Effects of cytochalasin congeners, microtubule-directed agents, and doxorubicin alone or in combination against human ovarian carcinoma cell lines in vitro

Cytochalasins are mycotoxins known to disrupt the formation of filamentous (F)-actin, thereby preventing the formation of functional microfilaments. These congeners are characterized by a highly substituted perhydro-isoindolone structure that is typically attached to a macrocyclic ring [1]. More than 60 different cytochalasins from several species of fungi have been classified into various subgroups based on the size of the macrocyclic ring and the substituent of the perhydroisoindolyl-1-one residue at the C-3 position [2]; structures of representative cytochalasins are shown in Fig. 1. While most of our previous work has focused on cytochalasin B, there are many other congeners with similar activity toward microfilaments. As microfilament-disrupting agents, cytochalasins alter cell motility, adherence, secretion, drug efflux, deformability, morphology, and size, among many other cell properties critical to neoplastic cell pathology [1, 2]. In addition, two of the congeners (cytochalasins B and D) have shown partial specificity against neoplastic cells [3‐10], consistent with the substantial differences known to exist between the microfilament biochemistry of neoplastic and normal cells [11, 12]. These differences in microfilament structure may be related to key neoplastic characteristics, including altered adherence, anchorage independent growth, invasiveness, and altered plasma membrane cytoskeletal interactions involving expression of oncoproteins [12, 13].

Previously, we have demonstrated that cytochalasin B and its reduced congener 21,22-dihydrocytochalasin B (DiHCB) are able to sensitize multidrug resistant P388/ADR murine leukemia cells to doxorubicin, with both congeners showing considerable drug synergy with the nucleic acid-directed agent [14]. In addition, prior research has indicated that cytochalasin B efflux is less affected by overexpression of ATP binding cassette (ABC) transporters than other cytotoxic drug classes (vinca alkaloids and anthracyclines) [15] that often exhibit drug resistance in the clinical setting. Based on these observations, it appears that cytochalasin B and potentially other cytochalasin congeners might be active against multidrug resistant neoplastic cells and might also be able to overcome resistance to other cytotoxic agents currently used in the clinical setting. Therefore, this study seeks to determine the effects of cytochalasin congeners toward drug sensitive and multidrug resistant human cancer cell lines.

SKOV3 is a human ovarian carcinoma cell line frequently used in vitro and also in vivo as a xenograft in immunosuppressed mice. SKOV3 cells have slight, but noticeable resistance to tumor necrosis factor, as well as to cisplatin and doxorubicin [16, 17]. The inherent drug resistance of SKOV3 cells can be dramatically elevated through progressively increasing exposure to either vinblastine or vincristine [18]. One of the most notable multidrug resistant cell lines, SKVLB1, is 2,000-fold more resistant to vinblastine, 10,000-fold more resistant to vincristine, 260-fold more resistant to doxorubicin, and 510-fold more resistant to the non-clinically approved colchicine when compared to the parental cell line [18]. Further, this increase in drug resistance is mirrored by increasing overexpression of P-glycoprotein (P-gp), a known ABC transporter [19, 20]. Since cytochalasin B efflux is notably resistant to P-gp overexpression, drug sensitive and drug resistant SK human ovarian carcinoma cell lines are ideal models to examine cytochalasin sensitivity in multidrug resistant cancers. These cell lines can also reveal potential drug synergism when cytochalasin congeners are combined with chemotherapeutic agents, or with calcium ion channel blockers known to inhibit P-gp drug efflux [20‐24].

With respect to SK human ovarian carcinoma cells, it appears that the nine cytochalasin congeners examined in this study fall into three groups. Against the SKOV3 cell line, cytochalasins C, D, E and H were less cytotoxic than are the clinically approved antineoplastic agents (doxorubicin, paclitaxel and vinblastine), with 96 h continuous exposure IC₉₀ values ranging from 80 to 330 nM (Table 1). IC₉₀ values for the three clinically approved agents ranged from 2 to 11 nM. Cytochalasins C, D, E, and H as a group appeared to be subject to drug resistance against multidrug resistant SKVLB1 cells as exemplified by cytochalasin D which had a RI = 100 against SKVLB1. While this RI was not as high as for any of the clinically approved chemotherapeutic agents in the study, it is likely that overexpression of P-gp does reduce the cytotoxicity of these congeners, presumably due to drug efflux.

