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Acrylic Resins

Acrylic Resins are a class of synthetic resins derived from acrylic acid and its derivatives.
These materials are widely used in a variety of applications, including coatings, adhesives, paints, and plastics.
Acrylic resins offer excellent weather resistance, color stability, and optical clarity, making them a popular choice for both industrial and consumer products.
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Most cited protocols related to «Acrylic Resins»

1
Atmospheric Pressure Cell Culture Device
Our dish sample holder comprised upper Al and lower acrylic resin portion that maintained the sample solution at atmospheric pressure between the SiN films (Fig. 1). The upper W-coated SiN film was attached to the Al holder using two-sided sticky tape (No. 7602, Teraoka Seisakusho Co., Ltd, Tokyo, Japan). The W layer on SiN film was connected to the Al holder using silver conductive ink (CW2900, ITW Chemtronics, Kennesaw, GA, USA). A hand-made Al holder (15 × 15 mm square) was attached under a 35-mm culture dish adhered with double-sided tape to a 4 × 4 mm square hole in the centre (Fig. 1a,a’). A 50-nm-thick SiN film in the 0.4 × 0.4 mm square window of a Si frame (4 × 4 mm) was fixed to the square hole in the culture dish bottom. The dish was subsequently UV sterilised for 17–18 h.
4T1E/M3 mouse breast cancer cells31 32 were cultured in the holder dish for 4–5 days as described above. Next, the Al holder containing cells and second SiN film on an acrylic plate were attached and sealed as described above (Fig. 1c,c’). The Al holder received voltage bias from four nickel–hydrogen batteries (approximately 8 V each), with a total bias voltage of approximately −32 V. The resin holder, which had high electrical resistivity, insulated the terminal underside of the holder from the metal-coated SiN film (Fig. 1d).
Okada T, & Ogura T. (2016). Nanoscale imaging of untreated mammalian cells in a medium with low radiation damage using scanning electron-assisted dielectric microscopy. Scientific Reports, 6, 29169.
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Publication 2016
Acrylic Resins Atmospheric Pressure Cells Electric Conductivity Electricity Hydrogen Hyperostosis, Diffuse Idiopathic Skeletal Malignant Neoplasm of Breast Metals Mus Nickel Reading Frames Resins, Plant Silver
2
Finite Element Analysis of Molar Crown Simulation
-Generation of the Geometric Models
A 3D model of a sound tooth was scanned (InEos, Sirona Dental Systems GmbH, Bensheim, Germany) generating a stereolithographic file. The file was exported to CAD Rhinoceros software (Rhinoceros version 5.0 SR8, McNeel North America, Seattle, WA, USA). The generation of the geometric model followed the methodology in Dal Piva et al. (25 (link)), with similar characteristics. The model was replicated in five models for in vitro mechanical testing of molar crown simulation, according to the abutment preparation related in the literature ( Table 1). A preparation for a full-monolithic molar crown was designed with 5.5 mm of height and 12 degrees of occlusal convergence in the axial walls for all groups. Next, a 70-µm thick cement layer was created (27 (link)) between the intaglio surface of the restoration and the external bonding surface of the abutment.
Group distribution according to the substrate design, average (aS) and stress peak values (Sp) in MPa and stress concentration factor (SC) obtained in the restoration.-Finite element analysis (FEA)
Five different abutment preparations (Fig. 1) were obtained to determine the substrate influence on the crown behavior during a mechanical test. The crown model was defined to simulate zirconia reinforced lithium disilicate glass-ceramic [Vita Suprinity, Vita Zhanfabrick, Bad Säckingen, Germany, (E) = 70 GPa and Poisson ratio (ν) = 0.23] (28 (link)), embedded in the acrylic resin presented [E = 2.7 GPa and ν = 0.35] by a dentin root [ E = 18.6 GPa and ν = 0.32] or by an epoxy root [E = 18 GPa and ν = 0.30] (29 (link)). The incorporated resin cement had E = 6 GPa and ν = 0.30 (linear shrinkage = 2.7%) (27 (link)).

Illustration of the in vitro specimen and the modeling substrates design. A) In vitro specimen embedded in acrylic resin. B) Tooth+pl: A human tooth embedded into acrylic resin with a simulated periodontal ligament. C) Tooth-pl: A human tooth embedded into acrylic resin without a simulated periodontal ligament. D) ER+pc: A tooth made of epoxy resin and root with the exact geometry of dentin root. E) ER-pc: A solid epoxy resin root similar to a dye manufactured in a CAD/CAM facility. F) SiER: A solid epoxy substrate without an anatomic root.

