Probing kinase activities by electrochemistry, contact-angle measurements, and molecular-force interactions

Ofer I. Wilner; Claudio Guidotti; Agnieszka Wieckowska; Ron Gill; Itamar Willner

doi:10.1002/chem.200800765

Probing kinase activities by electrochemistry, contact-angle measurements, and molecular-force interactions

Ofer I. Wilner, Claudio Guidotti, Agnieszka Wieckowska, Ron Gill, Itamar Willner

Research output: Contribution to journal › Article › peer-review

49 Scopus citations

Abstract

Three different methods to investigate the activity of a protein kinase (casein kinase, CK2) are described. The phosphorylation of the sequence-specific peptide (1) by CK2 was monitored by electrochemical impedance spectroscopy (EIS). Phosphorylation of the peptide monolayer assembled on a Au electrode yields a negatively charged surface that electrostatically repels the negatively charged redox label [Fe(CN)₆]^3-/4-, thus increasing the interfacial electron-transfer resistance. The phosphorylation process by CK2 is further amplified by the association of the anti-phosphorylated peptide antibody to the monolayer. Binding of the antibody insulates the electrode surface, thus increasing the interfacial electron-transfer resistancein the presence of the redox label. This method enabled the quantitative analysis of the concentration of CK2 with a detection limit of ten units. The second method employed involved contact-angle measurements. Although the peptide 1-functionalized electrode revealed a contact angle of 67.5°, phosphorylation of the peptide yielded a surface with enhanced hydrophilicity, 36.8°. The biocatalyzed cleavage of the phosphate units with alkaline phosphatase regenerates the hydrophobic peptide monolayer, contact angle 55.3°. The third method to characterize the system involved chemical force measurements between the phosphorylated peptide monolayer associated with the Au surface and a Au tip functionalized with the anti-phosphorylated peptide antibody. Although no significant rupture forces existed between the modified tip and the 1-functionalized surface (6±2pN), significant rupture forces (multiples of 120±20 pN) were observed between the phosphorylated monolayer-modified surface and the antibody-functionalized tip. This rupture force is attributed to the dissociation of a simple binding event between the phosphorylated peptide and the fluorescent antibody (Fab) binding region. ω 2008 Wiley-VCH Verlag GmbH& Co. KGaA.

Original language	English
Pages (from-to)	7774-7781
Number of pages	8
Journal	Chemistry - A European Journal
Volume	14
Issue number	26
DOIs	https://doi.org/10.1002/chem.200800765
State	Published - 8 Sep 2008
Externally published	Yes

Keywords

Antibodies
Biosensors
Contact angles
Electrochemistry
Protein kinases

ASJC Scopus subject areas

Catalysis
Organic Chemistry

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10.1002/chem.200800765

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title = "Probing kinase activities by electrochemistry, contact-angle measurements, and molecular-force interactions",

abstract = "Three different methods to investigate the activity of a protein kinase (casein kinase, CK2) are described. The phosphorylation of the sequence-specific peptide (1) by CK2 was monitored by electrochemical impedance spectroscopy (EIS). Phosphorylation of the peptide monolayer assembled on a Au electrode yields a negatively charged surface that electrostatically repels the negatively charged redox label [Fe(CN)6]3-/4-, thus increasing the interfacial electron-transfer resistance. The phosphorylation process by CK2 is further amplified by the association of the anti-phosphorylated peptide antibody to the monolayer. Binding of the antibody insulates the electrode surface, thus increasing the interfacial electron-transfer resistancein the presence of the redox label. This method enabled the quantitative analysis of the concentration of CK2 with a detection limit of ten units. The second method employed involved contact-angle measurements. Although the peptide 1-functionalized electrode revealed a contact angle of 67.5°, phosphorylation of the peptide yielded a surface with enhanced hydrophilicity, 36.8°. The biocatalyzed cleavage of the phosphate units with alkaline phosphatase regenerates the hydrophobic peptide monolayer, contact angle 55.3°. The third method to characterize the system involved chemical force measurements between the phosphorylated peptide monolayer associated with the Au surface and a Au tip functionalized with the anti-phosphorylated peptide antibody. Although no significant rupture forces existed between the modified tip and the 1-functionalized surface (6±2pN), significant rupture forces (multiples of 120±20 pN) were observed between the phosphorylated monolayer-modified surface and the antibody-functionalized tip. This rupture force is attributed to the dissociation of a simple binding event between the phosphorylated peptide and the fluorescent antibody (Fab) binding region. ω 2008 Wiley-VCH Verlag GmbH& Co. KGaA.",

keywords = "Antibodies, Biosensors, Contact angles, Electrochemistry, Protein kinases",

author = "Wilner, {Ofer I.} and Claudio Guidotti and Agnieszka Wieckowska and Ron Gill and Itamar Willner",

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T1 - Probing kinase activities by electrochemistry, contact-angle measurements, and molecular-force interactions

AU - Wilner, Ofer I.