The second group composed of cytochalasins B, J, DiHCB and DiHCBγ-L were less cytotoxic against the parental cell line SKOV3. IC₉₀ values ranged from 0.8 to 40 μM (800 to 40,000 nM), and were not subject to strong resistance by SKVLB1 (RIs ranged from 1 to 4-fold). Further, cytochalasin B, DiHCB, and DiHCBγ-L were more cytotoxic against SKVCR0.015 and SKVCR0.1 than against the parental cell line with RI values below 1 (Table 1).

Finally, Cytochalasin A is unique in that it demonstrated less cytotoxicity against the parental cell line (IC₉₀ = 1 μM) than against SKVLB1 (IC₉₀ = 0.75 μM), indicating that it is not subject to SKVLB1 drug resistance. This suggests that cytochalasin A has unique properties with respect to inhibiting P-gp, possibly due to increased binding affinity for the drug efflux pump in conjunction with its electrophilic α, β-unsaturated ketone moiety (Fig. 1), which could potentiate alkylation of key structures within the neoplastic cell (including P-gp). The α, β-unsaturated ketone in cytochalasin A is particularly electrophilic, as it is conjugated to another ketone, making the double bond highly reactive.

It is also very likely that DiHCBγ-L is not influenced by SKVLB1 drug resistance, as the IC₉₀ values were the same against SKOV3 and SKVLB1. The potential of DiHCBγ-L to inhibit P-gp may be related to its relatively low cytotoxicity. DiHCBγ-L had the highest IC₉₀ value against SKOV3 among the nine cytochalasins (40 μM). This suggests that P-gp and other ABC transporters may become saturated by 40 μM DiHCBγ-L in SKVLB1, and that the efflux pumps have difficulty removing such a high concentration. It is also possible that DiHCBγ-L may have increased reactivity deriving from the generation of an α-hydroxyacetamido-group with a reactive secondary hydroxyl group at C-9 when the original lactone of DiHCB is hydrolyzed (Fig. 1), or it may have unique binding capability with ABC transporters. Along with cytochalasin A, DiHCBγ-L may have properties with respect to the drug efflux pump system that would make these two congeners of special interest in preclinical evaluations.

With respect to the intermediately resistant cell line SKVCR0.015, all of the cytochalasins tested (cytochalasins A, B, C, D, DiHCB, and DiHCBγ-L) were equally or more cytotoxic than against SKOV3. All of these cytochalasins except for cytochalasin C also showed equal or enhanced sensitivity rather than resistance when tested against the intermediately resistant cell line SKVCR0.1 (cytochalasins E, H, and J were not tested against the intermediately resistant cell lines). These data suggest that multidrug resistant pumps can be completely overridden by cytochalasins unless there is very high expression of the pumps as in the highly resistant SKVLB1 cell line.

As shown with cytochalasins B, C, D and DiHCB, verapamil was able to increase the cytotoxicity of congeners affected by P-gp overexpression in SKVLB1 cells (Table 3). This increase in cytotoxicity was substantial with the more cytotoxic cytochalasins C and D (32- and 64-fold increase in sensitivity against SKVLB1), which had much higher RIs against SKVLB1 than other congeners. Nevertheless, even less cytotoxic congeners such as cytochalasin B and DiHCB had lower IC₉₀ values against all drug resistant cell lines when combined with 30 μM verapamil (Fig. 3a). Further, growth inhibition of SKVCR0.015 cells at varying concentrations of cytochalasin B was more pronounced after the addition of 30 μM verapamil (Fig. 3e), validating previous observations that calcium ion channel blockers can be used to overcome P-gp mediated drug resistance [28‐30]. Interestingly, it appeared that verapamil had some propensity to modulate P-gp expression (Fig. 5a), suggesting that it may perturb P-gp function through mechanisms other than direct inhibition of the efflux protein. In addition, verapamil had a slight, but noticeable influence on F/G-actin ratios in both SKOV3 and SKVLB1 (Fig. 4), an observation in accord with prior studies that have noted Ca²⁺ oscillations trigger the depolymerization of microfilaments [31‐33]. Together, these data indicate that microfilaments may be a feasible target for inhibiting drug efflux (although the influence verapamil has on microfilaments may merely be an off target effect). This is in accord with Table 3 and Figs. 3 and 4, as concomitant administration of cytochalasin B and verapamil potentiates the cytotoxicity and reduction of F-actin significantly more than cytochalasin B administered as a single agent.