The models were imported through STEP format to the analysis software (ANSYS 17.2, ANSYS Inc., Houston, TX, USA), in which they were divided into mesh composed by nodes (mean value = 183,147, standard deviation = 22,189) and tetrahedral elements (mean value = 102,510, standard deviation = 10,256) (Fig. 2). The aspect ratio of mesh metrics presented average of 1.82 with a standard deviation of 0.49. Mechanical properties of each structure/material were inserted into the analysis software and each material was considered isotropic and homogeneous. Non-linear contact were considered as “Non-separated” between restoration/resin cement/tooth, in which the target and contact surfaces are tied for the remainder of the analysis, although sliding is permitted (26 (link)). The contact between the tooth and the fixation cylinder was considered perfectly bonded. Model fixation occurred at the base of the acrylic resin cylinder in all groups and an axial load of 600 N (32 (link),34 (link)) was applied to the occlusal surface considering the tripoidism concept (26 (link)). A mesh convergence test (10%) was performed to guarantee that the mesh would not interfere in the results (30 (link)). To determine the average stresses, stress peaks and stress concentration factors, one hundred highest peaks were observed in each restoration.

A) Mesh generation. B) 600-N load application area/points.

Dal Piva A.M., Tribst J.P., Borges A.L., de Melo R.M, & Bottino M.A. (2019). Influence of substrate design for in vitro mechanical testing. Journal of Clinical and Experimental Dentistry, 11(2), e119-e125.
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Publication 2019
Acrylic Resins Dental Cements Dental Health Services Epoxy Resins Glass ceramics Homo sapiens lithia disilicate Models, Dental Molar Periodontal Ligament Resin Cements Sound Tooth Tooth Root VITA Suprinity zirconium oxide
3
Mechanical Coupler for Reliable Muscle Contraction Sensing
Muscle contraction is associated with volumetric and stiffness changes, which exert radial forces (or pressures). A force-sensitive resistor (FSR) placed on a patient’s skin in correspondence with a muscle belly was used to sense contraction. Generally, FSRs consist of a conductive polymer, which changes its resistance when a force is applied to its surface. They can be made small and very thin (e.g., less than 0.5 mm), offer good shock resistance, can operate in moderately hostile environments, and are low-cost. However, there should only be concentrated and uniformly distributed force within the FSR active (or sensing) area for reliable use of the FSR. The assembling of the Interlink FSR [38 ] includes perimetral spacers that separate the two membranes holding the metallic contacts and the conductive polymer. A direct application of the FSR on skin to sense muscle contraction proved to be quite unsatisfactory. The mere sensor, without any mechanical coupler, provided uncertain and unreliable results. Contact with the patient’s skin was unstable and uncertain—the perimetral spacers of the FSR sensor transmits part of the applied force directly to the back of the sensor without involving the sensing area, and prevents the membrane with electrical contacts from properly flexing onto the resistive polymer layer. A specific mechanical coupler was designed in response to these drawbacks (see Figure 1). A rigid spherical cap, made of acrylic resin, provides advantageous force transmission to FSR. The spherical cap base was glued onto the FSR’s sensitive area (leaving out the perimetral spacers) and its convex part was made to face the patient’s skin. When the sensor is applied onto the patient, the dome creates a little subsidence that gently but firmly attaches to the skin. Furthermore, a flat, rigid sheet of plastic was attached to the back of the sensor to prevent improper bending. The elastic modulus of both the spherical cap and the back support were much higher than that of skin and muscle. The mechanical coupler provides a much more convenient and reliable muscle force transmission to FSR.
The assembly of the FSR and the mechanical coupler can be held in place onto a patient’s skin by a belt or other fastening methods (e.g., scotch tape). The increase of muscular transverse section during contraction, as well as the resultant skin stretching, impresses uniform pressure on the FSR active area via the rigid spherical cup. Furthermore, the small mechanical vibrations generated during muscle contraction (i.e., the mechanomyography MMG signal) are suitably transmitted to the FSR sensor.
Esposito D., Andreozzi E., Fratini A., Gargiulo G.D., Savino S., Niola V, & Bifulco P. (2018). A Piezoresistive Sensor to Measure Muscle Contraction and Mechanomyography. Sensors (Basel, Switzerland), 18(8), 2553.
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Publication 2018
Acrylic Resins ARID1A protein, human Electric Conductivity Electricity Face Hostility Metals Muscle Contraction Muscle Rigidity Muscle Tissue Patients Polymers Pressure Shock Skin Tissue, Membrane Vibration
4
Immunogold-based Ultrastructural Morphometry
