mitotic cells had complex arrays of relatively long microtubules that formed a spiral pattern. Such "spiral spindles" had only one apparent or two poorly separated microtubule organizing centers (Fig. 2H, arrowhead). The third distinct type of mitotic cell was most abundant following treatment with EpA. These "spike spindles" (not shown) had short clusters of thick microtubules originating from one or two microtubule organizing centers, and they may represent a variant of the aster spindles resulting when the microtubule organizing center remained intact. We do not know if these aberrant spindles represent any sort of progression, although the spikes were observed only at the later time points, and with both EpA and Ptx asters were observed before either spirals or spikes. Finally, additional mitotic cells had patterns of microtubule organization that did not fit any of these categories (Fig. 2J, arrowhead).
Effects of EpA and EpB on the Polymerization of Purified Tubulin with and without MAPs and/or GTPPtx and other taxoids induce tubulin assembly under conditions where the reaction usually does not occur, and taxoid-induced polymers are more stable than normal microtubules. Thus, with these drugs assembly can occur at low temperatures and in the absence of MAPs and/or exogenous GTP, and the polymers formed are resistant to disassembly by calcium, dilution, or low temperatures (7, 8, 21-24).
In their studies Bollag et al. (11) showed that EpA and EpB induced the assembly of microtubule protein in the absence of GTP at 37°C, with substoichiometric (relative to tubulin) concentrations of the scarcer EpB inducing more extensive assembly than an equivalent concentration of EpA or Ptx, which had nearly identical activities. They also showed that microtubules induced by the epothilones were resistant to cold- or calcium-induced disassembly. However, no studies were performed with purified tubulin and MAPs to define their relative importance in the interactions of polymer with the epothilones, nor was assembly at low temperatures evaluated.
To address these issues we performed the experiments presented in Fig.
3, examining assembly reactions induced by the
epothilones and Ptx. Assembly was followed at a series of progressively
higher temperatures, and polymer stability was evaluated by a final
incubation at 0°C. Panel A presents reactions with both
MAPs and GTP, panel B with MAPs only, and panel C
with GTP only. Equimolar concentrations (10 µM) of
tubulin and drug were used. EpB always caused the most vigorous
polymerization of tubulin, while the relative activities observed with
EpA and Ptx depended on the reaction condition.
In the presence of GTP and MAPs (Fig. 3A), the only condition that supported microtubule assembly without drug, EpB and to a lesser extent EpA, induced tubulin polymerization at 0°C, whereas assembly with Ptx required a higher temperature. Assembly was near its maximum with all compounds after 10 min at 25°C, with the highest turbidity reading obtained with EpB. When the reaction temperature was reduced to 0°C, there was a slight decrease in turbidity with EpA and Ptx but not with EpB. Tubulin polymer formed without drug disassembled to near base-line level at 0°C, and, without drug, assembly required a 25°C incubation. Electron micrographs of aliquots taken from reaction mixtures after 1 h at 0°C with all three drugs showed that microtubules remained intact (data not shown). Addition of 5 mM CaCl2 at 0°C resulted in nearly complete disassembly of Ptx and EpA polymers, while the EpB polymer remained intact (data not shown). This total stability of the EpB-induced polymer is thus identical to that observed with Dcd (12).
When reaction mixtures contained tubulin and MAPs but no GTP (Fig. 3B), more vigorous assembly occurred with EpA or EpB than with Ptx. The epothilones induced assembly at 10°C, and maximum turbidity readings occurred at 25°C. With Ptx, no assembly occurred until the temperature reached 25°C, and a 37°C incubation was required for maximum assembly. When the temperature was returned to 0°C, little disassembly occurred with any of the drug-induced polymers.
A different pattern was obtained when GTP, but not MAPs, was added (Fig. 3C). While each drug nucleated polymer growth at 25°C, under this reaction condition greater apparent activity (see below) was observed with Ptx than with EpA. EpB induced near maximum turbidity at 25°C, whereas Ptx and EpA caused modest reactions. At 37°C, little additional assembly occurred with EpB, but further polymerization was observed with Ptx and EpA. The turbidity reading with Ptx was nearly twice that which occurred with EpA. When the reaction temperature was returned to 0°C, the epothilone-induced polymer was somewhat more resistant to disassembly than the Ptx-induced polymer.
