Thermodynamic Analysis of Protein–Ligand Interactions in Complex Biological Mixtures using a Shotgun Proteomics Approach

DeArmond, Patrick D.; Xu, Ying; Strickland, Erin C; Daniels, Kyle G.; Fitzgerald, Michael C.

doi:10.1021/pr200403c

Cited by 63 publications

(85 citation statements)

References 41 publications

(96 reference statements)

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“…five times the number of peptide and proteins assayed in Gel Experiment 2, Solution Experiment 1B, or in Solution Experiment 2). This is ϳthree-fivefold more peptide and protein coverage than that previously reported in SPROX experiments using an isobaric mass tagging strategy (16). It is also noteworthy that the solution and gel-based protocols were to some degree complementary in their peptide and protein coverage.…”

Section: Fig 2 Schematic Representation Of Silac-sprox Data Expectementioning

confidence: 56%

“…Two energetics-based approaches, the stability of proteins from rates of oxidation (SPROX) 1 (10,16,17) and pulse proteolysis techniques (13,18), have shown promise for protein-ligand binding analyses on the proteomic scale, but so far have been limited in their proteomic coverage. Although the pulse pro-teolysis technique does utilize targeted mass spectrometrybased proteomics analyses for the identification of hit proteins, the technique relies on gel-based strategies for the resolution, detection, and quantitation of potential protein targets (13,18).…”

mentioning

confidence: 99%

“…This reliance on gel-based strategies for protein resolution, detection, and quantitation, ultimately limits the complexity of protein samples that can be interrogated for ligand binding. In contrast, the SPROX technique has been interfaced with conventional bottom-up shotgun proteomics platforms that exploit the capabilities of modern LC-MS/MS systems to resolve, detect, and quantify the protein components of complex biological mixtures (10,16,17).…”

mentioning

confidence: 99%

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Stable Isotope Labeling with Amino Acids in Cell Culture (SILAC)-Based Strategy for Proteome-Wide Thermodynamic Analysis of Protein-Ligand Binding Interactions

Tran

Adhikari

Fitzgerald

2014

Molecular & Cellular Proteomics

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109

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Section: Fig 2 Schematic Representation Of Silac-sprox Data Expectementioning

confidence: 56%

mentioning

confidence: 99%

mentioning

confidence: 99%

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Stable Isotope Labeling with Amino Acids in Cell Culture (SILAC)-Based Strategy for Proteome-Wide Thermodynamic Analysis of Protein-Ligand Binding Interactions

Tran

Adhikari

Fitzgerald

2014

Molecular & Cellular Proteomics

Self Cite

109

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“…The SPROX technique is a mass spectrometry-based approach for measuring the thermodynamic stability of proteins and protein-ligand complexes [26,27,29,30]. The technique has been previously validated using a series of different model systems, which have included both purified and unpurified proteins and protein-ligand complexes [27,29,30]. Of particular significance to the present study is that the SPROX technique does not require any special labeling of the ligand and that the technique is amenable to the thermodynamic analysis of protein-ligand binding reaction in whole cell lysates.…”

Section: Introductionmentioning

confidence: 99%

Thermodynamic Analysis of the Geldanamycin–Hsp90 Interaction in a Whole Cell Lysate Using a Mass Spectrometry-Based Proteomics Approach

Wallace

Fitzgerald

2016

J. Am. Soc. Mass Spectrom.

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Abstract. Geldanamycin is a natural product with well-established and potent anticancer activities. Heat shock protein 90 (Hsp90) is the known target of geldanamycin, which directly binds to Hsp90's N-terminal ATP binding domain and inhibits Hsp90's ATPase activity. The affinity of geldanamycin for Hsp90 has been measured in multiple studies. However, there have been large discrepancies between the reported dissociation constants (i.e., K d values), which have ranged from low nanomolar to micromolar. Here the stability of proteins from rates of oxidation (SPROX) technique was used in combination with an isobaric mass tagging strategy to measure the binding affinity of geldanamycin to unpurified Hsp90 in an MCF-7 cell lysate. The K d values determined here were dependent on how long geldanamycin was equilibrated with the lysate prior to SPROX analysis. The K d values determined using equilibration times of 0.5 and 24 h were 1 and 0.03 μM, respectively. These K d values, which are similar to those previously reported in a geldanamycinHsp90 binding study that involved the use of a fluorescently labeled geldanamycin analogue, establish that the slow-tight binding behavior previously observed for the fluorescently labeled geldanamycin analogue is not an artifact of the fluorescent label, but rather an inherent property of the geldanamycin-Hsp90 binding interaction. The slow-tight binding property of this complex may be related to time-dependent conformational changes in Hsp90 and/or to time-dependent chemical changes in geldanamycin, both of which have been previously proposed to explain the slow-tight binding behavior of the geldanamycin-Hsp90 complex.

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“…Therefore, the determination of the binding of small molecules to proteins has attracted considerable research attention in recent years [2][3][4]. Owing to large synthetic and natural product compound libraries becoming more easily accessible, the availability of efficient methods for the rapid screening of the binding of these compounds to proteins becomes imperative.…”

Section: Introductionmentioning

confidence: 99%

Screening of the Binding of Small Molecules to Proteins by Desorption Electrospray Ionization Mass Spectrometry Combined with Protein Microarray

Yao

Wang

Zhang

et al. 2015

J. Am. Soc. Mass Spectrom.

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Abstract. The interaction between bioactive small molecule ligands and proteins is one of the important research areas in proteomics. Herein, a simple and rapid method is established to screen small ligands that bind to proteins. We designed an agarose slide to immobilize different proteins. The protein microarrays were allowed to interact with different small ligands, and after washing, the microarrays were screened by desorption electrospray ionization mass spectrometry (DESI MS). This method can be applied to screen specific protein binding ligands and was shown for seven proteins and 34 known ligands for these proteins. In addition, a high-throughput screening was achieved, with the analysis requiring approximately 4 s for one sample spot. We then applied this method to determine the binding between the important protein matrix metalloproteinase-9 (MMP-9) and 88 small compounds. The molecular docking results confirmed the MS results, demonstrating that this method is suitable for the rapid and accurate screening of ligands binding to proteins.

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Thermodynamic Analysis of Protein–Ligand Interactions in Complex Biological Mixtures using a Shotgun Proteomics Approach

Cited by 63 publications

References 41 publications

Stable Isotope Labeling with Amino Acids in Cell Culture (SILAC)-Based Strategy for Proteome-Wide Thermodynamic Analysis of Protein-Ligand Binding Interactions

Stable Isotope Labeling with Amino Acids in Cell Culture (SILAC)-Based Strategy for Proteome-Wide Thermodynamic Analysis of Protein-Ligand Binding Interactions

Thermodynamic Analysis of the Geldanamycin–Hsp90 Interaction in a Whole Cell Lysate Using a Mass Spectrometry-Based Proteomics Approach

Screening of the Binding of Small Molecules to Proteins by Desorption Electrospray Ionization Mass Spectrometry Combined with Protein Microarray

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