Specimens were post-fixed in 1% OsO4 for 1 h at 4°C and then they were dehydrated in ethanol and embedded in epoxy resin. Ultrathin sections (40–50 nm) of U87MG were cut at ultramicrotome. Similarly to fixing, post-fixing and embedding procedures were validated on pilot studies and they were reported by current literature as optimal conditions for immunogold-based ultrastructural morphometry. We avoided routine method, which consists in avoiding osmium post-fixing and embedding specimens in acrylic resins after fixing with aldehydes only. In fact, such a procedure despite preserving epitopes impairs the preservation of the finest sub-cellular architecture. The method employed here, which combines aldehyde and mild OsO4 as first and second fixing steps allows minimal epitope covering while preserving cell architecture and providing an optimal “contrast effect” of various cell compartments. This method allows preserving sub-cellular structures with acceptable epitope integrity (Bendayan and Zollinger, 1983 (link); D’Alessandro et al., 2004 (link)).
In fact, osmium enhances the contrast of various cytosolic compartments by marking membranes phospholipids, as clearly confirmed by Swanlund in describing the gold standard of TEM procedures in studying autophagy (Swanlund et al., 2010 (link)). Again, the binding of osmium to cell membranes prevents the formation of membranous artifacts, which may mimic ATG vacuoles.
Post-fixed samples were then embedded using epoxy resin. We used epoxy resin, instead of acrylic resin such as LR White, since it is well-established and commonly used as embedding media for TEM, allowing an optimal ultrastructural resolution.
The post-embedding was carried out collecting ultrathin sections on nickel grids and incubating them in aqueous saturated sodium metaperiodate (NaIO4) for roughly 30 min at room temperature in order to remove OsO4 from the samples. After washing with PBS pH 7.4, ultrathin sections were processed for immunocytochemistry. The NaIO4 is an oxidizing agent which attacks the hydrophobic alkane side-chains of epoxy resin (Bendayan and Zollinger, 1983 (link); Causton, 1984 ) making the sections more hydrophilic and allowing a closer contact between immunogold-conjugated antibodies and the antigens exposed on the surface of each section. The solution enables the detection of specific immunogold placement within a context of subcellular integrity, which allows counting molecules within well-delineated specific cell compartments.
Lenzi P., Lazzeri G., Biagioni F., Busceti C.L., Gambardella S., Salvetti A, & Fornai F. (2016). The Autophagoproteasome a Novel Cell Clearing Organelle in Baseline and Stimulated Conditions. Frontiers in Neuroanatomy, 10, 78.
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Publication 2016
Acrylic Resins Aldehydes Alkanes Antibodies Antigens Autophagy Biologic Preservation Cells Cellular Structures Cytosol Epitopes Epoxy Resins Ethanol Gold Immunocytochemistry LR white Nickel Osmium Oxidants Phospholipids Plasma Membrane sodium metaperiodate Tissue, Membrane Ultramicrotomy Vacuole
5
Ultrastructural immunogold morphometry
Fixing and postfixing solutions and the use of epoxy resin were validated in our previous studies for immunogold-based ultrastructural morphometry [47 (link)]. In fact, a combination of aldehydes, OsO4, and epoxy resin allows a minimal epitope covering, while preserving cell ultrastructure [47 (link), 77 (link), 78 (link)]. In particular, OsO4 binds to cell membranes, thus enhancing the contrast of cytosolic compartments, and it prevents the formation of membrane's artifacts, which may mimic vacuoles. Moreover, epoxy resin is advantageous over acrylic resin in preserving cell morphology.
Postembedding procedure was carried out on ultrathin sections collected on nickel grids, which were incubated on droplets of aqueous sodium metaperiodate (NaIO4), for 30 min, at room temperature in order to remove OsO4. NaIO4 is an oxidizing agent allowing a closer contact between antibodies and antigens by removing OsO4 [77 (link)]. This step improves the visualization of immunogold particles specifically located within a sharp context of cell integrity, and it allows the counting of molecules within specific cell compartments. Then, grids were washed in PBS and incubated in a blocking solution containing 10% goat serum and 0.2% saponin for 20 min, at room temperature. Grids were then incubated with the primary antibody solution containing both rabbit anti-LC3 (Abcam, Cambridge, UK, diluted 1 : 50) and mouse anti-P20S (Abcam, Cambridge, UK, diluted 1 : 50), with 0.2% saponin and 1% goat serum in a humidified chamber overnight, at 4°C. After washing in PBS, grids were incubated with the secondary antibodies conjugated with gold particles (10 nm mean diameter, for gold particle anti-rabbit; 20 nm mean diameter, for gold particle anti-mouse, BB International), diluted 1 : 30 in PBS containing 0.2% saponin and 1% goat serum for 1 h, at room temperature. Control sections were incubated with the secondary antibody only. After washing in PBS, grids were incubated on droplets of 1% glutaraldehyde for 3 min; additional extensive washing of grids on droplets of distilled water was carried out to remove extensive salt traces and prevent precipitation of uranyl acetate.
Lazzeri G., Biagioni F., Fulceri F., Busceti C.L., Scavuzzo M.C., Ippolito C., Salvetti A., Lenzi P, & Fornai F. (2018). mTOR Modulates Methamphetamine-Induced Toxicity through Cell Clearing Systems. Oxidative Medicine and Cellular Longevity, 2018, 6124745.
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Publication 2018
Acrylic Resins Aldehydes Antibodies Antigens Cells Cytosol Epitopes Epoxy Resins Glutaral Goat Gold Immunoglobulins Mus Nickel Oxidants Plasma Membrane Rabbits Saponin Serum Sodium Chloride sodium metaperiodate uranyl acetate Vacuole