In the absence of both GTP and MAPs, none of the drugs stimulated significant tubulin polymerization at 10 µM drug + 10 µM tubulin. Reactions did occur at higher concentrations of tubulin or drug.
The ability of the taxoids, Dcd, and the epothilones to induce assembly at low temperatures and without MAPs and/or GTP are probably manifestations of the ability of these agents to cause hypernucleation of tubulin polymerization. Perhaps the best quantitative measure of this property is the [T]cr. We recently reported on [T]cr values obtained with a series of taxoids that included compounds both more and less active than Ptx (8). The quantitative results were in excellent agreement with the qualitative effects of these agents on assembly at low temperatures and in the absence of MAPs or GTP. We therefore compared [T]cr values of the 37°C reactions induced by the epothilones with those induced by Ptx at 10 µM drug (Table III).
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With MAPs and GTP, the [T]cr with all three drugs was less than 1 µM, as compared with 3 µM without drug. Differences between drugs were readily detected under the other reaction conditions. Generally the values obtained were in accord with the qualitative results shown in Fig. 3. With MAPs only, Ptx and EpA yielded [T]cr values of 1.4-1.7 µM and EpB, 0.8 µM. With GTP only, the [T]cr with EpB was 2 µM, less than half those obtained with EpA and Ptx (4.3-4.5 µM). With neither MAPs nor GTP, the [T]cr values were still higher, 7.4 µM with EpB, 22 µM with Ptx, and 19 µM with EpA. In summary, EpA and Ptx have similar [T]cr values under all reaction conditions, while the [T]cr values with EpB are about 50% lower.
Another parameter of nucleation is microtubule lengths. These were quantitated on samples taken from reaction mixtures containing equimolar (10 µM) tubulin and drug (Table IV) under conditions where polymerization occurred. With MAPs and GTP, all three drugs yielded polymer with a shorter average length than that formed without drug, consistent with enhanced nucleation. The EpB polymers were shorter and the EpA polymers longer than the Ptx polymers. With MAPs but not GTP, microtubules were longer than those formed in the complete system with all three drugs. The EpA polymers were slightly longer than the Ptx polymers, and the EpB microtubules were about half as long as those formed with the other drugs. With GTP but not MAPs, average microtubule length further increased, but the relative lengths induced with the three drugs remained about the same.
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In the current studies, all samples taken for electron microscopic evaluation displayed primarily the morphology of microtubules, with occasional, short areas of open microtubules (ribbons). There were no obvious differences between the Ptx-induced polymers and those formed with the epothilones, other than the length differences summarized above. Predominant microtubule morphology was observed under all reaction conditions (MAPs + GTP, MAPs only, GTP only, no MAPs/no GTP) and whether or not calcium had been added to the reaction. Moreover, microtubules persisted for a least 1 h at 0°C following incubation at higher temperatures.
Competitive Binding of Epothilones and Ptx to MicrotubulesDespite the similarity of the effects of the epothilones and Ptx on assembly reactions, the disparate structures of these compounds caused us to undertake studies to gain information about their binding site(s). With purified tubulin, we confirmed the findings of Bollag et al. (11) with microtubule protein that both EpA and EpB displaced [3H]Ptx from preformed polymers, but we found EpB distinctly more potent than EpA. In detailed kinetic experiments we demonstrated that both EpA and EpB are competitive inhibitors of the binding of [3H]Ptx to polymer. (A similar finding, as a control experiment, was made with docetaxel, generously provided by Dr. D. G. I. Kingston.)
Fig. 4 presents our binding data with EpB in the Hanes
format, in which a competitive inhibitor generates a family of parallel curves at different inhibitor concentrations. Analysis of these data
and similar, but less extensive, data with EpA yielded apparent Ki values of 1.4 µM for EpA and 0.71 µM for EpB from the abscissa intercepts (25). (The value
obtained for docetaxel was 1.2 µM.) Dixon analysis of the
same data yielded slightly different apparent Ki
values, 0.6 and 0.4 µM for EpA and EpB, respectively.
