Pickering emulsions as templates for smart colloidosomes

San Miguel Delgadillo, Adriana

08 August 2011

Stimulus-responsive colloidosomes which completely dissolve upon a mild pH change are developed. pH-Responsive nanoparticles that dissolve upon a mild pH increase are synthesized by a nanoprecipitation method and are used as stabilizers for a double water-in-oil-in-water Pickering emulsion. These emulsions serve as templates for the production of pH-responsive colloidosomes. Removal of the middle oil phase produces water-core colloidosomes that have a shell made of pH-responsive nanoparticles, which rapidly dissolve above pH 7. The permeability of these capsules is assessed by FRAP, whereby the diffusion of a fluorescent tracer through the capsule shell is monitored. Three methods for tuning the permeability of the pH-responsive colloidosomes were developed: ethanol consolidation, layer-by-layer assembly and the generation of PLGA-pH-responsive nanoparticle hybrid colloidosomes. The resulting colloidosomes have different responses to the pH stimulus, as well as different pre-release permeability values. Additionally, fundamental studies regarding the role of particle surface roughness on Pickering emulsification are also shown. The pH-responsive nanoparticles were used as a coating for larger silica particles, producing rough raspberry-like particles. Partial dissolution of the nanoparticle coating allows tuning of the substrate surface roughness while retaining the same surface chemistry. The results obtained show that surface roughness increases the emulsion stability of decane-water systems (to almost twice), but only up to a certain point, where extremely rough particles produced less stable emulsions presumably due to a Cassie-Baxter wetting regime. Additionally, in an octanol-water system, surface roughness was shown to affect the type of emulsion generated. These results are of exceptional importance since they are the first controlled experimental evidence regarding the role of particle surface roughness on Pickering emulsification, thus clarifying some conflicting ideas that exist regarding this issue.

Colloidosomes

Pickering emulsions

Roughness

Stimulus-response

Triggered release

Microcapsules

Drug carriers (Pharmacy)

Nanocapsules

Nanoparticles

Microencapsulation

Characterization of enzyme sensitive responsive hydrogel/lipid system for triggered release

Jónsson, Pétur

January 2013

This master thesis aimed to create and characterize multilayer coatings upon mesoporous silica particles (MSP). The properties of the coating aimed for, was to have a triggerable controlled release, where a targeted enzyme within the intestine, alpha-amylase, is supposed to degrade the coating. The coating was created from a bilayer consisting of DOTAP and DOPC in a 1:3 molar ratio, which serves as a protective coating. The second layer interacting with the surroundings consisted of a starch component, amylopectin, which is degraded by alpha-amylase. The study of the coating was performed with ellipsometry, where the adsorption of the different layers of the coating on a planar silica surface and the enzyme-triggered degradation was recorded. The adsorbed amount of DOTAP/DOPC was 4,22 ± 0,11 mg/m2 and amylopectin 1,82 ± 0,94. The effects of different pH where performed, simulating the coated particle going through the gastro-intestinal system. Two enzymes alpha-amylase and phospholipase A2 (PLA2) where used for degradation of the coating. The knowledge from ellipsometry was applied to coating mesoporous silica particles and it was confirmed that the two layers had formed with zeta- potential measurement.

liposomes

mesoporous silica

ellipsometry

coating

Formulation de capsules à cœur aqueux pour la délivrance stimulable de protéines / Formulation of aqueous core capsules for the triggered release of proteins

