Vanadate trapping of nucleotide at the ATP-binding sites of human multidrug resistance P-glycoprotein exposes different residues to the drug-binding site

Loo, Tip W.; Clarke, David M.

doi:10.1073/pnas.022049799

Cited by 72 publications

(76 citation statements)

References 59 publications

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“…A sample of the membrane was then incubated in the presence or absence of various concentrations of vinblastine, cyclosporin A, or rhodamine B for 15 min at 20°C. The samples were then cooled on ice for 10 min and treated with 0.2 mM concentrations of the homobifunctional methanethiosulfonate cross-linker 3,6,9,12-tetraoxatetradecane-1,14-diylbismethanethiosulfonate (M14M, 20.8 Å) (Toronto Research Chemicals, Toronto, ON) for 4 min on ice (9,22). The reactions were stopped by the addition of 2ϫ SDS sample buffer (125 mM Tris-HCl, pH 6.8, 20% (v/v) glycerol, and 4% (w/v) SDS) containing 50 mM EDTA and no reducing agent.…”

Section: Methodsmentioning

confidence: 99%

Arginines in the First Transmembrane Segment Promote Maturation of a P-glycoprotein Processing Mutant by Hydrogen Bond Interactions with Tyrosines in Transmembrane Segment 11

Loo

Bartlett

Clarke

2008

Journal of Biological Chemistry

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A key goal is to correct defective folding of mutant ATP binding cassette (ABC) transporters, as they cause diseases such as cystic fibrosis. P-glycoprotein (ABCB1) is a useful model system because introduction of an arginine at position 65 of the first transmembrane (TM) segment could repair folding defects. To determine the mechanism of arginine rescue, we first tested the effects of introducing arginines at other positions in TM1 (residues 52-72) of a P-glycoprotein processing mutant (G251V) that is defective in folding and trafficking to the cell surface (20% maturation efficiency). We found that arginines introduced into one face of the TM1 helix (positions 52, 55, 56, 59, 60, 62, 63, 66, and 67) inhibited maturation, whereas arginines on the opposite face of the helix promoted (positions 64, 65, 68, and 71) or had little effect (positions 61, and 69) on maturation. Arginines at positions 61, 64, 65, and 68 appeared to lie close to the drug binding sites as they reduced the apparent affinity for drug substrates such as vinblastine and verapamil. Therefore, arginines that promoted maturation may face an aqueous drug translocation pathway, whereas those that inhibited maturation may face the lipid bilayer. The highest maturation efficiencies (60 -85%) were observed with the Arg-65 and Arg-68 mutants. Mutations that removed hydrogen bond acceptors (Y950F/Y950A or Y953F/Y953A) in TM11 predicted to lie close to Arg-65 or Arg-68 inhibited maturation but did not affect maturation of the G251V parent. Therefore, arginine may rescue defective folding by promoting packing of the TM segments through hydrogen bond interactions.

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Section: Methodsmentioning

confidence: 99%

Arginines in the First Transmembrane Segment Promote Maturation of a P-glycoprotein Processing Mutant by Hydrogen Bond Interactions with Tyrosines in Transmembrane Segment 11

Loo

Bartlett

Clarke

2008

Journal of Biological Chemistry

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“…Cross-linking in the absence of vanadate was done at 37°C rather than 4°C because molecular motion might make it easier to form cross-links. Vanadate trapping of nucleotide locks the protein in the transition state (38) and can alter the conformational state of P-gp (39). For most of the mutants (e.g.…”

Section: Residue Tyrmentioning

confidence: 99%

Introduction of the Most Common Cystic Fibrosis Mutation (ΔF508) into Human P-glycoprotein Disrupts Packing of the Transmembrane Segments

