In vitro and in vivo evaluation of WK-X-34, a novel inhibitor of P-glycoprotein and BCRP, using radio imaging techniques

Abstract

Overexpression of the multidrug resistance proteins P‐glycoprotein (Pgp) and breast cancer resistance protein (BCRP) results in treatment failure of many malignancies including ovarian cancer. Dual inhibition of Pgp and BCRP may restore the sensitivity of resistant cells to anticancer drugs. We report the synthesis and characterization of a novel anthranilic‐acid based Pgp and BCRP modulator, WK‐X‐34. In vitro inhibition of Pgp activity was evaluated using ^99m^Tc‐Sestamibi and daunorubicin accumulation in Pgp overexpressing human ovarian cancer cells (A2780/Adr) and its sensitive counterpart (A2780/wt). Interaction with BCRP was examined with a mitoxantrone‐efflux assay in BCRP‐overexpressing MCF7/mx cells, with flow cytometry. Interactions with the multidrug resistance associated proteins (MRP) were evaluated in transfected MRP1, MRP2 and MRP3 cell lines, using a 5‐CFDA efflux assay. In vivo^99m^Tc‐Sestamibi imaging of human ovarian cancer xenografts was used to evaluate the in vivo efficacy of WK‐X‐34 in mice. Daunorubicin accumulation in A2780/Adr cells was inhibited by WK‐X‐34 at nanomolar concentrations (IC~50~: 82.1 ± 6 nM). WK‐X‐34 inhibited mitoxantrone accumulation in BCRP‐overexpressing cells at micromolar concentrations (IC~50~ = 26.5 ± 4.6 μM), whereas WK‐X‐34 did not significantly alter 5‐CFDA accumulation in MRP transfected cells. In vivo, uptake of ^99m^Tc‐Sestamibi was significantly increased in A2780/Adr xenograft tumors, brain and intestine (AUCs~0‐4h~ 136%, 147% and 138%; p < 0.05) in mice dosed with WK‐X‐34 (20 mg/kg i.p.). WK‐X‐34 selectively modulates Pgp and BCRP in vitro and in vivo in multidrug resistant ovarian cancer cells, and thus may have potential utility in the treatment of multidrug resistant tumors. © 2006 Wiley‐Liss, Inc.