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MODULAR, OXYGEN-GENERATING MICROBEAD MATERIALS FOR SUPPORTING CELL VIABILITY AND FUNCTION

20220395463 · 2022-12-15

    Inventors

    Cpc classification

    International classification

    Abstract

    The present disclosure provides for spherical microbeads, methods of making, and methods of use. The spherical microbeads can be tailored to deliver one or more agents over a desired time frame (e.g., short burst or extended-release or combinations thereof). For example, spherical microbeads can be used for the extended-release of oxygen. The spherical microbeads are amendable for an injectable approach and/or ease of integration within cellular implants due in part to their spherical dimensions and size.

    Claims

    1. A composition comprising: a plurality of spherical microbeads having the characteristic for extended release of oxygen for a first time frame, wherein the microbead has an average particle diameter of about 100 to 1000 μm, wherein the microbeads have a hydrophobic polymeric support structure containing solid oxygen-generating peroxide particles in an amount sufficient for extended release of oxygen.

    2. The composition of claim 1, wherein the microbead each have the characteristic of extended release of oxygen for about 30 days or more.

    3. The composition of claim 1, wherein the microbeads each have the characteristic of extended release of oxygen for about 1 week or more.

    4. The composition of claim 1, wherein the microbeads each have the characteristic of extended release of oxygen at levels of 1×10.sup.−6 mmol of oxygen per day or more for about 30 days or more.

    5. The composition of claim 1, wherein the hydrophobic polymeric support structure is made of a material selected from: organosilicones, poly(ethersulfone), poly(ethylene oxide terephthalate) block copolymers, polysulfone, and combinations thereof.

    6. The composition of claim 1, wherein the solid oxygen-generating peroxide particles is a CaO.sub.2 particle.

    7. The composition of claim 1, wherein the solid oxygen-generating peroxide particles have a diameter of about 1 to 50 μm.

    8. The composition of claim 1, wherein the microbeads have a weight ratio of hydrophobic polymeric support structure material to solid oxygen-generating peroxide particles of about 1:1 to 99:1 or optionally about 1 to 10:1.

    9. The composition of claim 1, wherein the microbeads have an outer layer that is made of a material selected from: organosilicones, poly(ethersulfone), poly(ethylene oxide terephthalate) block copolymers, polysulfone, and combinations thereof and optionally has a thickness of about 11 to 25 μm, optionally, the outer layer includes a therapeutic agent, a solid oxygen-generating peroxide particle, or a combination thereof.

    10. The composition of claim 1, wherein the microbeads have porogens within the microbead, optionally wherein the porogens are selected from salt, glucose, or hydrogels or a combination thereof.

    11. The composition of claim 1, wherein the microbeads have a therapeutic agent within the pores, wherein the microbeads have a characteristic for extended release of the therapeutic agent for a second time frame.

    12. The composition of claim 11, wherein the microbead each have the characteristic of extended release of the therapeutic agent for about 30 days or more.

    13. The composition of claim 11, wherein the microbead each have the characteristic of extended release of the therapeutic agent for about 3 days or more.

    14. A composition comprising: a plurality of spherical microbeads, wherein the microbead has an average particle diameter of about 100 to 1000 μm, wherein the microbeads have a hydrophobic polymeric support structure containing solid oxygen-generating peroxide particles in an amount sufficient for extended release of oxygen, wherein the microbeads each have the characteristic of extended release of oxygen at levels of 1×10.sup.−6 mmol of oxygen per day or more for about 30 days or more.

    15. The composition of claim 14, wherein the microbeads have porogens within the microbead, wherein the porogens are selected from salt, glucose, or hydrogels or a combination thereof, wherein the microbeads have a therapeutic agent within the pores, wherein the microbead each have the characteristic of extended release of the therapeutic agent for about 30 days or more.

    16. The composition of claim 15, wherein the hydrophobic polymeric support structure is made of a material selected from: organosilicones, poly(ethersulfone), poly(ethylene oxide terephthalate) block copolymers, polysulfone, and combinations thereof, wherein the solid oxygen-generating peroxide particles is a CaO.sub.2 particle.

