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Literature DB >> 20142515

Heterospecies partition analysis reveals binding curve and stoichiometry of protein interactions in living cells.

Abstract

Measuring the binding curve and stoichiometry of protein complexes in living cells is a prerequisite for quantitative modeling of cellular processes. Dual-color fluorescence fluctuation spectroscopy provides a general framework for detecting protein interactions, but lacks suitable methods for quantifying protein heterointeractions in the cell. We address this challenge by introducing heterospecies partition (HSP) analysis for protein heterointeractions of the type D + nA<-->DA(n). HSP directly identifies the heterointeracting species from the sample mixture and determines the binding curve and stoichiometry of the protein complex. The HSP method is applied to provide the first direct characterization of the ligand-dependent binding of the retinoic X receptor to the coactivator transcription intermediate factor 2. A previous study based on protein fragments observed a higher binding stoichiometry than biologically expected. We address this difference in stoichiometry by measuring the binding curves of the full-length proteins in living cells. This study provides proof-of-principle experiments that illustrate the potential of HSP as a general and robust analysis tool for the quantitative characterization of protein heterointeractions by dual-color fluorescence fluctuation spectroscopy in living cells.

Entities: Gene

Mesh：

Substances：
Retinoid X Receptors

Year: 2010 PMID： 20142515 PMCID： PMC2840129 DOI： 10.1073/pnas.0905670107

Source DB: PubMed Journal: Proc Natl Acad Sci U S A ISSN： 0027-8424 Impact factor: 11.205

27 in total

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6. The human estrogen receptor alpha dimer binds a single SRC-1 coactivator molecule with an affinity dictated by agonist structure.

Authors: E Margeat; N Poujol; A Boulahtouf; Y Chen; J D Müller; E Gratton; V Cavailles; C A Royer
Journal: J Mol Biol Date: 2001-02-23 Impact factor: 5.469

7. Ligand-dependent interactions of coactivators steroid receptor coactivator-1 and peroxisome proliferator-activated receptor binding protein with nuclear hormone receptors can be imaged in live cells and are required for transcription.

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Journal: Proc Natl Acad Sci U S A Date: 2000-04-11 Impact factor: 11.205

8. Cumulant analysis in fluorescence fluctuation spectroscopy.

Authors: Joachim D Müller
Journal: Biophys J Date: 2004-06 Impact factor: 4.033

9. Intracellular calmodulin availability accessed with two-photon cross-correlation.

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Review 10. The nuclear receptor superfamily: the second decade.

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22 in total

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2. Measuring the stoichiometry of functional PspA complexes in living bacterial cells by single molecule photobleaching.

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3. Brightness analysis by Z-scan fluorescence fluctuation spectroscopy for the study of protein interactions within living cells.

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Heterospecies partition analysis reveals binding curve and stoichiometry of protein interactions in living cells.

1. Fluorescence-intensity distribution analysis and its application in biomolecular detection technology.

Review 2. The renaissance of fluorescence resonance energy transfer.

3. Probing protein oligomerization in living cells with fluorescence fluctuation spectroscopy.

4. Fluorescence fluctuation spectroscopy of mCherry in living cells.

5. High-order fluorescence fluctuation analysis of model protein clusters.

6. The human estrogen receptor alpha dimer binds a single SRC-1 coactivator molecule with an affinity dictated by agonist structure.

7. Ligand-dependent interactions of coactivators steroid receptor coactivator-1 and peroxisome proliferator-activated receptor binding protein with nuclear hormone receptors can be imaged in live cells and are required for transcription.

8. Cumulant analysis in fluorescence fluctuation spectroscopy.

9. Intracellular calmodulin availability accessed with two-photon cross-correlation.

Review 10. The nuclear receptor superfamily: the second decade.

1. Factors affecting the quantification of biomolecular interactions by fluorescence cross-correlation spectroscopy.

2. Measuring the stoichiometry of functional PspA complexes in living bacterial cells by single molecule photobleaching.

3. Brightness analysis by Z-scan fluorescence fluctuation spectroscopy for the study of protein interactions within living cells.

4. Characterization of brightness and stoichiometry of bright particles by flow-fluorescence fluctuation spectroscopy.

5. Comobility of GABARAP and Phosphatidylinositol 4-Kinase 2A on Cytoplasmic Vesicles.

6. An elegant way to quantitatively analyze oligomer formation in solution.

7. Fluorescence fluctuation spectroscopy enables quantitative imaging of single mRNAs in living cells.

8. Characterization of Ternary Protein Systems In Vivo with Tricolor Heterospecies Partition Analysis.

9. Identifying Heteroprotein Complexes in the Nuclear Envelope.

10. Quantifying Protein-mRNA Interactions in Single Live Cells.