15 research outputs found
Acoustic enhancement of intracellular delivery for ex vivo therapeutics
Recent advances in gene editing and therapy have highlighted the potential of ex vivo cell-based techniques to treat many diseases, wherein a patientâs cells are harvested, engineered to insert various therapeutic agents such as nucleic acids or proteins, and re-infused. Considerable challenges however remain in the ability not just to insert these agents into cells whilst retaining high levels of cellular viability, but also to ensure that they are not lysed within the cell.
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Nebulization of siRNA for inhalation therapy based on a microfluidic surface acoustic wave platform.
The local delivery of therapeutic small interfering RNA or siRNA to the lungs has the potential to improve the prognosis for patients suffering debilitating lung diseases. Recent advances in materials science have been aimed at addressing delivery challenges including biodistribution, bioavailability and cell internalization, but an equally important challenge to overcome is the development of an inhalation device that can deliver the siRNA effectively to the lung, without degrading the therapeutic itself. Here, we report the nebulization of siRNA, either naked siRNA or complexed with polyethyleneimine (PEI) or a commercial transfection agent, using a miniaturizable acoustomicrofluidic nebulization device. The siRNA solution could be nebulised without significant degradation into an aerosol mist with tunable mean aerodynamic diameters of approximately 3 ”m, which is appropriate for deep lung deposition via inhalation. The nebulized siRNA was tested for its stability, as well as its toxicity and gene silencing properties using the mammalian lung carcinoma cell line A549, which demonstrated that the gene silencing capability of siRNA is retained after nebulization. This highlights the potential application of the acoustomicrofluidic device for the delivery of efficacious siRNA via inhalation, either for systemic delivery via the alveolar epithelium or local therapeutic delivery to the lung
mRNA Treatment Rescues NiemannâPick Disease Type C1 in Patient Fibroblasts
Messenger RNA (mRNA) holds great potential as a disease-modifying
treatment for a wide array of monogenic disorders. NiemannâPick
disease type C1 (NP-C1) is an ultrarare monogenic disease that arises
due to loss-of-function mutations in the NPC1 gene,
resulting in the entrapment of unesterified cholesterol in the lysosomes
of affected cells and a subsequent reduction in their capacity for
cholesterol esterification. This causes severe damage to various organs
including the brain, liver, and spleen. In this work, we describe
the use of NPC1-encoded mRNA to rescue the protein insufficiency and
pathogenic phenotype caused by biallelic NPC1 mutations
in cultured fibroblasts derived from an NP-C1 patient. We first evaluated
engineering strategies for the generation of potent mRNAs capable
of eliciting high protein expression across multiple cell types. We
observed that âGC3â codon optimization, coupled with
N1-methylpseudouridine base modification, yielded an mRNA that was
approximately 1000-fold more potent than wild-type, unmodified mRNA
in a luciferase reporter assay and consistently superior to other
mRNA variants. Our data suggest that the improved expression associated
with this design strategy was due in large part to the increased secondary
structure of the designed mRNAs. Both codon optimization and base
modification appear to contribute to increased secondary structure.
Applying these principles to the engineering of NPC1-encoded mRNA,
we observed a normalization in NPC1 protein levels after mRNA treatment,
as well as a rescue of the mutant phenotype. Specifically, mRNA treatment
restored the cholesterol esterification capacity of patient cells
to wild-type levels and induced a significant reduction in both unesterified
cholesterol levels (>57% reduction compared to Lipofectamine-treated
control in a cholesterol esterification assay) and lysosome size (157
ÎŒm2 reduction compared to Lipofectamine-treated control).
