Changing stroke rehab and research worldwide now.Time is Brain! trillions and trillions of neurons that DIE each day because there are NO effective hyperacute therapies besides tPA(only 12% effective). I have 523 posts on hyperacute therapy, enough for researchers to spend decades proving them out. These are my personal ideas and blog on stroke rehabilitation and stroke research. Do not attempt any of these without checking with your medical provider. Unless you join me in agitating, when you need these therapies they won't be there.

What this blog is for:

My blog is not to help survivors recover, it is to have the 10 million yearly stroke survivors light fires underneath their doctors, stroke hospitals and stroke researchers to get stroke solved. 100% recovery. The stroke medical world is completely failing at that goal, they don't even have it as a goal. Shortly after getting out of the hospital and getting NO information on the process or protocols of stroke rehabilitation and recovery I started searching on the internet and found that no other survivor received useful information. This is an attempt to cover all stroke rehabilitation information that should be readily available to survivors so they can talk with informed knowledge to their medical staff. It lays out what needs to be done to get stroke survivors closer to 100% recovery. It's quite disgusting that this information is not available from every stroke association and doctors group.

Saturday, December 18, 2021

Humanized Biomimetic Nanovesicles for Neuron Targeting

 I'm hoping there are two working neurons in all of stroke we can rub together to figure out how to use this for stroke recovery.

Humanized Biomimetic Nanovesicles for Neuron Targeting

First published: 11 August 2021

Zinger and Cvetkovic contributed equally to this work.

Abstract

Nanovesicles (NVs) are emerging as innovative, theranostic tools for cargo delivery. Recently, surface engineering of NVs with membrane proteins from specific cell types has been shown to improve the biocompatibility of NVs and enable the integration of functional attributes. However, this type of biomimetic approach has not yet been explored using human neural cells for applications within the nervous system. Here, this paper optimizes and validates the scalable and reproducible production of two types of neuron-targeting NVs, each with a distinct lipid formulation backbone suited to potential therapeutic cargo, by integrating membrane proteins that are unbiasedly sourced from human pluripotent stem-cell-derived neurons. The results establish that both endogenous and genetically engineered cell-derived proteins effectively transfer to NVs without disruption of their physicochemical properties. NVs with neuron-derived membrane proteins exhibit enhanced neuronal association and uptake compared to bare NVs. Viability of 3D neural sphere cultures is not disrupted by treatment, which verifies the utility of organoid-based approaches as NV testing platforms. Finally, these results confirm cellular association and uptake of the biomimetic humanized NVs to neurons within rodent cranial nerves. In summary, the customizable NVs reported here enable next-generation functionalized theranostics aimed to promote neuroregeneration.

1 Introduction

Restoration of neural function after traumatic injury, neurodegeneration, or neuroinflammation is currently hindered by a lack of effective and clinically practicable biotechnologies for precise, cell-targeted therapies or diagnostics. As such, there remains a need for biotechnological breakthroughs that can enhance and sustain the delivery of therapeutic cargos (e.g., genetic material and chemical compounds using nanomaterials),[1] while also mimicking the microenvironment of the brain to avoid foreign body response.[2] One promising pathway is the utilization of nanotechnologies inspired by nature, more commonly referred to as bio-inspired or biomimetic tools. By mimicking the composition and biological functions of the cells in our body, biomimetic tools avoid potential side effects that occur from systemic administration of potential therapeutics or imaging tools, such as the inflammation that can occur when using viral-based delivery approaches.[3, 4] Thus, they offer the opportunity to gain insight into potentially safer and more tractable methodologies.[5] For example, cell-derived exosomes are promising drug delivery systems as they are one mechanism for natural extracellular communication.[6-10] Still, new approaches are needed, given that the complexity and variability of biomimetic tools from cellular sources appropriate for the nervous system reduces their potential for scalable precision medicine.[11]

Functionalized nanoparticles (NPs) have high potential as well-defined carriers for the selective and targeted delivery of therapeutic cargo to neural cells due to their size scale.[12, 13] For example, NPs have been used for the functional delivery of drugs to the rodent brain in multiple pathologies.[14-16] Various surface modifications, such as coupling targeting peptides[17] or antibodies[18] to NPs or modifying surface charge for selective neuron-specific targeting,[19] have been employed to increase targeting efficacy. Alternatively to NPs, exosome-like lipid nanovesicles (NVs) have been used as both contrast agents and drug delivery vehicles to the brain while mimicking neural cellular communication.[20, 21] However, standardized protocols for the storage and characterization of NVs have yet to be fully established,[22, 23] while the low yield from biological sample sources[24] reduces the potential of translating NVs to clinical applications. Here, we sought to devise and optimize enhancements to existing lipid NVs using a well-defined and scalable cell source.

Previously, we endeavored to achieve enhanced bioactivity targeted to specific cell types by developing innovative hybrid biomimetic NVs that took advantage of specific cell types (e.g., native cellular targeting moieties) and synthetic NPs (e.g., ease of fabrication, scalability, and reproducibility) while bridging the gaps in therapeutic translation.[5, 23] In particular, we demonstrated that the incorporation of leukocyte-derived plasma membrane proteins into the phospholipid bilayer of NVs enables immune system avoidance and association with inflamed endothelial cells while delivering a therapeutic payload.[25] We also determined the integration location and orientation of these membrane proteins on the NV lipid membranes and revealed an equal distribution of the cytoplasmic and exoplasmic domains on one representative leukocyte-derived membrane protein, CD11b.[26] Moreover, the biomimetic properties of these NVs resulted from the transfer of cellular adhesion proteins to the surface of NVs, which then mediated protein–protein interactions with target cells.[27] Given that cellular interactions of neurons are in part attributed to cell–cell binding of adhesion proteins at the cell membrane surface, a similar approach for targeting neural cell types holds promising potential.[28, 29] Nonetheless, testing of this approach with human neural cells (in order to aid in potential clinical translation) has been hampered by the lack of pure cell sources for reproducible and scalable production. Recent advances in the differentiation of human pluripotent stem cells (hPSC) into specific neural cell types[30, 31] may enable the generation of biomimetic NVs and experimental testing platforms which, compared to platforms using rodent-derived neural cells, would be less likely to induce an immunogenic reaction in humans and thus more appropriate for clinical translation.

Based on this premise, we have developed and defined a new class of biomimetic human neural NVs (a.k.a. neurosomes) using a reproducible and scalable protein source from a pure population of rapidly derived hPSC-derived excitatory cortical neurons (iNeurons). Specifically, we used a bottom-up microfluidic-based synthesis method to bioengineer our novel NVs by combining phospholipids with the membrane proteins from iNeurons. We found that incorporation of neuron-derived membrane proteins does not affect the physicochemical properties of NVs and, in fact, enhances their uptake into cultured neurons. We further confirmed proof-of-principle cellular targeting efficacy both in vitro and in vivo using sphere (a.k.a. organoid) cultures and direct administration to the rodent trigeminal ganglion, respectively.[32] These studies advance the current paradigm of NV bioengineering for improved cellular targeting within the nervous system.

 

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