The approach enables the testing of cellular responses to individual signaling molecules as well as their spatial ordering.
For the testing of cellular cytotoxicity of empty nanoparticles, they were diluted with serum-free RPMI1640 media and sterilized with a 0.8-μm syringe filter and added to 2 × 104 Hcells cells.
Details for randomization tests of cellular networks have been described previously [ 31].
As such, it can represent a useful model for preclinical testing of cellular populations and stem cell-derived cardiomyocytes for tissue engineering.
Furthermore, testing of cellular antioxidant protection using the CAP-e assay showed that NAE-8® contains more antioxidants that are bioavailable at the cellular level, compared to AQ-NOE.
This approach is very powerful, since it enables the testing of cellular responses to individual cRGD nanopatches and their spatial ordering which is very important for comparing the impact of different ligands for integrin activation as reported here.
Though tests of cellular or humoral stimulation index, are not as yet capable of differentiating the transient from the non-transient patients upon their presentation, significant isotype and mitogen specific variability is evident.
However, closely related SUT/SUC proteins in different species can localize to different membranes [ 57] and, indeed, they may change their location in order to drive particular cellular processes; direct testing of cellular location would therefore be required for the cotton fibre homologs.