AU - Guidotti, Claudio

AU - Wieckowska, Agnieszka

AU - Gill, Ron

AU - Willner, Itamar

PY - 2008/9/8

Y1 - 2008/9/8

N2 - Three different methods to investigate the activity of a protein kinase (casein kinase, CK2) are described. The phosphorylation of the sequence-specific peptide (1) by CK2 was monitored by electrochemical impedance spectroscopy (EIS). Phosphorylation of the peptide monolayer assembled on a Au electrode yields a negatively charged surface that electrostatically repels the negatively charged redox label [Fe(CN)6]3-/4-, thus increasing the interfacial electron-transfer resistance. The phosphorylation process by CK2 is further amplified by the association of the anti-phosphorylated peptide antibody to the monolayer. Binding of the antibody insulates the electrode surface, thus increasing the interfacial electron-transfer resistancein the presence of the redox label. This method enabled the quantitative analysis of the concentration of CK2 with a detection limit of ten units. The second method employed involved contact-angle measurements. Although the peptide 1-functionalized electrode revealed a contact angle of 67.5°, phosphorylation of the peptide yielded a surface with enhanced hydrophilicity, 36.8°. The biocatalyzed cleavage of the phosphate units with alkaline phosphatase regenerates the hydrophobic peptide monolayer, contact angle 55.3°. The third method to characterize the system involved chemical force measurements between the phosphorylated peptide monolayer associated with the Au surface and a Au tip functionalized with the anti-phosphorylated peptide antibody. Although no significant rupture forces existed between the modified tip and the 1-functionalized surface (6±2pN), significant rupture forces (multiples of 120±20 pN) were observed between the phosphorylated monolayer-modified surface and the antibody-functionalized tip. This rupture force is attributed to the dissociation of a simple binding event between the phosphorylated peptide and the fluorescent antibody (Fab) binding region. ω 2008 Wiley-VCH Verlag GmbH& Co. KGaA.

AB - Three different methods to investigate the activity of a protein kinase (casein kinase, CK2) are described. The phosphorylation of the sequence-specific peptide (1) by CK2 was monitored by electrochemical impedance spectroscopy (EIS). Phosphorylation of the peptide monolayer assembled on a Au electrode yields a negatively charged surface that electrostatically repels the negatively charged redox label [Fe(CN)6]3-/4-, thus increasing the interfacial electron-transfer resistance. The phosphorylation process by CK2 is further amplified by the association of the anti-phosphorylated peptide antibody to the monolayer. Binding of the antibody insulates the electrode surface, thus increasing the interfacial electron-transfer resistancein the presence of the redox label. This method enabled the quantitative analysis of the concentration of CK2 with a detection limit of ten units. The second method employed involved contact-angle measurements. Although the peptide 1-functionalized electrode revealed a contact angle of 67.5°, phosphorylation of the peptide yielded a surface with enhanced hydrophilicity, 36.8°. The biocatalyzed cleavage of the phosphate units with alkaline phosphatase regenerates the hydrophobic peptide monolayer, contact angle 55.3°. The third method to characterize the system involved chemical force measurements between the phosphorylated peptide monolayer associated with the Au surface and a Au tip functionalized with the anti-phosphorylated peptide antibody. Although no significant rupture forces existed between the modified tip and the 1-functionalized surface (6±2pN), significant rupture forces (multiples of 120±20 pN) were observed between the phosphorylated monolayer-modified surface and the antibody-functionalized tip. This rupture force is attributed to the dissociation of a simple binding event between the phosphorylated peptide and the fluorescent antibody (Fab) binding region. ω 2008 Wiley-VCH Verlag GmbH& Co. KGaA.

KW - Antibodies

KW - Biosensors

KW - Contact angles

KW - Electrochemistry

KW - Protein kinases

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DO - 10.1002/chem.200800765

M3 - Article

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AN - SCOPUS:53849147610

SN - 0947-6539

VL - 14

SP - 7774

EP - 7781

JO - Chemistry - A European Journal

JF - Chemistry - A European Journal

IS - 26

ER -

Probing kinase activities by electrochemistry, contact-angle measurements, and molecular-force interactions

Abstract

Keywords

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