A Simple and Versatile Strategy for Oriented Immobilization of His-Tagged Proteins on Magnetic Nanoparticles

A Simple and Versatile Strategy for Oriented Immobilization of His-Tagged Proteins on Magnetic Nanoparticles

Oriented and covalent immobilization of proteins on magnetic nanoparticles (MNPs) is particularly challenging as it requires both the functionality of the protein and the colloidal stability of the MNPs to be preserved. Here, we describe a simple, straightforward, and efficient strategy for MNP func...

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Bibliographic Details
Published in:Bioconjugate chemistry Vol. 34; no. 12; pp. 2275 - 2292
Main Authors: Castro-Hinojosa, Christian, Del Sol-Fernández, Susel, Moreno-Antolín, Eduardo, Martín-Gracia, Beatriz, Ovejero, Jesús G., de la Fuente, Jesús Martínez, Grazú, Valeria, Fratila, Raluca M., Moros, María
Format: Journal Article
Language:English
Published: United States American Chemical Society 20-12-2023
Subjects:
Cadherins
Cadherins - chemistry
Chelating Agents
Density
E-cadherin
Fragments
Immobilization
Indicators and Reagents
Magnetite Nanoparticles - chemistry
Metal ions
Metals
Nanoparticles
Nitrilotriacetic acid
Nitrilotriacetic Acid - chemistry
Polyethylene glycol
Polyhistidine
Proteins
Stability
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Summary:Oriented and covalent immobilization of proteins on magnetic nanoparticles (MNPs) is particularly challenging as it requires both the functionality of the protein and the colloidal stability of the MNPs to be preserved. Here, we describe a simple, straightforward, and efficient strategy for MNP functionalization with proteins using metal affinity binding. Our method involves a single-step process where MNPs are functionalized using a preformed, ready-to-use nitrilotriacetic acid-divalent metal cation (NTA-M2+) complex and polyethylene glycol (PEG) molecules. As a proof-of-concept, we demonstrate the oriented immobilization of a recombinant cadherin fragment engineered with a hexahistidine tag (6His-tag) onto the MNPs. Our developed methodology is simple and direct, enabling the oriented bioconjugation of His-tagged cadherins to MNPs while preserving protein functionality and the colloidal stability of the MNPs, and could be extended to other proteins expressing a polyhistidine tag. When compared to the traditional method where NTA is first conjugated to the MNPs and afterward free metal ions are added to form the complex, this novel strategy results in a higher functionalization efficiency while avoiding MNP aggregation. Additionally, our method allows for covalent bonding of the cadherin fragments to the MNP surface while preserving functionality, making it highly versatile. Finally, our strategy not only ensures the correct orientation of the protein fragments on the MNPs but also allows for the precise control of their density. This feature enables the selective targeting of E-cadherin-expressing cells only when MNPs are decorated with a high density of cadherin fragments.
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ISSN:1043-1802
1520-4812
DOI:10.1021/acs.bioconjchem.3c00417