    17. A composition comprising: a plurality of spherical microbeads having the characteristic for extended release of oxygen for a first time frame, wherein the microbead has an average particle diameter of about 100 to 1000 μm, wherein the microbeads have a hydrophobic polymeric support structure containing solid oxygen-generating peroxide particles in an amount sufficient for extended release of oxygen, wherein the microbeads have an outer layer that is made of a material selected from: organosilicones, poly(ethersulfone), poly(ethylene oxide terephthalate) block copolymers, polysulfone, and combinations thereof, the wherein outer layer has a thickness of about 11 to 25 μm, and wherein the outer layer includes a therapeutic agent, a solid oxygen-generating peroxide particle, or a combination thereof.

    18. The composition of claim 17, wherein the microbeads have porogens within the microbead, wherein the porogens are selected from salt, glucose, or hydrogels or a combination thereof, wherein the microbeads have a therapeutic agent within the pores.

    19. The composition of claim 18, wherein the microbead each have the characteristic of extended release of the therapeutic agent for about 3 days or more.

    20. The composition of claim 19, wherein the hydrophobic polymeric support structure is made of a material selected from: organosilicones, poly(ethersulfone), poly(ethylene oxide terephthalate) block copolymers, polysulfone, and combinations thereof, wherein the solid oxygen-generating peroxide particles is a CaO.sub.2 particle.

    Description

    BRIEF DESCRIPTION OF THE DRAWINGS

    [0007] Further aspects of the present disclosure will be more readily appreciated upon review of the detailed description of its various embodiments, described below, when taken in conjunction with the accompanying drawings.

    [0008] FIG. 1 illustrates a schematic of microbead fabrication and layering.

    [0009] FIGS. 2A-2C illustrate SEM Images of unmodified (FIG. 2A) microporous (FIG. 2B) and layered microporous oxygen-generating microbeads (FIG. 2C).

    [0010] FIG. 3 illustrates modular microbead prototypes, their release profiles, and properties.

    [0011] FIG. 4 illustrates an overview of release rates for microporous oxygen-generating microbeads (also referred to as “MOBs”), layered microporous solid oxygen-generating microbeads (LMOBs), and high-loading layered microporous oxygen-generating microbeads (HLMOB) compared to unmodified microporous oxygen-generating microbeads (oxybead).

    [0012] FIG. 5 illustrates the release of 17β-Estradiol (E2) from 25 mg of LMOBs layered with a 0.01 wt % solution of E2 in PDMS. O.o.r indicates values out of the assay detection range

    [0013] FIG. 6 illustrates live/dead imaging of microbeads and Min6 β-cells encapsulated within an agarose hydrogel. Gels were cultured over 72 hrs under hypoxic conditions before analysis

    [0014] FIG. 7 illustrates AlamarBlue fluorescence and total insulin content of agarose-encapsulated Min6 after 72 hrs of hypoxic culture.

    [0015] FIG. 8 illustrates live/dead imaging, AlamarBlue fluorescence, and total insulin content of agarose hydrogel containing microbeads and primary rat islet cells. Gels were cultured over 48 hrs under hypoxic conditions before analysis

    [0016] FIG. 9 illustrates total insulin content of C57BL/6 islets after transplantation in the murine kidney capsule alongside oxygen generating microbeads

    DETAILED DESCRIPTION

    [0017] This disclosure is not limited to particular embodiments described, and as such may, of course, vary. The terminology used herein serves the purpose of describing particular embodiments only, and is not intended to be limiting, since the scope of the present disclosure will be limited only by the appended claims.

    [0018] Where a range of values is provided, each intervening value, is to the tenth of the unit of the lower limit unless the context clearly dictates otherwise, between the upper and lower limit of that range and any other stated or intervening value in that stated range, is encompassed within the disclosure. The upper and lower limits of these smaller ranges may independently be included in the smaller ranges and are also encompassed within the disclosure, subject to any specifically excluded limit in the stated range. Where the stated range includes one or both of the limits, ranges excluding either or both of those included limits are also included in the disclosure.

    [0019] As will be apparent to those of skill in the art upon reading this disclosure, each of the individual embodiments described and illustrated herein has discrete components and features which may be readily separated from or combined with the features of any of the other several embodiments without departing from the scope or spirit of the present disclosure. Any recited method may be carried out in the order of events recited or in any other order that is logically possible.

    [0020] Embodiments of the present disclosure will employ, unless otherwise indicated, techniques of inorganic chemistry, materials science, nanotechnology and the like, which are within the skill of the art. Such techniques are explained fully in the literature.

    [0021] Prior to describing the various embodiments, the following definitions are provided and should be used unless otherwise indicated.