These findings show that engineered mRNA can correct the deficit caused
by NPC1 mutations. More broadly, they also serve
to further validate the potential of this technology to correct diseases
associated with loss-of-function mutations in genes coding for large,
complex, intracellular proteins
Distribution of Particles in Human Stem Cell-Derived 3D Neuronal Cell Models: Effect of Particle Size, Charge, and Density
Neurodegenerative diseases are generally characterized by a progressive loss of neuronal subpopulations, with no available cure to date. One of the main reasons for the limited clinical outcomes of new drug formulations is the lack of appropriate in vitro human cell models for research and validation. Stem cell technologies provide an opportunity to address this challenge by using patient-derived cells as a platform to test various drug formulations, including particle-based drug carriers. The therapeutic efficacy of drug delivery systems relies on efficient cellular uptake of the carrier and can be dependent on its size, shape, and surface chemistry. Although considerable efforts have been made to understand the effects of the physiochemical properties of particles on two-dimensional cell culture models, little is known of their effect in three-dimensional (3D) cell models of neurodegenerative diseases. Herein, we investigated the role of particle size (235-1000 nm), charge (cationic and anionic), and density (1.05 and 1.8 g cm-3) on the interactions of particles with human embryonic stem cell-derived 3D cell cultures of sensory neurons, called sensory neurospheres (sNSP). Templated layer-by-layer particles, with silica or polystyrene cores, and self-assembled glycogen/DNA polyplexes were used. Particles with sizes Additionally, effective plasmid DNA delivery was observed up to 6 days post-transfection with glycogen/DNA polyplexes. The findings provide guidance in nanoparticle design for therapies aimed at neurodegenerative diseases, in particular Friedreich\u27s ataxia, whereby sensory neurons are predominantly affected. They also demonstrate the application of 3D models of human sensory neurons in preclinical drug development
Distribution of Particles in Human Stem Cell-Derived 3D Neuronal Cell Models: Effect of Particle Size, Charge, and Density
Neurodegenerative diseases are generally characterized by a progressive loss of neuronal subpopulations, with no available cure to date. One of the main reasons for the limited clinical outcomes of new drug formulations is the lack of appropriate in vitro human cell models for research and validation. Stem cell technologies provide an opportunity to address this challenge by using patient-derived cells as a platform to test various drug formulations, including particle-based drug carriers. The therapeutic efficacy of drug delivery systems relies on efficient cellular uptake of the carrier and can be dependent on its size, shape, and surface chemistry. Although considerable efforts have been made to understand the effects of the physiochemical properties of particles on two-dimensional cell culture models, little is known of their effect in three-dimensional (3D) cell models of neurodegenerative diseases. Herein, we investigated the role of particle size (235-1000 nm), charge (cationic and anionic), and density (1.05 and 1.8 g cm-3) on the interactions of particles with human embryonic stem cell-derived 3D cell cultures of sensory neurons, called sensory neurospheres (sNSP). Templated layer-by-layer particles, with silica or polystyrene cores, and self-assembled glycogen/DNA polyplexes were used. Particles with sizes <280 nm effectively penetrated sNSP. Additionally, effective plasmid DNA delivery was observed up to 6 days post-transfection with glycogen/DNA polyplexes. The findings provide guidance in nanoparticle design for therapies aimed at neurodegenerative diseases, in particular Friedreich's ataxia, whereby sensory neurons are predominantly affected. They also demonstrate the application of 3D models of human sensory neurons in preclinical drug development
Supramolecular polyphenolâDNA microparticles for in vivo adjuvant and antigen coâdelivery and immune stimulation
DNA-based materials have attracted interest due to the tunable structure and encoded biological functionality of nucleic acids. A simple and general approach to synthesize DNA-based materials with fine control over morphology and bioactivity is important to expand their applications. Here, we report the synthesis of DNA-based particles via the supramolecular assembly of tannic acid (TA) and DNA. Uniform particles with different morphologies are obtained using a variety of DNA building blocks. The particles enable the co-delivery of cytosine-guanine adjuvant sequences and the antigen ovalbumin in model cells. Intramuscular injection of the particles in mice induces antigen-specific antibody production and T cell responses with no apparent toxicity. Protein expression in cells is shown using capsules assembled from TA and plasmid DNA. This work highlights the potential of TA as a universal material for directing the supramolecular assembly of DNA into gene and vaccine delivery platforms