EpA and EpB are non-taxoid natural products of bacterial origin that Bollag et al. (11) found paralleled Ptx in their effects on cultured cells and in promoting the assembly of microtubule protein. They further found that EpA and EpB displaced [3H]Ptx from microtubules, implying that the target for these agents is tubulin itself. In the cellular studies, Ptx was more effective than the epothilones in inhibiting the growth of two cell lines, and EpB was 2.5 times more effective than Ptx in one line. Most importantly, both EpA and EpB remained cytotoxic for the MDR line KBV-1, which was highly resistant to Ptx. In the biochemical studies, EpB was more active than EpA in inducing microtubule assembly but less active than EpA in displacing [3H]Ptx from polymer.
A reisolation of the epothilones allowed us to further evaluate these compounds. First, we wanted to confirm that the target of the epothilones was in fact tubulin by studying interactions of EpA and EpB with purified tubulin and to evaluate specific effects of MAPs, GTP, and reduced temperature in assembly reactions induced by these agents. Second, we wanted to determine whether or not the epothilones bound to tubulin in polymer in the same or a different site than Ptx by kinetic criteria. Third, we wanted to determine the relative effects of the epothilones and Ptx on the growth of additional cell lines, in particular lines resistant to Ptx. Fourth, we wanted to determine whether subtle differences in microtubule rearrangement could be detected in cells treated with EpA and/or EpB in comparison with those treated with Ptx.
We unequivocally showed that tubulin is the target of the epothilones. These agents, like Ptx, other taxoids, and Dcd will induce purified tubulin to form microtubules both with and without GTP in the reaction mixture. MAPs do not appear to form part of the binding site for EpA and EpB, and the quantitative effects of MAPs (Tables III and IV) are equivalent for Ptx and the epothilones.
Under all conditions studied, EpB was more active than both EpA and Ptx, suggesting that the methyl group at C-12 enhances a hydrophobic interaction between drug and tubulin. More extensive assembly occurred at lower temperatures with EpB, the [T]cr was half that observed with the other drugs, and shorter microtubules were formed with EpB. EpB is thus a more potent inducer of microtubule nucleation reactions than either Ptx or EpA.
The comparison of effects of EpA and Ptx is more complex. With MAPs as a component of the reaction mixture, assembly was slightly more extensive with EpA than with Ptx, with assembly occurring somewhat more readily at lower temperatures. Without MAPs but with GTP, the Ptx reaction was more extensive than the EpA reaction. Although we could detect no significant difference in the [T]cr between EpA and Ptx, EpA microtubules were longer than Ptx microtubules. This may indicate that there are subtle differences in the relative effects of Ptx and EpA on nucleation and elongation reactions.
For our second goal, to obtain kinetic evidence for the binding of Ptx and the epothilones at the same or different sites on tubulin polymers, we devised a reaction condition with tubulin as the only protein component in which virtually all of the tubulin was first driven into microtubules. We exploited the finding that ddGTP is more potent than virtually any other nucleotide in inducing tubulin polymerization (17-19). Initial displacement studies (constant [3H]Ptx, varying epothilone concentrations) demonstrated that EpB was more potent than EpA, in contrast to the results of Bollag et al. (11). When both substrate ([3H]Ptx) and inhibitor (epothilone) concentrations were varied and analyzed, we obtained classic competitive inhibition patterns with EpA and EpB, as well as with the docetaxel control. Generally, this is interpreted as indicating binding at the same site, although binding in overlapping sites or allosteric phenomena are probably not excluded. The apparent Ki values derived from these experiments indicated that EpB bound 1.5-2 times as tightly as EpA, relative values comparable to those obtained for the [T]cr value and microtubule lengths (the EpB values about half the EpA values). It is possible that the difference between the relative activities of EpA and EpB in inhibiting [3H]Ptx binding that we found versus those observed by Bollag et al. (11) with microtubule protein may indicate a modulating effect of MAPs in the latter system.
The relationship of the Ptx site on polymer to other drug binding sites
on tubulin is uncertain. Binding of radiolabeled taxoids has only been
observed with polymer, and many inhibitors of assembly inhibit both
taxoid-driven assembly and binding of taxoid to tubulin (23, 26-28).
Recent observations suggest that Ptx and the colchicine tropolone ring
interact with the same region of -tubulin (29-31) (cf.