    [0022] Unless otherwise defined, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art of chemistry, materials science, medicine, and/or nanotechnology. Although methods and materials similar or equivalent to those described herein can be used in the practice or testing of the present disclosure, suitable methods and materials are described herein.

    [0023] As used in the specification and the appended claims, the singular forms “a,” “an,” and “the” may include plural referents unless the context clearly dictates otherwise. Thus, for example, reference to “a support” includes a plurality of supports. In this specification and in the claims that follow, reference will be made to a number of terms that shall be defined to have the following meanings unless a contrary intention is apparent.

    Discussion

    [0024] Embodiments of the present disclosure provide for spherical microbeads, methods of making, and methods of use. Spherical microbeads of the present disclosure can be tailored to deliver one or more agents over a desired time frame (e.g., short burst or extended-release or combinations thereof). For example, spherical microbeads of the present disclosure can be used for the extended-release of oxygen. The spherical microbeads are amendable for an injectable approach and/or ease of integration within cellular implants due in part to their spherical dimensions and size. In an aspect, the spherical microbeads provide for a customizable oxygen generating material that easily integrates into any cellular transplant to minimize hypoxia-induced cell death by locally delivering the appropriate amount of oxygen to the cells over a desired time frame (e.g., on the order of day or 30 days or longer), while also providing the option to simultaneously deliver other therapeutic agents over the desired time frame. The flexibility and options for delivering multiple agents allow the spherical microbeads to be used as a microbead platform or for integration into a 3D scaffold.

    [0025] Microbeads for delivering dynamic, extended-release of oxygen is disclosed. The microbead diameter can range from 100 to 1000 μm. The geometrical shape is predominantly (e.g., about 95-100%) or substantially spherical (e.g., about 80 to 95%). The composition can include a hydrophobic polymeric support structure and optional outer layers of polymeric material. The hydrophobic polymeric support structure can contain one or more types of agents, such as solid oxygen-generating peroxide particles or soluble therapeutic agents. With this design, the microbeads can be tailored to release more than 1×10.sup.−6 mmol of oxygen per day over an extended time period (e.g. over 30 days). The weight ratio of the hydrophobic polymeric support structure to solid peroxide particles can range from 1:1 to 99:1 or 20:80 to 80:20 or 30:70 to 70:30. Alongside fabrication of the base microbead platform, further methods for microbead modification are detailed, including porogen inclusion and use of outer polymer layering, to provide for tailored and unique oxygen release profiles and/or co-delivery systems for release of oxygen and another agent such as a therapeutic agent.

    [0026] Compositions of the present disclosure provide for a plurality of spherical microbeads that have the characteristic for extended release of one or more agents over a time frame. The extended release can be tailored as desired by designing the microbeads to release over a time frame of a week to a few weeks or 30 days or more. The agent can include solid oxygen-generating peroxide particles or a therapeutic agent (e.g., 17β-estradiol, dexamethasone, cylosporin, fingolimod, fluticasone propionate, mometasone furoate, and other therapeutic glucocorticoids or therapeutic proteins such as CXCL12 and TGF-beta). The microbead can have an average particle diameter of about 100 to 1000 μm or with tailored ranges based on desired applications (e.g. about 100-200 μm for microscale, about 300-600 μm for macroencapsulation). The microbeads have a hydrophobic polymeric support structure that can be biocompatible. The hydrophobic polymeric support structure material can be mixed with one or more types of agents (e.g., solid oxygen-generating peroxide particles, therapeutic agents) in an amount sufficient for extended release of agent for the desired time frame. In a particular aspect, the agent can be an oxygen-generating agent and the microbead can have the characteristic of extended release of oxygen at levels of 1×10.sup.−6 mmol of oxygen per day for about 30 days or more. The time frame can be customized to less than 14 days to over 30 days, depending on the desired application and oxygen needs of the tissue.

    [0027] The hydrophobic polymeric structure can be made of a material selected from: organosilicones, poly(ethersulfone), poly(ethylene oxide terephthalate) block copolymers, polysulfone, and combinations thereof. The weight ratio of biocompatible polymeric support to agent(s) can range from 1:1 to 99:1 or about 1:1 to 10:1 or 20:80 to 80:20 or 30:70 to 70:30 depending on the intended use (e.g., concentration to be released as a function of time for a desired time frame).