Brun, Geoffrey

18 December 2015

Les gradients de concentration de peptides ou de protéines, ou leur relargage localisé, jouent un rôle primordial dans les voies de communication inter-cellulaire. L'activation locale de cellules est étudiée in vitro à l'aide de sources artificielles contraignantes ou invasives de protéines (pipettes, dispositifs microfluidiques). Des méthodes plus douces et moins invasives sont très demandées. À cet effet, nous avons développé deux types de capsules capables de libérer des macromolécules sous l'effet d'une stimulation extérieure. Le premier système emploie des liposomes additionnés d'un amphiphile à azobenzène, tensioactif ou polyélectrolyte, capable de générer des pores à travers la membrane sous l'effet de la lumière. Les temps de dissolution des assemblages lipides/tensioactifs et les cinétiques de relargage (perméabilité) sous irradiation lumineuse ont été étudiées par diffusion dynamique de la lumière et fluorescence. Le second système repose sur des capsules à cœur aqueux et à coque polymère, formées par polyaddition interfaciale. Nous avons montré que l'inclusion de chaînes thermosensibles dans la membrane (polyNIPAM, par ex.) rendait la stabilité de la capsule dépendante de la température. Nous avons démontré sur des capsules millimétriques, chargées avec du dextrane ou des protéines, que cela permettait le contrôle du relargage. L'utilisation de polymère à UCST en milieu aqueux nous a permis d'obtenir les premières capsules thermosensibles capables de libérer leur contenu par élévation de la température au dessus d'une valeur critique. Cela ouvre une voie prometteuse au développement d'un système biocompatible de libération de protéines. / Concentration gradients and local delivery of peptides or proteins play a crucial role in intercellular communication. In vitro, the effects of local activation of cells are studied with constrained or invasive artificial protein sources (pipettes, microfluidics). Milder and remotely-triggered techniques for the release of encapsulated biomolecules are highly in demand. To this aim we developed two classes of capsules able to release macromolecules upon an external stimulation. The first system is based on liposomes sensitized with azobenzene-containing amphiphiles (surfactants or polyelectrolytes) that can open pores in the membrane upon exposure to light. The dissolution time of lipids/surfactants assemblies and rate of release (permeability) under light irradiation has been assessed by dynamic light scattering and fluorescence measurements. The second system is a model of capsules with an aqueous core and a polymer shell, formed by interfacial polyaddition. We showed that inclusion of temperature-responsive chains in the membrane, e.g. polyNIPAM, confers temperature-dependant stability to the capsules; we demonstrated with millimeter-sized capsules loaded with dextran or proteins that this can be used to trigger the release. Using chains with UCST in water, we obtained the first temperature-sensitive capsules able to release their content upon increasing the temperature above a threshold. This represents a promising route to the biocompatible delivery of proteins.

Protéine

Encapsulation

Libération contrôlée

Liposomes photosensibles

Capsules thermosensibles

Polymères à UCST/LCST

Protein

Encapsulation

Triggered release

541.3

Physico-Chemical Investigations of Bilayer Discs and Related Lipid Structures Formed in Liposomal Systems Intended for Triggered Release

Sandström, Maria

January 2007

<p>This thesis describes results from fundamental studies of liposomes intended for drug delivery and pH or temperature triggered release. In addition, the effect of lipid composition on bilayer disc formation and a potential application of the bilayer discs were investigated.</p><p>The lower pH encountered by endocytosed liposomes can be utilized to trigger drug release. The mechanisms behind cytosolic drug delivery were investigated using two different kinds of pH-sensitive liposomes. The results indicate that incorporation of non-lamellar forming lipids into the endosome membrane may allow for drug escape into the cytosol.</p><p>Temperature-sensitive liposomes containing lysolipid (LTSL) release their content almost instantly when heated to temperatures close to the gel to liquid crystalline phase transition temperature (T<i>C</i>). Morphological changes of the liposomes in response to temperature cycling were studied. Temperature cycling induced liposome openings and disintegration of the liposomes into bilayer discs. Incubation of LTSL in the presence of multilamellar liposomes (MLVs) resulted in relocalisation of lysolipid into the MLVs, which affected the rapid release from LTSL. We propose that the presence of micelle-forming components, such as lysolipids and PEG-lipids, facilitates the formation of defects and membrane openings during the initial phase of membrane melting, resulting in the observed rapid release. Similar to added lysolipids, also hydrolysis generated lysolipids induce disc-formation upon heating through T<i>C</i> of the lipid mixture.</p><p>Two fundamentally different micelles may form in PEG-lipid/lipid mixtures. We found that discoidal structures are preferred over cylindrical micelles when the mixture contains components that reduce the spontaneous curvature, increase the monolayer bending modulus, or reduce PEG-lipid/lipid miscibility. The large discoidal micelles found at low PEG-lipid content are better described as bilayer discs. We evaluated such discs as model membranes in drug partitioning studies, and suggest that they, in some cases, produce more accurate data than liposomes.</p>

