Abstract
ABCG2 is an exporter type ABC protein that can expel numerous chemically unrelated xeno- and endobiotics from cells. When expressed in tumor cells or tumor stem cells, ABCG2 confers multidrug resistance, contributing to the failure of chemotherapy.
Molecular details orchestrating substrate translocation and ATP hydrolysis remain elusive. Here we present methods to concomitantly investigate substrate and nucleotide binding by ABCG2 in cells. Using the conformation-sensitive antibody 5D3, we show that the switch from the inward-facing (IF) to the outward-facing (OF) conformation of ABCG2 is induced by nucleotide binding. IF-OF transition is facilitated by substrates, and hindered by the inhibitor Ko143. Direct measurements of 5D3 and substrate binding to ABCG2 indicate that the high-to-low affinity switch of the drug binding site coincides with the transition from the IF to the OF conformation. Low substrate binding persists in the post-hydrolysis state, supporting that dissociation of the ATP hydrolysis products is required to reset the high substrate affinity IF conformation of ABCG2.
Competing Interest Statement
The authors have declared no competing interest.
Abbreviations
- A647
- Alexa 647 succinimidyl ester
- ABCP
- Placenta-Specific ABC transporter
- ADME-Tox
- absorption, distribution, metabolism, excretion and toxicity
- AMP-PNP
- adenylyl-imidodiphosphate
- BCRP
- Breast Cancer Resistance Protein
- E3S
- estrone-3-sulfate
- cryo-EM
- cryogenic electron microscopy
- CFTR
- Cystic Fibrosis Transmembrane Conductance Regulator (ABCC7)
- FCS
- fluorescence correlation spectroscopy
- FBS
- foetal bovine serum
- GFP
- green fluorescent protein
- IF
- inward-facing
- mAb
- monoclonal antibody
- MX
- mitoxantrone
- MXR
- Mitoxantrone Resistance Protein
- NBD
- nucleotide binding domain
- OF
- outward-facing
- PI
- propidium iodide
- SLO
- streptolysin-O
- TMD
- transmembrane domain
- Vi
- vanadate
