Interaction of P-Glycoprotein with Defined Phospholipid Bilayers:  A Differential Scanning Calorimetric Study

Romsicki, Yolanda; Sharom, Frances J.

doi:10.1021/bi963120l

Cited by 43 publications

(52 citation statements)

References 42 publications

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“…In the case of Pgp, it appears that a rate-limiting step is, in fact, enhanced when the host lipid is in the gel phase. Along the same lines, we recently reported [35] that Pgp was reconstituted into Myr 2GroPCho with higher efficiency and specific ATPase activity at temperatures below t m , suggesting that the protein may have a preference for gel-phase lipid. Clearly, the nature of the chemical barrier for catalysis by Pgp is affected by the lipid-phase state quite differently than for other membrane-bound enzymes.…”

Section: Discussionmentioning

confidence: 53%

“…SDS/PAGE was carried out as described previously [22]. Differential scanning calorimetry (DSC) measurements were used to determine the gel/ liquid-crystalline phase transition temperature, t m , of liposomes of PamMyrGroPCho and Myr 2 GroPCho alone, and proteoliposomes of PamMyrGroPCho and Myr 2 GroPCho containing 13:1 (by mass) and 10:1 (by mass) Pgp, respectively, as described previously [35].…”

Section: Methodsmentioning

confidence: 99%

“…Pgp purified to Ͼ 90% purity was fluorescently labeled with 2-(4′-maleimidylanilino)naphthalene-6-sulfonic acid (MIANS) as described previously [30]. MIANS-labeled Pgp was then reconstituted into PamMyrGroPCho or Myr 2 GroPCho proteoliposomes as outlined above [35], except that dithioerythritol was omitted from the lipid-solubilization buffer and the Sephadex G-50 column buffer. The proteoliposomes, which had a final lipid/protein ratio of Ϸ10:1 (by mass) were resuspended in 50 mM Tris/HCl, 0.15 M NH 4 Cl, 5 mM MgCl 2 , 0.02% (mass/ vol.)…”

Section: Methodsmentioning

confidence: 99%

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The ATPase and ATP‐binding functions of P‐glycoprotein

Romsicki

Sharom

1998

European Journal of Biochemistry

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P-glycoprotein functions as an active efflux pump for lipophilic compounds and plays an important role in the resistance of human cancers to chemotherapeutic drugs. Drug transport is powered by ATP hydrolysis at two highly conserved nucleotide-binding domains, which are proposed to be located at the cytosolic face of the protein. The ATPase activity of P-glycoprotein depends on the presence of phospholipids, and various lipids affect both basal ATPase activity and its stimulation or inhibition by drug substrates. The modulating effects of the lipid-phase state and effects on the function of the nucleotidebinding domains of P-glycoprotein have been studied in reconstituted vesicles of the synthetic phospholipids 1-palmitoyl-2-myristoylphosphatidylcholine (PamMyrGroPCho) and dimyristoylphosphatidylcholine (Myr 2GroPCho). The kinetic parameters for P-glycoprotein ATPase activity were determined, and a fluorescence-quenching technique was used to measure the K d for ATP binding. The values of both the K m for ATP hydrolysis and K d for ATP binding were significantly different above and below the gel/liquidcrystalline phase transition temperature (t m) of PamMyrGroPCho and Myr2GroPCho, whereas they were similar at the same temperatures for P-glycoprotein in detergent solution. A discontinuity at 21Ϫ24°C was observed in the Arrhenius plots of P-glycoprotein ATPase activity in a membrane environment, but not in detergent solution. In addition, the activation energies for ATP hydrolysis in the gel and liquidcrystalline phases of the lipid bilayer were significantly different. P-glycoprotein in PamMyrGroPCho bilayers displayed an unusually low activation energy just below the melting transition. These results indicate that both ATP binding and ATP hydrolysis by P-glycoprotein are affected by the phase state of the host lipids in which it is reconstituted. Lipids may modulate the function of the nucleotide-binding domains of P-glycoprotein by interacting with the transmembrane regions of the protein, or the nucleotidebinding domains themselves may interact with the surface of the bilayer.