Physical chemistry

liposome

triggered release

pH-sensitive liposomes

temperature-sensitive liposomes

drug partitioning

cryo-TEM

discs

Fysikalisk kemi

Light-Triggered Release of DNA from Plasmon-Resonant Nanoparticles

Huschka, Ryan

05 June 2013

Plasmon-resonant nanoparticle complexes show promising potential for light-triggered, controllable delivery of deoxyribonucleic acids (DNA) for research and therapeutic purposes. For example, the approach of RNA interference (RNAi) ‒ using antisense DNA or RNA oligonucleotides to silence activity of a specific pathogenic gene transcript and reduce expression of the encoded protein ‒ is very useful in dissecting genetic function and holds promise as a molecular therapeutic. Herein, we investigate the mechanism and probe the in vitro therapeutic potential of DNA light-triggered release from plasmonic nanoparticles. First, we investigate the mechanism of light-triggered release by dehybridizing double-stranded (dsDNA) via laser illumination from two types of nanoparticle substrates: gold (Au) nanoshells and Au nanorods. Both light-triggered and thermally induced releases are distinctly observable from nanoshell-based complexes. Surprisingly, no analogous measurable light-triggered release was observable from nanorod-based complexes below the DNA melting temperature. These results suggest that a nonthermal mechanism may play a role in light-triggered DNA release. Second, we demonstrate the in vitro light-triggered release of molecules non-covalently attached within dsDNA bound to the Au nanoshell surface. DAPI (4',6-diamidino-2-phenylindole), a bright blue fluorescent molecule that binds reversibly to double-stranded DNA, was chosen to visualize this intracellular light-induced release process. Illumination through the cell membrane of the nanoshell-dsDNA-DAPI complexes dehybridizes the DNA and releases the DAPI molecules within living cells. The DAPI molecules diffuse to the nucleus and associate with the cell’s endogenous DNA. This work could have future applications towards drug delivery of molecules that associate with dsDNA. Finally, we demonstrate an engineered Au nanoshell (AuNS)-based therapeutic oligonucleotide delivery vehicle, designed to release its cargo on demand upon illumination with a near-infrared (NIR) laser. A poly(L)lysine peptide (PLL) epilayer coated onto the AuNS surface (AuNS-PLL) is used to capture intact, single-stranded antisense DNA oligonucleotide, or alternatively, double-stranded short-interfering RNA (siRNA) molecules. A green fluorescent protein (GFP)-expressing human lung cancer H1299 cell line was used to determine cellular uptake and GFP gene silencing mediated by AuNS-PLL delivery vector. The light-triggered release of oligonucleotides could have broad applications in the study of cellular processes and in the development of intracellular targeted therapies.

Nanoparticle

plasmon

gene therapy

controlled release

DNA

siRNA

nanoshell

gold nanoshell

plasmon resonance

light-triggered release

downregulation

Physico-Chemical Investigations of Bilayer Discs and Related Lipid Structures Formed in Liposomal Systems Intended for Triggered Release

Sandström, Maria

January 2007

This thesis describes results from fundamental studies of liposomes intended for drug delivery and pH or temperature triggered release. In addition, the effect of lipid composition on bilayer disc formation and a potential application of the bilayer discs were investigated. The lower pH encountered by endocytosed liposomes can be utilized to trigger drug release. The mechanisms behind cytosolic drug delivery were investigated using two different kinds of pH-sensitive liposomes. The results indicate that incorporation of non-lamellar forming lipids into the endosome membrane may allow for drug escape into the cytosol. Temperature-sensitive liposomes containing lysolipid (LTSL) release their content almost instantly when heated to temperatures close to the gel to liquid crystalline phase transition temperature (TC). Morphological changes of the liposomes in response to temperature cycling were studied. Temperature cycling induced liposome openings and disintegration of the liposomes into bilayer discs. Incubation of LTSL in the presence of multilamellar liposomes (MLVs) resulted in relocalisation of lysolipid into the MLVs, which affected the rapid release from LTSL. We propose that the presence of micelle-forming components, such as lysolipids and PEG-lipids, facilitates the formation of defects and membrane openings during the initial phase of membrane melting, resulting in the observed rapid release. Similar to added lysolipids, also hydrolysis generated lysolipids induce disc-formation upon heating through TC of the lipid mixture. Two fundamentally different micelles may form in PEG-lipid/lipid mixtures. We found that discoidal structures are preferred over cylindrical micelles when the mixture contains components that reduce the spontaneous curvature, increase the monolayer bending modulus, or reduce PEG-lipid/lipid miscibility. The large discoidal micelles found at low PEG-lipid content are better described as bilayer discs. We evaluated such discs as model membranes in drug partitioning studies, and suggest that they, in some cases, produce more accurate data than liposomes.