Most recents protocols related to «Acrylic Resins»

1
Synthesis of an Acrylic Resin Solution
Not available on PMC !

Example 3

37 parts of ethylene glycol monobutyl ether was placed in a reactor equipped with a thermometer, a thermostat, a stirrer, a reflux condenser, and a dropping funnel; and heated with stirring to maintain the reaction mixture at 110° C. A mixture of 10 parts of styrene, 35 parts of methyl methacrylate, 20 parts of 2-ethylhexyl methacrylate, 5 parts of N,N-dimethylaminoethyl methacrylate, 10 parts of 2-hydroxyethyl methacrylate, 20 parts of methoxy polyethylene glycol monomethacrylate (molecular weight: about 2080), 1 part of azobisisobutyronitrile, and 5 parts of isobutyl alcohol was added dropwise thereto over 3 hours. After the completion of dropwise addition, the mixture was aged at 110° C. for 30 minutes. Subsequently, an additional catalyst mixture of 20 parts of ethylene glycol monobutyl ether and 0.5 parts of azobisisobutyronitrile was added dropwise over 1 hour. After aging at 110° C. for 1 hour, the mixture was cooled, thereby obtaining an acrylic resin (R-3) solution with a solids content of 50%. The obtained resin had a weight average molecular weight of 20000.

US11865576B2. Layered body (2024-01-09). KANSAI PAINT CO., LTD. [JP]. Inventors: Ikumi Ono [JP], Nobuhiko Narita [JP], Hirokazu Okazaki [JP].
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Patent 2024
2-butoxyethanol 2-hydroxyethyl methacrylate Acrylic Resins azobis(isobutyronitrile) isobutyl alcohol Methacrylate Methylmethacrylate monomethoxypolyethylene glycol Parts, Body polyethylene glycol methacrylate Resins, Plant Styrene Thermometers
2
Synthesis of Hydroxy-Containing Acrylic Resin
Not available on PMC !

Example 2

35 parts of propylene glycol monopropyl ether was placed in a reactor equipped with a thermometer, a thermostat, a stirrer, a reflux condenser, a nitrogen inlet tube, and a dropping funnel; and heated to 85° C. A mixture of 32 parts of methyl methacrylate, 27.7 parts of n-butyl acrylate, 20 parts of 2-ethylhexyl acrylate, 10 parts of 4-hydroxybutyl acrylate, 3 parts of hydroxypropyl acrylate, 6.3 parts of acrylic acid, 1 part of 2-acryloyloxyethyl acid phosphate, 15 parts of propylene glycol monopropyl ether, and 2.3 parts of 2,2′-azobis(2,4-dimethylvaleronitrile) was added dropwise over 4 hours. After the completion of dropwise addition, the mixture was aged for 1 hour. Thereafter, a mixture of 10 parts of propylene glycol monopropyl ether and 1 part of 2,2′-azobis(2,4-dimethylvaleronitrile) was further added dropwise over 1 hour. After the completion of dropwise addition, the mixture was aged for 1 hour. 7.4 parts of diethanolamine was further added, thereby obtaining a hydroxy-containing acrylic resin (R-2) solution with a solids content of 55%. The obtained hydroxy-containing acrylic resin (R-2) had an acid value of 51 mg KOH/g and a hydroxy value of 52 mg KOH/g.

