AI Article Synopsis

  • Magnetic nanoparticles (NiFeO) were synthesized and coated with (3-Aminopropyl) triethoxysilane through a sol-gel method, and then functionalized with EDTA-dianhydride to enhance their ability to selectively bind to His-tagged proteins.
  • Multiple characterization techniques (TEM, XRD, SEM, etc.) were used to study their physical and chemical properties, confirming their effectiveness for protein purification.
  • Safety assessments revealed low nickel leakage during the purification of His-tagged green fluorescence protein, with in vitro tests showing no cytotoxic effects related to the nanoparticles or the purified proteins compared to commercial samples.

Article Abstract

Magnetic nanoparticles NiFeO was synthesized and covered in the silicate lattice of (3-Aminopropyl) triethoxysilane (APS) by the sol-gel process. Subsequently, the EDTA-dianhydride was attached to the amino surface of magnetic nanoparticles (MNPs) during the nucleophilic attack. This polycarboxylic layer trapped the high level of nickel ions for selective bonding to the His-tagged recombinant protein. The surface of MNPs was investigated by TEM, XRD, SEM (EDSA), VSM, BET, FT-IR and zeta potential analysis which characterized the size, chemical lattice, morphology, magnetic strength, specific surface area, functional groups and charge of the surface of nanoparticles. The performance and validity of the nanoparticles were studied by the purification of His-tagged green fluorescence protein (His-GFP). Also, the safety of proposed Ni-MNPs in the purification procedure of His-tagged proteins for pharmaceutical applications was proved by the determination of the nickel leakage level in the purified final protein using atomic absorption spectroscopy. In vitro cytotoxicity of Ni-MNPs and trace metal ions was investigated by the MTS assay technique. In addition, the comparison of biological activity in purified protein (GM-CSF) and commercial sample did not show any toxic effect.

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Source
http://dx.doi.org/10.1016/j.pep.2017.10.015DOI Listing

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