Loo

Bartlett

Clarke

2002

Journal of Biological Chemistry

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The most common mutation in cystic fibrosis (deletion of phenylalanine 508 (⌬F508) in the cystic fibrosis conductance transmembrane regulator (CFTR) gene) causes defective synthesis of CFTR protein. To understand how this deletion interferes with protein folding, we made the equivalent deletion (⌬Y490) in P-glycoprotein (P-gp). A Cys-less P-gp with cysteines in transmembrane (TM) 4 or TM5 can be cross-linked with a cysteine in TM12. Deleting Tyr 490 in P-gp resulted in an inactive and defectively processed mutant in which no crosslinking between TM4 or TM5 and TM12 was detected. Expression of the ⌬Y490 mutant in the presence of a chemical chaperone corrected the processing defect and yielded active P-gp mutants that could be cross-linked between TM4 or TM5 and TM12. Cross-linking between TM4 or TM5 and TM12 was also detected when residues 483 TIAENIRYG 491 in P-gp were replaced with residues 501 TIKENIIFG 509 from CFTR (P-gp/CFTR). Deleting Phe 508 in the P-gp/CFTR chimera, however, caused defective processing of the mutant protein and no detectable cross-linking between TM4 or TM5 and TM12. The processing defect was corrected with a chemical chaperone and yielded active P-gp/CFTR mutant proteins that could be cross-linked. These results show that deletion at residue 490 disrupts packing of the TM segments possibly by affecting interaction between the first nucleotide-binding domain (Tyr 490 ) and the first cytoplasmic loop (Glu 184 ).

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“…In addition to this model of P-glycoprotein, another model has been proposed, which consists of two membrane-embedded sixteen-strand β-barrels, connected by short loops to two six-helix bundles beneath each barrel [45,46]. The involvement of TM segments and NBDs in substrate recognition and ATP binding/hydrolysis, respectively, have been established [47][48][49][50][51][52]. Substantial biochemical evidence, including changes in drug binding, epitope accessibility, fluorescent and spectroscopic measurements, and protease susceptibility [53][54][55][56][57][58][59], suggests that TM segments undergo conformational change upon nucleotide binding.…”

Section: P-gp Structure and Functionmentioning

confidence: 99%

“…Considerable effort has been invested in characterizing drug resistance changes caused by Pglycoprotein mutations [52,53,[127][128][129][130][131][132][133][134][135][136][137][138][139][140][141][142][143][144][145]. P-glycoprotein mutations that have appeared in cultured cells selected for resistance to particular drugs [130][131][132], and mutations incorporated by site-directed mutagenesis have been evaluated [52,53,127,129,[134][135][136][137][138][139][140][141][142][143][144][145].…”

Section: B Analysis Of Mutations Affecting the Drug Binding Sites Ofmentioning

confidence: 99%

Identification and Characterization of the Binding Sites of P-Glycoprotein for Multidrug Resistance-Related Drugs and Modulators

Safa

2004

CMCACA

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A major problem in cancer treatment is the development of resistance to multiple chemotherapeutic agents in tumor cells. A major mechanism of this multidrug resistance (MDR) is overexpression of the MDR1 product P-glycoprotein, known to bind to and transport a wide variety of agents. This review concentrates on the progress made toward understanding the role of this protein in MDR, identifying and characterizing the drug binding sites of P-glycoprotein, and modulating MDR by P-glycoprotein-specific inhibitors. Since our initial discovery that Pglycoprotein binds to vinblastine photoaffinity analogs, many P-glycoprotein-specific photoaffinity analogs have been developed and used to identify the particular domains of Pglycoprotein capable of interacting with these analogs and other P-glycoprotein substrates. Furthermore, significant advances have been made in delineating the drug binding sites of this protein by studying mutant P-glycoprotein. Photoaffinity labeling experiments and the use of sitedirected antibodies to several domains of this protein have allowed the localization of the general binding domains of some of the cytotoxic agents and MDR modulators on P-glycoprotein. Moreover, site-directed mutagenesis studies have identified the amino acids critical for the binding of some of these agents to P-glycoprotein. Furthermore, equilibrium binding assays using plasma membranes from MDR cells and radioactive drugs have aided our understanding of the modes of drug interactions with P-glycoprotein. Based on the available data, a topological model of Pglycoprotein and the approximate locations of its drug binding sites, as well as a proposed classification of multiple drug binding sites of this protein, is presented in this review.

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Vanadate trapping of nucleotide at the ATP-binding sites of human multidrug resistance P-glycoprotein exposes different residues to the drug-binding site

Cited by 72 publications

References 59 publications

Arginines in the First Transmembrane Segment Promote Maturation of a P-glycoprotein Processing Mutant by Hydrogen Bond Interactions with Tyrosines in Transmembrane Segment 11

Arginines in the First Transmembrane Segment Promote Maturation of a P-glycoprotein Processing Mutant by Hydrogen Bond Interactions with Tyrosines in Transmembrane Segment 11

Introduction of the Most Common Cystic Fibrosis Mutation (ΔF508) into Human P-glycoprotein Disrupts Packing of the Transmembrane Segments

Identification and Characterization of the Binding Sites of P-Glycoprotein for Multidrug Resistance-Related Drugs and Modulators

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