Although verapamil appears to increase the cytotoxicity of most cytochalasins examined in the present study, it is evident that at least some of these congeners have ABC transporter inhibitory activity. As demonstrated in Figs. 5b and c, cytochalasins A and B, but not cytochalasin C, are able to inhibit the ability of SKVLB1 cells to efflux Rh123. These data parallel the 4 day IC₉₀ values attained for these agents against SKVLB1, suggesting that the marked cytotoxicity cytochalasin A and potentially other cytochalasins had against the multidrug resistant cell line was at least partially attributed to inhibition of drug efflux. This appears feasible as congeners more cytotoxic against the parental SKOV3 cell line potentiated lower F-actin levels against SKOV3 than they did against SKVLB1, a cell line that has an inherently lower F/G-actin ratio (Fig. 4). By contrast, cytochalasin A elicited a significantly lower F/G-actin ratio against SKVLB1, suggesting that the compound was not being pumped out at as high of a rate as the more potent F-actin inhibitors. In addition, this figure highlights the potential utility of microfilament-disrupting agents, as multidrug resistant SKVLB1 appears to have a lower ratio of F/G-actin than drug sensitive SKOV3, and normal cells often have higher levels of F-actin than their neoplastic counterparts [34, 35]. Disruption of the actin cytoskeleton is known to induce apoptosis in malignant cells [1, 35], and exploiting their already perturbed microfilament network may provide a novel antineoplastic mechanism that warrants clinical investigation.

Besides the potential of using cytochalasin congeners against certain drug resistant cancers, there exists the possibility of concomitant chemotherapy with clinically approved agents to increase their cytotoxicity. As demonstrated in Table 4, sufficient concentrations of cytochalasin B can increase the drug sensitivity of SKVLB1 to doxorubicin and paclitaxel. A formal assessment of drug synergy through isobolographic analysis (Fig. 6) and Chou-Talalay statistics (Fig. 7 and Table 5) further confirmed the potential utility of facilitating the cytotoxicity of currently approved agents with cytochalasins, as both cytochalasin B and DiHCB demonstrated notable synergism with doxorubicin and paclitaxel. The extent of the drug synergy between cytochalasin B, DiHCB, and doxorubicin against SKVLB1 was comparable to the activity we previously observed in P388/ADR leukemia [14], another multidrug resistant cell line. These observations, along with previous studies that noted drug synergy between cytochalasin B and cytarabine [36] as well as vincristine [37], provide compelling evidence that cytochalasin B and its reduced congener have clinically applicable synergistic potential.

These data are in alignment with the antineoplastic mechanisms of microfilament-disrupting agents such as cytochalasin B. Due to cytokinesis inhibition potentiated by this class of agents, neoplastic cells become enlarged and multinucleated; ideal targets for microtubule-directed (paclitaxel) and for nucleic acid-directed (doxorubicin) agents [1, 38]. Further, the concomitant perturbation of the cell cycle via microtubule-targeting G₂/M arrest and microfilament-targeting cytokinesis inhibition leaves two unique mechanisms that neoplastic cells would have to circumvent in order to continuously proliferate. Indeed, we have previously observed that concomitant administration of cytochalasin B and vincristine substantially precludes the clonogenic potential of U937 human monocytic leukemia, thereby potently inhibiting its propensity to proliferate [39]. Therefore, cytochalasins have unique microfilament-directed mechanisms that may substantiate potent drug synergy with agents that target microtubules or nucleic acids.

Interestingly, we have demonstrated that pulsed low-frequency ultrasound in the 20 to 40 kHz range is able to induce preferential destruction of neoplastic cells enlarged by treatment with cytoskeletal-directed agents [39, 40]. The ability of cytochalasins to affect multidrug resistant neoplastic cells presents the possibility of cell enlargement and multinucleation in these cells that has been observed in all other neoplastic cell lines tested. Consequently, cytochalasins may sensitize multidrug resistant cells to sonodynamic therapy with low frequency ultrasound, paralleling the effects obtained to this point with leukemic cell targets.

Currently, ovarian carcinoma presents significant clinical issues, as the 5 year survival rate for all stages and types is 44 %, while stage IV invasive ovarian carcinoma has a 5 year survival rate of 17 % [41]. Further, only 15 % of all ovarian tumors are found at stage I [41], indicating that clinicians often have to treat aggressive malignancies. These data suggest that novel antineoplastic agents need to be devised for the treatment of ovarian carcinoma. Cytochalasins offer novel mechanisms for exploitation in cancer therapy that may improve the efficacy of treatments against cancers refractory to standard chemotherapeutic protocols. In vivo efficacy of cytochalasins in preclinical models of drug resistant ovarian carcinoma has yet to be determined. Such preclinical investigation is warranted based on the results of this study.