US11865576B2. Layered body (2024-01-09). KANSAI PAINT CO., LTD. [JP]. Inventors: Ikumi Ono [JP], Nobuhiko Narita [JP], Hirokazu Okazaki [JP].
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Patent 2024
Acids acrylate Acrylic Resins diethanolamine Ethers Hypromellose Methylmethacrylate n-butyl acrylate Nitrogen Parts, Body Phosphates Propylene Glycol Thermometers
3
Extender Pigment Dispersion Formulation
Not available on PMC !

Example 8

327 parts of the hydroxy-containing acrylic resin solution (R-2) (solids content: 180 parts), 360 parts of deionized water, 6 parts of Surfynol (registered trademark) 104A (trade name, produced by Evonik Industries AG, an antifoaming agent, solids content: 50%), and 250 parts of Barifine BF-20 (trade name, produced by Sakai Chemical Industry Co., Ltd., barium sulfate powder, average particle size: 0.03 μm) were placed in a paint mixer, and a glass beads medium was added thereto; followed by mixing and dispersing at room temperature for 1 hour, thereby obtaining an extender pigment dispersion (P-3) with a solids content of 44%.

US11865576B2. Layered body (2024-01-09). KANSAI PAINT CO., LTD. [JP]. Inventors: Ikumi Ono [JP], Nobuhiko Narita [JP], Hirokazu Okazaki [JP].
Full text: Click here
Patent 2024
Acrylic Resins Antifoaming Agents Parts, Body Pigmentation Powder Sulfate, Barium
4
Antibacterial Dental Adhesives with Doped TiO2 NPs
Not available on PMC !

Example 4

The antibacterial efficacy of unaltered and experimental (doped) dental adhesive resins against non-disrupted cariogenic (caries producing) biofilms was further assessed in terms of relative luminescence units (RLUs) using a real-time luciferase-based bioluminescence assay. Toward this end, experimental dental adhesive resins containing either N—TiO2 NPs (5%-30%, v/v), N—F—TiO2 NPs (30%, v/v) and N—Ag—TiO2 NPs (30%, v/v) were synthesized by dispersing the nanoparticles in OBSP adhesive resin using a sonicator (4 cycles of 1 min, intervals of 15-sec between cycles; Q700, QSonica, USA). Two non-antibacterial (OBSP, and Scotchbond Multipurpose, 3M ESPE, USA) and one antibacterial (Clearfil SE Protect, Kuraray, Noritake Dental Inc., Japan) commercially available dental adhesive resins were also tested for antibacterial functionalities. Streptococcus mutans biofilms were grown (UA 159-ldh, JM 10; 37° C., microaerophilic) on the surfaces of disk-shaped specimens (n=18/group, d=6.0 mm, t=0.5 mm) for either 24 or 48 hours with or without continuous visible light irradiation (405±15 nm). One set of specimens was fabricated with OBSP and was treated with Chlorhexidine 2% (2 min) that served as our control group. Results for the antibacterial efficacies of both unaltered and experimental dental adhesive resins containing either doped or co-doped TiO2 NPs under continuous visible light irradiation for either 24 or 48 hours, demonstrated that all groups tested displayed similar antibacterial behaviors under continuous visible light irradiation. Such findings suggest that under the conditions investigated (wavelength and power intensity), visible light irradiation had a very strong antibacterial behavior that took place independently of the antibacterial activity of the substrate where biofilms were grown (either antibacterial or not). Such impact made impossible the determination of the materials' real antibacterial efficacies under such light irradiation conditions.