Physical chemistry

liposome

triggered release

pH-sensitive liposomes

temperature-sensitive liposomes

drug partitioning

cryo-TEM

discs

Fysikalisk kemi

Clot-Targeted Enzyme-Responsive Nanoparticles for Thrombolytic Therapy

Sun, Michael

26 August 2022

No description available.

Biomedical Engineering

targeted thrombolysis

fibrinolysis

plasmin

thrombin

nanomedicine

lipid vesicle

drug delivery

enzyme-triggered release

platelets

fibrin

Liposomes for Drug Delivery : from Physico-chemical Studies to Applications

Bergstrand, Nill

January 2003

<p>Physico-chemical characterisation of structure and stability of liposomes intended for drug delivery is the central issue in this thesis. In addition, targeted liposomes to be used in boron neutron capture therapy (BNCT) were developed.</p><p>Lysolipids and fatty acids are products formed upon hydrolysis of PC-lipids. The aggregate structure formed upon mixing lysolipids, fatty acids and EPC were characterised by means of cryo-TEM. A relatively monodisperse population of unilamellar liposomes was detected in mixtures containing equimolar concentration of the three components. </p><p>The interactions between alternative steric stabilisers (PEO-PPO-PEO copolymers) and conventional PC-and pH-sensitive PE-liposomes were investigated. Whereas the PE-liposomes could be stabilised by the PEO-PPO-PEO copolymers, the PC-liposomes showed an enhanced permeability concomitant with the PEO-PPO-PEO adsorption.</p><p>Permeability effects induced by different PEG-stabilisers on EPC liposomes were shown to be dependent on the length of the PEG chain but also on the linkage used to connect the PEG polymer with the hydrophobic membrane anchor.</p><p>An efficient drug delivery requires, in most cases, an accumulation of the drug in the cell cytoplasm. The mechanism behind cytosolic drug delivery from pH-sensitive liposomes was investigated. The results suggest that a destabilisation of the endosome membrane, due to an incorporation of non-lamellar forming lipids, may allow the drug to be released. </p><p>Furthermore, sterically stabilised liposomes intended for targeted BNCT have been characterised and optimised concerning loading and retention of boronated drugs. </p>

Physical chemistry

liposome

steric stabilisation

BNCT

cryo-TEM

EGF

targeting

stability

permeability

pH-sensitive liposomes

triggered release

Fysikalisk kemi

Physical chemistry

Fysikalisk kemi

Liposomes for Drug Delivery : from Physico-chemical Studies to Applications

Bergstrand, Nill

January 2003

Physico-chemical characterisation of structure and stability of liposomes intended for drug delivery is the central issue in this thesis. In addition, targeted liposomes to be used in boron neutron capture therapy (BNCT) were developed. Lysolipids and fatty acids are products formed upon hydrolysis of PC-lipids. The aggregate structure formed upon mixing lysolipids, fatty acids and EPC were characterised by means of cryo-TEM. A relatively monodisperse population of unilamellar liposomes was detected in mixtures containing equimolar concentration of the three components. The interactions between alternative steric stabilisers (PEO-PPO-PEO copolymers) and conventional PC-and pH-sensitive PE-liposomes were investigated. Whereas the PE-liposomes could be stabilised by the PEO-PPO-PEO copolymers, the PC-liposomes showed an enhanced permeability concomitant with the PEO-PPO-PEO adsorption. Permeability effects induced by different PEG-stabilisers on EPC liposomes were shown to be dependent on the length of the PEG chain but also on the linkage used to connect the PEG polymer with the hydrophobic membrane anchor. An efficient drug delivery requires, in most cases, an accumulation of the drug in the cell cytoplasm. The mechanism behind cytosolic drug delivery from pH-sensitive liposomes was investigated. The results suggest that a destabilisation of the endosome membrane, due to an incorporation of non-lamellar forming lipids, may allow the drug to be released. Furthermore, sterically stabilised liposomes intended for targeted BNCT have been characterised and optimised concerning loading and retention of boronated drugs.

Physical chemistry

liposome

steric stabilisation

BNCT

cryo-TEM

EGF

targeting

stability

permeability

pH-sensitive liposomes

triggered release

Fysikalisk kemi

Physical chemistry

Fysikalisk kemi