Abstract

Drug targets are typically confined to a single organelle population within a cell. Likewise, drugs themselves often have the tendency to selectively accumulate within specific cellular compartments. Our research is focused on understanding driving forces important in the transport of small molecule type drugs within the array of intracellular compartments associated with mammalian cells.
We aim to use this understanding to rationally develop novel drug delivery strategies to maximize the interaction of a drug with its target in the context of a single cell. The goal of the research outlined in this application is to understand mechanisms that are involved in the sequestration of anti-cancer drugs into cytoplasmic organelles of multi-drug resistant (MDR) cancer cell lines and is a process that does not seem to occur in drug sensitive cells. This sequestration has been shown to cause drastic reductions in the amount of drug available to partition into cellular compartments housing drug targets. For experiments outlined in this application, we have acquired three pairs of human leukemic cell lines. Each pair is comprised of a drug sensitive line and its corresponding MDR variant created through drug selection. We have shown that each MDR variant is able to sequester the anticancer drug, daunorubicin, into distinct cytoplasmic organelles. The first segment of this application is focused on identifying drug sequestering organelle(s). The sequestration will be assessed using a series of fluorescent molecules with different physicochemical properties, which will broadly represent different categories of anticancer agents. Drug sequestering organelles will be identified using fluorescence co-localization studies with organelle specific fluorescent probes and vital stains. The second phase of this application describes methods used to reveal the fundamental mechanisms involved in drug sequestration. Comparative proteomic approaches will be used to determine differences in protein expression between drug sequestering organelles isolated from MDR cells and the same organelles isolated from drug sensitive cells. To confirm their involvement in drug sequestration, identified proteins will be specifically down-regulated in MDR cells, and the sequestration capacity will be reevaluated. The final phase of this application will examine the substrate specificity for sequestration in identified organelles. We will utilize novel quantitative assays to measure drug accumulation into sequestering organelles. Using these assays, structure transport relationships will be designed in order to identify the key structural requirements that are essential for drug sequestration. Together these studies will give us a fundamental understanding of this drug sequestration phenotype. This understanding will guide us in the development of novel drug design/modification strategies that will be useful in producing drugs with reduced sequestration tendency and, therefore, an improved capacity to interact with relevant target sites within MDR cancer cells.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA106655-03
Application #
7194224
Study Section
Drug Discovery and Molecular Pharmacology Study Section (DMP)
Program Officer
Forry, Suzanne L
Project Start
2005-01-01
Project End
2009-12-31
Budget Start
2007-01-01
Budget End
2007-12-31
Support Year
3
Fiscal Year
2007
Total Cost
$205,489
Indirect Cost

  Institution

Name
University of Kansas Lawrence
Department
Pharmacology
Type
Schools of Pharmacy
DUNS #
076248616
City
Lawrence
State
KS
Country
United States
Zip Code
66045

  Publications

Funk, Ryan S; Krise, Jeffrey P (2012) Cationic amphiphilic drugs cause a marked expansion of apparent lysosomal volume: implications for an intracellular distribution-based drug interaction. Mol Pharm 9:1384-95
Ndolo, Rosemary A; Luan, Yepeng; Duan, Shaofeng et al. (2012) Lysosomotropic properties of weakly basic anticancer agents promote cancer cell selectivity in vitro. PLoS One 7:e49366
Goldman, Stephen D B; Krise, Jeffrey P (2010) Niemann-Pick C1 functions independently of Niemann-Pick C2 in the initial stage of retrograde transport of membrane-impermeable lysosomal cargo. J Biol Chem 285:4983-94
Ndolo, Rosemary A; Forrest, M Laird; Krise, Jeffrey P (2010) The role of lysosomes in limiting drug toxicity in mice. J Pharmacol Exp Ther 333:120-8
Ndolo, Rosemary A; Jacobs, Damon T; Forrest, M Laird et al. (2010) Intracellular Distribution-based Anticancer Drug Targeting: Exploiting a Lysosomal Acidification Defect Associated with Cancer Cells. Mol Cell Pharmacol 2:131-136
Kaufmann, A M; Goldman, S D B; Krise, J P (2009) A fluorescence resonance energy transfer-based approach for investigating late endosome-lysosome retrograde fusion events. Anal Biochem 386:91-7
Goldman, Stephen D B; Funk, Ryan S; Rajewski, Roger A et al. (2009) Mechanisms of amine accumulation in, and egress from, lysosomes. Bioanalysis 1:1445-59
Kaufmann, Allyn M; Krise, Jeffrey P (2008) Niemann-Pick C1 functions in regulating lysosomal amine content. J Biol Chem 283:24584-93
Kaufmann, Allyn M; Toro-Ramos, Alana J; Krise, Jeffrey P (2008) Assessment of golgi apparatus versus plasma membrane-localized multi-drug resistance-associated protein 1. Mol Pharm 5:787-94
Kaufmann, Allyn M; Krise, Jeffrey P (2007) Lysosomal sequestration of amine-containing drugs: analysis and therapeutic implications. J Pharm Sci 96:729-46

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