Enrichment strategies for phosphoproteomics: state-of-the-art

Šalovská, Barbora; Tichý, Aleš; Řezáčová, Martina; Vávrová, Jiřina; Novotná, Eva

doi:10.1515/revac-2011-0025

Cited by 9 publications

(5 citation statements)

References 138 publications

(124 reference statements)

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“…Systematic identication and characterization of phosphoproteins is vital to help us understand this important modication; however, it remains a challenging task due to the relatively low abundance of phosphorylated proteins in biological samples. [3][4][5] Current approaches to capture phosphoproteins generally rely on the interaction of phosphate anions with metal ions, such as in immobilized metal affinity chromatography (IMAC) and in metal oxide affinity chromatography (MOAC). [6][7][8][9][10] Even though these techniques have been demonstrated with success to a certain extent, some disadvantages are encountered with these techniques: including poor selectivity, low adsorption efficiency and signicant loss of phosphorylated proteins during the wash steps.…”

Section: Introductionmentioning

confidence: 99%

Guanidinium functionalized superparamagnetic silica spheres for selective enrichment of phosphopeptides and intact phosphoproteins from complex mixtures

Deng

Yang

et al. 2014

J. Mater. Chem. B

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Section: Introductionmentioning

confidence: 99%

Guanidinium functionalized superparamagnetic silica spheres for selective enrichment of phosphopeptides and intact phosphoproteins from complex mixtures

Deng

Yang

et al. 2014

J. Mater. Chem. B

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“…Thus, the study of protein phosphorylation states is important for defining protein kinase substrates, and revealing the activation states of signal transduction pathways. [5][6][7] Currently, high-throughput proteomic analysis is mainly accomplished by mass spectrometry (MS). 8 However, the determination of phosphopeptides in complex biological samples has remained a significant challenge because their scarcity in the total proteome as well as their deficient ionization and ion suppression during the mass spectrometric analysis.…”

Section: Introductionmentioning

confidence: 99%

Zinc Ion-immobilized Magnetic Microspheres for Enrichment and Identification of Multi-phosphorylated Peptides by Mass Spectrometry

et al. 2017

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The selective isolation of phosphorylated peptides and subsequent analysis using mass spectrometry is important for understanding how protein kinase and phosphatase signals can precisely modulate the on/off states of signal transduction pathways. However, the isolation and detection of multi-phosphorylated peptides is still limited due to their distinct affinity to various materials and their poor ionization efficiency. Here, we report a highly efficient and selective enrichment of phosphorylated peptides using binuclear Zn 2+ -dipicolylamine complex-coated magnetic microspheres (ZnMMs). ZnMMs can utilize the rapid and selective isolation/enrichment of phosphorylated peptides and the subsequent mass spectrometric analysis, given the intrinsic magnetic property of magnetic microspheres and the highly selective binding ability of the binuclear Zn 2+ -dipicolylamine complex to phosphate groups. α-Casein and β-casein were chosen for a proof-of-concept demonstration. We contemplated that phosphopeptides were selectively isolated and enriched from both the tryptic digests of casein proteins and mixed samples with a high degree of sensitivity by facilitating ZnMMs. Especially, ZnMMs showed high efficiency with multi-phosphopeptides, which are in general difficult to be examined by mass analysis on account of their poor ionization efficiency. For the model protein α, β-casein mixture of the tryptic digest, 17 phosphopeptides were identified with ZnMMs and 82% of the enriched phosphopeptides were multiphosphorylated peptides, indicating that ZnMMs have excellent enrichment efficiency and strong affinity towards multiphosphorylated peptides.

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“…Substantial research efforts have been devoted to improve separation and identification of phosphoproteome by chromatographic techniques and mass spectrometry. − Still, this remains a challenging task, because phosphopeptides are present at very low abundancetypically <5% in a complex protein digestand their MS signals could be suppressed by the nonphosphorylated ones. One effective solution is to selectively enrich the phosphorylated proteins or peptides prior to MS detection. , …”

Section: Introductionmentioning

confidence: 99%

“…One effective solution is to selectively enrich the phosphorylated proteins or peptides prior to MS detection. 9,10 Antibodies or phosphoprotein-binding domains (PBDs) have been employed to isolate phosphorylated proteins or peptides with high specificity. 11,12 However, neither is readily available and both are expensive to obtain.…”

Section: ■ Introductionmentioning

confidence: 99%

ZrO₂ Nanofiber as a Versatile Tool for Protein Analysis

Wang

Duan

Zhong

2015

ACS Appl. Mater. Interfaces

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Phosphorylation is one of the most important post-translational modifications in proteins. Their essential roles in the regulation of cellular processes and alteration of protein-protein interaction networks have been actively studied. However, phosphorylated proteins are present at low abundance in cells, and ionization of the modified peptides is often suppressed by the more abundant species in mass spectrometry. Effective enrichment techniques are needed to remove the unmodified peptides and concentrate the phosphorylated ones before their identification and quantification. Herein, we prepared ZrO2 nanofibers by electrospinning, a straightforward and easy fabrication technique, and applied them to enrich phosphorylated peptides and proteins. The fibers showed good size homogeneity and porosity and could specifically bind to the phosphorylated peptides and proteins, allowing their separation from the unmodified analogues when present in either simple protein digests or highly complex cell lysates. The enrichment performance was superior to that of the commercially available nanoparticles. Moreover, modifying the solution pH could lead to selective adsorption of proteins with different pI values, suggesting the fibers' potential applicability in charge-based protein fractionation. Our results support that the electrospun ZrO2 nanofibers can serve as a versatile tool for protein analysis with great ease in preparation and handling.

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Enrichment strategies for phosphoproteomics: state-of-the-art

Cited by 9 publications

References 138 publications

Guanidinium functionalized superparamagnetic silica spheres for selective enrichment of phosphopeptides and intact phosphoproteins from complex mixtures

Guanidinium functionalized superparamagnetic silica spheres for selective enrichment of phosphopeptides and intact phosphoproteins from complex mixtures

Zinc Ion-immobilized Magnetic Microspheres for Enrichment and Identification of Multi-phosphorylated Peptides by Mass Spectrometry

ZrO₂ Nanofiber as a Versatile Tool for Protein Analysis

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Enrichment strategies for phosphoproteomics: state-of-the-art

Cited by 9 publications

References 138 publications

Guanidinium functionalized superparamagnetic silica spheres for selective enrichment of phosphopeptides and intact phosphoproteins from complex mixtures

Guanidinium functionalized superparamagnetic silica spheres for selective enrichment of phosphopeptides and intact phosphoproteins from complex mixtures

Zinc Ion-immobilized Magnetic Microspheres for Enrichment and Identification of Multi-phosphorylated Peptides by Mass Spectrometry

ZrO2 Nanofiber as a Versatile Tool for Protein Analysis

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Product

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ZrO₂ Nanofiber as a Versatile Tool for Protein Analysis