    [0028] The agent can be a solid oxygen-generating peroxide particle. The solid oxygen-generating particles can be CaO.sub.2, MgO, SPO, or other reactive peroxides. The solid oxygen-generating peroxide particles have a diameter of about 1 to 50 μm and become encapsulated within the polymeric structure. After exposure and migration of water into the microbead structure, peroxide particles react to rapidly release gaseous oxygen into the surrounding environment.

    [0029] In addition to an agent, the hydrophobic polymeric support structure material can be mixed with porogens that can be used to further modulate the release of the agents. The porogen can include salt, glucose, or hydrogels such as PEG.

    [0030] The modulation of the release time frame can also be tailored by applying an outer layer on the surface of the primary spherical microbeads. The microbeads can have an outer layer that is made of a material selected from: organosilicones, poly(ethersulfone), poly(ethylene oxide terephthalate) block copolymers, polysulfone, and combinations thereof. The outer layer can have a thickness of about 5 to 25 μm. In addition, the microbeads can be tailored so that one or more types of agents (e.g., a therapeutic agent, a solid oxygen-generating peroxide particle, or a combination thereof) or porogens are included in the outer layer.

    [0031] The biocompatible polymeric structure that comprises the microbead is non-degradable and hydrophobic, which provides unique control in the migration of water into the microbead structure, as well as in the release of the entrapped agent. For peroxide-based reactions, the resulting internal reaction of the housed oxygen-generating particles results in release of oxygen as well as sub-cytotoxic levels of hydrogen peroxide (H.sub.2O.sub.2) and Ca.sup.+ ions.

    EXAMPLE

    [0032] To address challenges of other technologies, oxygen-generating microbeads were designed, which permit easy manipulation within 3D structures and greater geometric flexibility. To facilitate improved, unique oxygen-release profiles, a process of generating porosity and modular layering of polymer was developed. Inclusion of these modifications allows for reduction in burst release of oxygen and extended release period due to greater control of osmotic gradients resulting in fundamentally different and improved oxygen release dynamics.

    [0033] Calcium peroxide (CaO.sub.2) was loaded within PDMS and homogenously distributed using a THINKY Mixer at 2000 rpm for 1 minute. If porosity within the polymeric structure was desired for the specific application, micron-scale porogens (i.e., salt particles) were also mixed into the PDMS alongside CaO.sub.2 particles. The resultant mixture was fabricated into cured microbeads via emulsion in 100° C. Polyethylene glycol (PEG) 8000 liquid (FIG. 1). If further modification was desired in order to facilitate different release profiles or the co-release of another therapeutic agent, microbeads were then dried and mixed into a PDMS, PDMS-CaO.sub.2, and/or PDMS-Therapeutic solution and injected into a vigorously stirred PEG 8000 liquid. After thermally curing at 100° C. for 2 hours, microbeads within the PEG media were submerged in a solution of 1% Pluronic-127 to dissolve PEG and prevent clumping of the microbeads due to hydrophobic-hydrophobic interactions. Microbeads were sorted using metal sieves to obtain the desired size range based on the application (e.g., about 100-600 micrometers in diameter). The resulting microbead size and shape were confirmed using a Scanning Electron Microscope (SEM).

    [0034] To characterize release, 10-25 mg of microbeads were immersed in 1 ml PBS solution at 37° C. for a 30-day in vitro release study. The kinetic release of oxygen was recorded by an optical sensor in a sealed chamber, hydrogen peroxide was characterized by colorimetric assays. To evaluate the ability of the oxygen-generating microbeads to mitigate hypoxia-induced beta cell death and dysfunction in vitro, different bead formulations (to be referred to as microporous solid oxygen-generating peroxide particles or beads) were mixed with Min6 beta cells or primary rat islet cells and co-encapsulated within an agarose hydrogel (3.5×10.sup.6 Min6 cells or 700 IEQ rat islets per construct) and incubated under low oxygen (0.01 mM oxygen tension) for 2 to 3 days. Beta cell viability and functionality were assessed by live/dead staining, Alamar Blue, and total insulin assays. For kidney capsule studies, mouse islets (400 IEQ) were isolated from C57BL/6 and then transplanted alongside 40 fibronectin-coated oxygen-generating microbeads, with a control group having blank-PDMS microbeads. After 24 hrs, kidneys were explanted, and total insulin content was quantified using ELISA.