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Section: Discussionmentioning

confidence: 53%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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The ATPase and ATP‐binding functions of P‐glycoprotein

Romsicki

Sharom

1998

European Journal of Biochemistry

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“…Detergents and additional adjuvants from the purification and reconstitution procedures can affect the behavior of the transporter, as we have shown for CHAPS. The most frequently used detergents for the purification of P-gp beside CHAPS (26,28,29,32,39,42) are n-octyl b-D-glucopyranoside (octyl glucoside) (27,30,(49)(50)(51)(52)(53) and n-dodecyl or n-decyl b-Dmaltoside (14,22,25,33,51,(54)(55)(56). Octyl glucoside had activating as well as inhibiting effects on the ATPase activity of CHAPS-solubilized P-gp, depending on the glucoside concentration (39).…”

Section: Discussionmentioning

confidence: 99%

P-Glycoprotein in Proteoliposomes with Low Residual Detergent: The Effects of Cholesterol

et al. 2007

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Purpose. There is evidence that cholesterol affects the ATPase and transport functions of P-glycoprotein (P-gp). To study the influence of cholesterol on P-gp in a well defined lipid environment, we reconstituted P-gp in egg phosphatidylcholine (PhC) and PhC/cholesterol proteoliposomes with negligible residual amounts of detergents. Materials and methods. P-gp proteoliposomes were prepared by continuous dialysis from micelles consisting of P-gp, lipids, sodium dodecyl sulfate and cholate. Basal and modulator-induced ATPase activities were studied in an established enzyme assay. Modulator affinities to P-gp and to the lipid bilayers were determined by equilibrium dialysis. Results. In the absence of cholesterol the basal ATPase activity was six fold lower than in the presence of 20 or 40% cholesterol, and no P-gp binding and ATPase induction was detected for the tested modulators verapamil and progesterone. In proteoliposomes containing 20 and 40% cholesterol, respectively, the modulators showed significant P-gp binding and ATPase activation. The concentration of the modulators for half maximal activation of the ATPase was higher with 40% than with 20% cholesterol. Conclusions. Cholesterol influences P-gp in three ways: (a) it enhances its basal ATPase activity, (b) it renders P-gp sensitive towards the modulators verapamil and progesterone and (c) it affects the modulator concentration at half maximal ATPase activation.

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“…The linearity of the plots indicated that single overall rate-limiting steps were being observed. In contrast, some plasma membrane preparations and Pgp reconstituted in synthetic lipid mixtures did not produce linear Arrhenius relationships due to lipid phase transitions and other effects (43)(44)(45). Arrhenius relationships were measured for the drugs listed above as a function of concentration such that all phases of drug-dependent ATPase activities were investigated.…”

Section: Tight Coupling Of Atp-binding and Drug Transport Sites-mentioning

confidence: 99%

Transition State Analysis of the Coupling of Drug Transport to ATP Hydrolysis by P-glycoprotein

Al‐Shawi

Polar

Omote

et al. 2003

Journal of Biological Chemistry

160

221

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, from which we calculated the intrinsic enthalpic, entropic, and free energy terms for the rate-limiting transition states. Linearity of the Arrhenius plots indicated that the same rate-limiting step was being measured over the temperature range employed. Using linear free energy analysis, two distinct transition states were found: one associated with uncoupled basal activity and the other with coupled drug transport activity. We concluded that basal ATPase activity associated with Pgp is not a consequence of transport of an endogenous lipid or other endogenous substrates. Rather, it is an intrinsic mechanistic property of the enzyme. We also found that rapidly transported substrates bound tighter to the transition state and required fewer conformational alterations by the enzyme to achieve the coupling transition state. The overall rate-limiting step of Pgp during transport is a carrier reorientation step.

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Interaction of P-Glycoprotein with Defined Phospholipid Bilayers: A Differential Scanning Calorimetric Study

Cited by 43 publications

References 42 publications

The ATPase and ATP‐binding functions of P‐glycoprotein

The ATPase and ATP‐binding functions of P‐glycoprotein

P-Glycoprotein in Proteoliposomes with Low Residual Detergent: The Effects of Cholesterol

Transition State Analysis of the Coupling of Drug Transport to ATP Hydrolysis by P-glycoprotein

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