Experiments were then conducted under dark conditions; bacteria were grown in dark conditions for either 24 and 48 hours. The results indicated that the TiO2-containing adhesive resins were more antibacterial than commercially available non-antibacterial dental adhesive resins (such as OptiBond Solo Plus and Scotchbond Multipurpose). The experimental dental adhesive resins containing 30% (v/v) of nanoparticles (N—TiO2 NPs, N—F—TiO2 NPs and N—Ag—TiO2 NPs) displayed antibacterial efficacies in dark conditions that were similar to Clearfil SE Protect (Fluoride-releasing material, Kuraray, Noritake Dental Inc., Japan). S. mutans biofilms grown on specimens treated with chlorhexidine 2% (2 min) displayed the lowest RLU values amongst all groups investigated, thereby confirming the strong antibacterial behavior of non-immobilized chlorhexidine. In addition, the antibacterial effect was demonstrated to be concentration-dependent, wherein experimental adhesive resins containing higher concentrations of antibacterial nanoparticles (either doped or co-doped) displayed stronger antibacterial effects against non-disrupted S. mutans biofilms. Since long intra-oral irradiation periods (24-hour and 48-hour) are impractical and clinically not feasible, associated with the fact that these materials are intended to be used in the oral cavity's dark conditions, these results were considered of paramount importance and clinically relevant for the commercialization pathway of recently developed antibacterial and bioactive nano-filled dental adhesive resins.

Optical and mechanical properties of both unaltered and experimental dental adhesive resins containing 5%-30% (v/v, 5% increments) of N—TiO2 NPs were assessed in terms of color stability and biaxial flexure strength. Color stability (n=5) and biaxial flexure strength (n=8) specimens (d=6.0 mm, t=0.5 mm) were fabricated and tested using a color analysis software (ScanWhite, Darwin Syst., Brazil) and an Instron universal testing machine (cross-head rate=1.27 mm/min), respectively. Color stability measurements were performed immediately after specimen fabrication and after water storage (1, 2, 3, 4, 5, 6 months; 37° C.). The color stability results demonstrated that specimens fabricated using either unaltered or experimental dental adhesive resins containing N—TiO2 NPs (5%-30%, v/v) were subjected to color changes induced by long-term water storage. The highest color variations were observed at two months of water storage (37° C.) for specimens pertaining to experimental groups containing either 5% or 10% of N—TiO2 NPs. Specimens fabricated with unaltered OptiBond Solo Plus have demonstrated color variations that were similar to the color variations observed for the experimental group containing 20% N—TiO2 NPs. Specimens fabricated with 30% N—TiO2 NP-containing dental adhesive resins have shown the least amount of color variation throughout the investigation time (6-mo), and therefore, were considered as the most color stable amongst all materials investigated. From the esthetic standpoint, the human eye can only detect differences in color above a certain threshold (ΔE≥3).

In at least one embodiment, dental composition specimens fabricated with at 30% N—TiO2 NPs displayed color variations that were either lower than or close to the human eye detection capability, thereby corroborating the long-term use of these highly esthetic experimental dental adhesive resins. In at least certain embodiments, the dental compositions contain at least 5% to 80% (v/v) of doped-TiO2 NPs as disclosed herein, such as at least 5% (v/v), at least 6% (v/v), at least 7% (v/v), at least 8% (v/v), at least 9% (v/v), at least 10% (v/v), at least 11% (v/v), at least 12% (v/v), at least 13% (v/v), at least 14% (v/v), at least 15% (v/v), at least 16% (v/v), at least 17% (v/v), at least 18% (v/v), at least 19% (v/v), at least 20% (v/v), at least 21% (v/v), at least 22% (v/v), at least 23% (v/v), at least 24% (v/v), at least 25% (v/v), at least 26% (v/v), at least 27% (v/v), at least 28% (v/v), at least 29% (v/v), at least 30% (v/v), at least 31% (v/v), at least 32% (v/v), at least 33% (v/v), at least 34% (v/v), at least 35% (v/v), at least 36% (v/v), at least 37% (v/v), at least 38% (v/v), at least 39% (v/v), at least 40% (v/v), at least 41% (v/v), at least 42% (v/v), at least 43% (v/v), at least 44% (v/v), at least 45% (v/v), at least 46% (v/v), at least 47% (v/v), at least 48% (v/v), at least 49% (v/v), at least 50% (v/v), at least 51% (v/v), at least 52% (v/v), at least 53% (v/v), at least 54% (v/v), at least 55% (v/v), at least 56% (v/v), at least 57% (v/v), at least 58% (v/v), at least 59% (v/v), at least 60% (v/v), at least 61% (v/v), at least 62% (v/v), at least 63% (v/v), at least 64% (v/v), at least 65% (v/v), at least 66% (v/v), at least 67% (v/v), at least 68% (v/v), at least 69% (v/v), at least 70% (v/v), at least 71% (v/v), at least 72% (v/v), at least 73% (v/v), at least 74% (v/v), at least 75% (v/v), at least 76% (v/v), at least 77% (v/v), at least 78% (v/v), at least 79% (v/v), or at least 80% (v/v), with the balance comprising the curable adhesive resin material, and optionally other components as described elsewhere herein.