    [0035] Microporous solid oxygen-generating peroxide particles or microbeads were successfully fabricated into the desired size ranges of either 100-200 or 300-600 μm. SEM Images confirmed the spherical shape and size of the microbead (FIG. 2A). SEM imaging of un-layered and layered microporous solid oxygen-generating peroxide beads demonstrated creation of porosity in the beads as well as successful conformal layering of (FIG. 2B-C). The measured in vitro release profiles indicated that the solid oxygen-generating peroxide beads could generate oxygen >8×10.sup.−6 mmol per day for over 30 days (FIG. 3A) and layered microporous solid oxygen-generating peroxide beads could generate oxygen >8×10.sup.−4 mmol per day for over 30 days (FIG. 3C). Microporous beads without a layer resulted in increased oxygen production, inferring that the layering process successfully controlled osmotic pressure (FIG. 3B), allowing for more sustained release of oxygen compared to unmodified beads. Further modification through varying the CaO.sub.2 loading in combination with porosity and layering resulted in distinct kinetics, demonstrating the modularity of the material and greater flexibility for alternative applications (FIG. 3D-F). Overview of release profiles for all types of oxygen-generating microbeads is presented in FIG. 4.

    [0036] To demonstrate the potential for the layering process to be used for release of multiple therapeutics simultaneously, microporous solid oxygen-generating peroxide beads were layered with the pro-angiogenic therapeutic 17β-Estradiol (E2) suspended in PDMS. Quantifying release in vitro demonstrated sustained release of E2 from the outer polymer layer over 7 days, showing the potential for this platform to co-deliver oxygen and other therapeutics to support the engraftment of transplanted cells in cell-based therapies (FIG. 5).

    [0037] Following 3-day in vitro culture with Min6 β-cells under hypoxic conditions, live/dead whole-mount images revealed a homogenous distribution of viable cells throughout the agarose macroconstruct containing oxygen-generating microbeads (FIG. 6; bottom row). This was in stark comparison to control constructs that contained PDMS-only microbeads, which exhibited viable cells only on the outer periphery of the construct ((FIG. 6; top row). This overall loss in viability was quantified via total metabolic activity using AlamarBlue. This assay showed over a 2.5-fold increase in overall metabolic activity, when compared to control constructs (FIG. 7A) for microporous solid oxygen-generating peroxide beads and a 2-fold increase for layered microporous solid oxygen-generating peroxide beads (FIG. 7C). This indicates that bead formulations can successfully support MIN6 metabolic activity under hypoxic conditions. Further, total insulin levels for groups with microporous oxygen-generating microbeads and layered microporous oxygen-generating microbeads were over 1.5-fold higher than the control group under the same hypoxic condition (FIG. 7B & D). Same trends were observed following 2-day in vitro culture with primary rat islet cells under hypoxic conditions, as agarose hydrogel containing oxygen-generating microbeads had more viable cells across the whole construct (FIG. 8A), 1.9-fold increased overall metabolic activity (FIG. 8B), and 1.6-fold increased total insulin content (FIG. 8C), when compared to control constructs that contained PDMS-only microbeads.

    [0038] Co-transplant of C57BL/6 mouse islets alongside microbeads in a murine kidney capsule model resulted in an increase in total insulin content after 24 hours compared to islets transplanted alongside PDMS-only

    [0039] The microporous oxygen-generating microbead based biomaterial can be reproducibly fabricated into a microbead form within controlled size ranges depending on the desired application. This microbead platform can be further modified to produce improved, unique release profiles not previously seen with this biomaterial. These microbeads can generate oxygen for more than 30 days, with minimal cytotoxic by-products. Layering instead with therapeutics suspended in PDMS allowed for sustained release of a pro-angiogenic agent, demonstrating the potential for this platform to permit the local release of multiple therapeutics simultaneously. Compared to control PDMS-only microbeads, the co-culture of beta cells with microbeads within immunoisolatory agarose macrogels resulted in sustained and significant elevations in viability and functionality under hypoxic condition in vitro. Co-transplantation of C57BL/6 islets with these modular microbeads into the murine kidney capsule resulted in significantly higher total insulin content after 24 hrs demonstrating the potential of this platform to provide oxygen in microscale transplant environments. With these promising results and the flexibility of the microbead platform, this approach could be easily translated to numerous tissue engineering platforms.

    REFERENCE LIST

    [0040] 1. Coronel et al., Biomaterials, 2019, 210; p1-11. [0041] 2. Coronel et al., Biomaterials, 2017, 129; p139-151. [0042] 3. Pedraza E, et al., Proc Natl Acad Sci USA, 2012, 109; p4245-4250.