Protocells (Nanoporous Particle Supported Lipid Bilayers) For Targeted Drug Delivery

To overcome the challenges of exisiting targeted nanocarriers, our team has recently devised a solution to this complex engineering problem through the creation of a composite nanocarrier termed a “protocell”. Targeted protocells, first reported in a 2011 article in Nature Materials and more recently in ACS Nano, are formed by fusion of liposomes on high surface area (> 1000 m²/g) porous silica nanoparticle cores (50-200 nm in diameter) followed by conjugation of the supported lipid bilayer with targeting and trafficking ligands and PEG. They synergistically combine the advantages of liposomes (low inherent toxicity, immunogenicity, and long circulation times) and porous nanoparticles (stability and an enormous capacity for multiple cargos and disparate cargo combinations). We have demonstrated that protocell-supported lipid bilayer membranes retain both high in-plane, two-dimensionalmobility and high stability against destabilization on exposure to blood components and leakage of drug cargos from the silica core. This desirable combination of fluidity and stability arises from the adhesion energy between the lipid headgroups and surface silanols (≡ Si-OH), which suppresses large scale membrane bilayer fluctuations responsible for leakage, along with surface nanopores that modulate lipid headgroup packing and enhance lateral fluidity. These factors allow protocells, incorporating very low densities of targeting peptide ligands or single chain antibodies as targeting moieties, to bind selectively to target cells via multivalent binding enabled by targeting ligand diffusivity and recruitment by cell surface receptors. This allows high affinity, cell-specific binding while minimizing off-target binding and immunogenicity. We have demonstrated that protocells have a 100-fold greater specificity in target-cell binding than equivalent fluid-phase liposomes. The design of the protocell has also overcome a second disadvantage of liposomal and most other nanocarrier drug delivery strategies, namely the inability to deliver high levels of multiple drug cargos, particularly where the drug combinations have different charges, polarities, and molecular weights. In contrast, protocells can simultaneously adsorb multiple diverse cargos (imaging agents, peptides, siRNAs, and drugs with different physicochemical properties) into their nanoporous silica cores, with reversible binding to silica providing the means to stably retain high levels of each cargo before envelopment of the particle into its protective lipid membrane shell. Adsorption-mediated drug loading into the silica cores leads to a 1,000-fold greater dose of doxorubicin on a per protocell particle basis, compared to FDA-approved liposomal doxorubicin. A third major advantage of the protocell is that combinatorial cargos are retained until they are efficiently delivered into intracellular compartments of the cytosol of the target cell “on cue” via pH-triggered destabilization of the protocell’s supported lipid bilayer and endosomic swelling and disruption orchestrated by endosomolytic peptides incorporated within the lipid bilayer. Until now, “endosomal escape” has been a major obstacle of other targeted nanocarrier strategies. Inclusion of an octa-arginine peptide, which stimulates macropinocytosis, enables both selective targeting and intracellular delivery for cells where cell-specific receptors are not readily endocytosed. Using a model of hepatocellular carcinoma, we demonstrated that protocells carrying a cocktail of doxorubicin, 5-FU, and cisplatin were so potent that a single targeted protocell could kill a multidrug-resistant hepatocellular carcinoma cell in vitro, representing a 10⁶-fold improvement over liposomes.