Ref. 32). The Ptx-like activity of Dcd and the epothilones may
strengthen this conclusion. A computer analysis of compounds of unknown
activity for structural features shared with colchicine site drugs was
the first indication that Dcd was a tubulin active agent (33). In the
epothilones, a prominent structural feature is the thiazole moiety in
the side chain at C-15. This is reminiscent of the thiazoline ring of
curacin A, a structurally unique competitive inhibitor of colchicine
binding (34). Ongoing structure-activity studies with curacin A analogs
have demonstrated that activity is retained when the thiazoline ring is
oxidized to a thiazole ring and largely lost when the thiazoline ring
is disrupted.4 These observations may
indicate that the thiazoline ring of curacin A interacts at the same
site on tubulin as the tropolone ring of colchicine and that the
thiazole ring of the epothilones is essential for their activity as
inducers of tubulin assembly.
For our third goal, we studied several human cancer cell lines: 1) the
Burkitt lymphoma CA46 line because of the high mitotic index it yields
with anti-tubulin agents; 2) the colon carcinoma line SW620, for
comparison with a line derived from it, SW620AD-300, that is highly
resistant to Ptx on the basis of overexpression of P-glycoprotein; 3)
the ovarian carcinoma line 1A9, for comparison with a line derived from
it, 1A9(PTX22), that has moderate resistance to Ptx based on expression
of a modified -tubulin. The Burkitt cells were 3-fold more sensitive
to EpB than to Ptx, while EpA was about 50% less active than Ptx. The
parental colon cells were 2-fold more sensitive to EpB than to Ptx, but
EpA was 10-fold less active. Importantly, however, we found that the
MDR colon line, like the MDR line studied by Bollag et al.
(11), remained sensitive to both epothilones. Thus, the Ptx-resistant
cells were over 80-fold more sensitive to EpA and over 800-fold more
sensitive to EpB than to Ptx. The parental ovarian line was equally
sensitive to Ptx and EpA, but over 30-fold more sensitive to EpB. Again the derived Ptx-resistant line retained nearly complete sensitivity to
both epothilones, so that it was 14-fold more sensitive to EpA than to
Ptx, and over 400-fold more sensitive to EpB. In conjunction with the
immunofluorescence studies, we found that PtK2 cells were
about 3-fold more sensitive to EpA and EpB than to Ptx. Höfle et al. (35) reported that among the cell lines they had
examined, EpB was usually twice as active as EpA.
The epothilones deserve a thorough evaluation as potential anticancer
drugs. The scarcer EpB is usually more active against cells in culture
relative to Ptx and EpA, concordant with its greater activity in
promoting tubulin assembly and in inhibiting the binding of
[3H]Ptx to polymers prepared from purified tubulin. The
epothilones can be obtained in bulk from fermentation cultures (11,
36), are active in MDR cell lines resistant to Ptx (Ref. 11; Table I),
are active in a cell line with Ptx resistance based on an alteration in
-tubulin (Table I), and are 30-fold more soluble than Ptx in aqueous
solution (35), thus permitting easier administration to patients and
avoiding side effects of Ptx administration attributed to the vehicle
(9).
Finally, we evaluated over time the effects of Ptx, EpA, and EpB on the microtubule network of PtK2 cells treated with 10 µM drug. At this high concentration, used to minimize effects of differential cytotoxicity, there were no clear-cut differences between the compounds. Massive microtubule bundles were apparent at 2 h only with EpB, probably because of its tighter binding to tubulin polymers. In mitotic cells (those with condensed chromosomes), three types of microtubule arrays were observed with all drugs. The first were multiple nucleation centers that had short microtubules attached that resembled short astral fibers. Cells with these structures were more abundant following Ptx or EpA treatment, but the attached microtubules were longer in epothilone-treated cells. The second tended to have a single nucleation center, perhaps derived from an undivided centrosome, and the microtubules were long and arranged in a spiral pattern. Cells with these structures were most abundant following treatment with EpB. The third tended to have one or two nucleation centers with multiple short microtubules originating at these centers. Cells with these spike-like spindle aberrations were most abundant in EpA-treated cells. There is no ready explanation for these mitotic differences from our biochemical studies. They may derive from different effects of the epothilones versus Ptx on microtubule dynamics (8, 20). Such effects may be more critical in mitotic as opposed to interphase cells.
We are indebted to Dr. Michael Goetz for the reisolation of EpA and EpB that made these studies possible and to Merck Research Laboratories for providing samples of the compounds.