Printing Therapeutic Proteins in 3D using Nanoengineered Bioink to Control and Direct Cell Migration.

Adv Healthc Mater

Biomedical Engineering, Dwight Look College of Engineering, Texas A&M University, College Station, TX, 77843, USA.

Published: June 2019

AI Article Synopsis

  • A bioink created from a degradable polymer and 2D nanoparticles is designed to influence cell function in 3D printed constructs.
  • The bioink, which is made through a specific polymerization process, exhibits properties like shear-thinning and good printability due to the addition of nanosilicates.
  • This innovative approach allows for controlled delivery of therapeutic proteins, enhancing cell migration and offering potential applications in regenerative medicine to create complex tissue structures.

Article Abstract

A nanoengineered bioink loaded with therapeutic proteins is designed to direct cell function in a 3D printed construct. The bioink is developed from a hydrolytically degradable polymer and 2D synthetic nanoparticle. The synthesis of poly(ethylene glycol)-dithiothreitol (PEGDTT) via a Michael-like step growth polymerization results in acrylate terminated degradable macromer. The addition of 2D nanosilicates to PEGDTT results in formation of shear-thinning bioinks with high printability and structural fidelity. The mechanical properties, swelling kinetics, and degradation rate of 3D printed constructs can be modulated by changing the ratio of PEG:PEGDTT and nanosilicates concentration. Due to high surface area and charged characteristic of nanosilicates, protein therapeutics can be sequestered in 3D printing structure for prolong duration. Sustained release of pro-angiogenic therapeutics from 3D printed structure, promoted rapid migration of human endothelial umbilical vein cell. This approach to design biologically active inks to control and direct cell behavior can be used to engineer 3D complex tissue structure for regenerative medicine.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC6554037PMC
http://dx.doi.org/10.1002/adhm.201801553DOI Listing

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