4.6 Article

A Simple Method for Synthesis of Chitosan Nanoparticles with Ionic Gelation and Homogenization

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MOLECULES
卷 28, 期 11, 页码 -

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MDPI
DOI: 10.3390/molecules28114328

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nanoparticle synthesis; chitosan; biopolymers; ionic gelation

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Chitosan nanoparticles (CNPs) with a size range of 68-77 nm were successfully synthesized through a simple and efficient method, using low molecular weight chitosan and tripolyphosphate as crosslinker. The CNPs showed monodispersity and high yield. Different purification methods and solution conditions were investigated and found to affect the size and polydispersity of CNP formation. The smaller CNPs synthesized using homogenization and filtration exhibited good interaction with negatively charged proteins and DNA, making them suitable for the development of virus surrogates for water applications.
Chitosan nanoparticles (CNPs) are known to have great utility in many fields (pharmaceutical, agricultural, food industry, wastewater treatment, etc.). In this study we aimed to synthesize sub-100 nm CNPs as a precursor of new biopolymer-based virus surrogates for water applications. We present a simple yet efficient synthesis procedure for obtaining high yield, monodisperse CNPs with size 68-77 nm. The CNPs were synthesized by ionic gelation using low molecular weight chitosan (deacetylation 75-85%) and tripolyphosphate as crosslinker, under rigorous homogenization to decrease size and increase uniformity, and purified by passing through 0.1 mu m polyethersulfone syringe filters. The CNPs were characterized using dynamic light scattering, tunable resistive pulse sensing, and scanning electron microscopy. We demonstrate reproducibility of this method at two separate facilities. The effects of pH, ionic strength and three different purification methods on the size and polydispersity of CNP formation were examined. Larger CNPs (95-219) were produced under ionic strength and pH controls, and when purified using ultracentrifugation or size exclusion chromatography. Smaller CNPs (68-77 nm) were formulated using homogenization and filtration, and could readily interact with negatively charge proteins and DNA, making them an ideal precursor for the development of DNA-labelled, protein-coated virus surrogates for environmental water applications.

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