TY - JOUR T1 - Analogues of tetramethylrosamine as transport molecules for and inhibitors of P-glycoprotein-mediated multidrug resistance. AU - Gibson,Scott L, AU - Hilf,Russell, AU - Donnelly,David J, AU - Detty,Michael R, PY - 2004/05/24/received PY - 2004/06/25/revised PY - 2004/06/26/accepted PY - 2004/9/11/pubmed PY - 2005/8/16/medline PY - 2004/9/11/entrez SP - 4625 EP - 31 JF - Bioorganic & medicinal chemistry JO - Bioorg Med Chem VL - 12 IS - 17 N2 - Tetramethylrosamine and its thio- and seleno- analogues (TMR-O, TMR-S, and TMR-Se, respectively) were examined for their ability to be transported by Pgp into chemo-resistant CR1R12 cells. Verapamil (7 x 10(-6)M) enhanced the uptake of TMR-O and TMR-S into CR1R12 cells compared to those cultures not previously exposed to verapamil. The uptake of TMR-O and TMR-S in CR1R12 cells in the presence of 7 x 10(-6)M verapamil was equivalent to its uptake in the chemo-sensitive parent cell line AUXB1 in the absence or presence of verapamil. None of the TMR analogues were effective alone as photosensitizers of CR1R12 cells. However, when either TMR-S or TMR-Se was added to CR1R12 cells after 7 x 10(-6)M verapamil exposure for 2h, irradiation of cultures with 5.0J cm(-2) of 350-750 nm light caused significant phototoxicity. TMR-O showed no significant phototoxicity in the presence of verapamil. Chemo-sensitive AUXB1 cells are equally susceptible to phototoxicity using TMR-Se with or without previous exposure to verapamil. The Pgp modulators verapamil and CsA increased the uptake of CAM into CR1R12. Exposure of CR1R12 cells to TMR-S or TMR-Se for 2h in the dark resulted in no significant change in the intracellular accumulation of CAM. However, 1h of light exposure after incubation of cells with TMR-S or TMR-Se resulted in an up to 2-fold increase in CAM uptake. SN - 0968-0896 UR - https://www.unboundmedicine.com/medline/citation/15358289/Highly_potent_PDE4_inhibitors_with_therapeutic_potential DB - PRIME DP - Unbound Medicine ER -