dimerization of abcg2 analysed by bimolecular fluorescence complementation二聚abcg2分析的双分子荧光互补.pdfVIP
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dimerization of abcg2 analysed by bimolecular fluorescence complementation二聚abcg2分析的双分子荧光互补
Dimerization of ABCG2 Analysed by Bimolecular
Fluorescence Complementation
Ameena J. Haider, Deborah Briggs, Tim J. Self, Hannah L. Chilvers, Nicholas D. Holliday, Ian D. Kerr*
School of Biomedical Sciences, University of Nottingham, Nottingham, United Kingdom
Abstract
ABCG2 is one of three human ATP binding cassette transporters that are functionally capable of exporting a diverse range of
substrates from cells. The physiological consequence of ABCG2 multidrug transport activity in leukaemia, and some solid
tumours is the acquisition of cancer multidrug resistance. ABCG2 has a primary structure that infers that a minimal
functional transporting unit would be a homodimer. Here we investigated the ability of a bimolecular fluorescence
complementation approach to examine ABCG2 dimers, and to probe the role of individual amino acid substitutions in dimer
formation. ABCG2 was tagged with fragments of venus fluorescent protein (vYFP), and this tagging did not perturb
trafficking or function. Co-expression of two proteins bearing N-terminal and C-terminal fragments of YFP resulted in their
association and detection of dimerization by fluorescence microscopy and flow cytometry. Point mutations in ABCG2 which
may affect dimer formation were examined for alterations in the magnitude of fluorescence complementation signal.
Bimolecular fluorescence complementation (BiFC) demonstrated specific ABCG2 dimer formation, but no changes in dimer
formation, resulting from single amino acid substitutions, were detected by BiFC analysis.
Citation: Haider AJ, Briggs D, Self TJ, Chilvers HL, Holliday ND, et al. (2011) Dimerization of ABCG2 Analysed by Bimolecular Fluorescence Complementation. PLoS
ONE 6(10): e25818. doi:10.1371/journal.pone.0025818
Editor: Hendrik W. van Veen, University of Cambridge, United Kingdom
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