The present results demonstrate that experimental dental adhesive resins containing varying concentrations of N—TiO2 NPs display biaxial flexure strengths that are either similar or better than the strength observed for specimens fabricated with the unaltered OBSP. No differences were observed among the flexure strengths of experimental groups, thereby indicating that the presently disclosed materials can behave very similar to commercially available materials when subjected to masticatory forces.

Specimens (d=6.0 mm, t=0.5 mm) of the unaltered resins and experimental dental adhesive resins containing 30% N—TiO2 NPs, 30% N—F—TiO2 NPs and 30% N—Ag—TiO2 NPs were fabricated and characterized using the state of the art scanning electron microscope. This dual focused ion-beam microscope (Dual-FIB SEM/EDS) is capable, through a destructive process, to characterize and map the chemical composition and distribution of elements in three dimensions. The 3-D characterization and localization of components clearly demonstrated that experimental materials containing co-doped nanoparticles (e.g., 30% v/v, N—F—TiO2 NPs) displayed an optimized dispersion of filler particles (part of the original composition) when compared to the filler particle distribution observed on specimens fabricated with the unaltered dental adhesive resin. The 3-D images demonstrated that the experimental adhesive resins had more filler particles per unit volume with a more homogeneous size distribution than the filler fraction and size distribution observed on OptiBond Solo Plus samples. In addition, results showed that larger and more agglomerated filler particles tend to result in a polymer matrix containing more pores per unit volume. This finding was corroborated by the pore-size distribution calculated for the unaltered samples and experimental dental adhesive resin samples, where it is possible to observe that the quantity and sizes of pores formed in experimental materials were smaller when compared to the unaltered OptiBond Solo Plus samples.

In at least one embodiment, the present disclosure includes a dental composition, comprising doped and/or coated TiO2 NPs, and a curable resin material, wherein the curable resin material comprises a polymer precursor component. The TiO2 NPs may comprise at least one dopant or coating selected from the group consisting of N (nitrogen), Ag (silver), F (fluorine), P (phosphorus), and PO4 (phosphate). As noted above, in non-limiting embodiments, the dental composition may comprise a volume to volume ratio of doped TiO2 NPs to curable resin material in a range of 1% to 80% (v/v), 5% to 50% (v/v), or 10% to 40% (v/v), for example. The polymer precursor component may be photocurable. The polymer precursor may be selected from the group consisting of acrylates, methacrylates, dimethacrylates, epoxies, vinyls and thiols. The polymer precursor may be selected from the group consisting of ethylenedimethacrylate (“EDMA”), bisphenol A glycidyl methacrylate (“BisGMA”), triethyleneglycol dimethacrylate (“TEGDMA”), 1,6-bis(methacryloxy-2-ethoxycarbonylamino)-2,4,4-trimethylhexane (UDMA), pyromellitic glycerol dimethacrylate (PMGDM), and 2-hydroxyethyl methacrylate (HEMA). The dental composition may comprise at least one solvent. The at least one solvent may be selected from the group consisting of water, ethanol, methanol, toluene, ethyl ether, cyclohexane, isopropanol, chloroform, ethyl acetate, acetone, hexane, and heptanes. The dental composition may comprise a polymerization initiator. The dental composition may comprise a filler. The dental composition may be selected from the group consisting of dental resins, dental bonding agents, dental adhesives, dental cements, dental restoratives, dentals coatings, dental sealants, acrylic resins, and denture teeth. The dental composition may comprise bioactive and/or antibacterial activity in the absence of visible or ultraviolet light. The dental composition may be used to form a hardened dental article after a photocuring step. In at least one embodiment, the disclosure includes an in vivo dental process, comprising applying the dental composition to at least one of a dental restorative and a dental substrate, and causing the dental restorative to be bonded to the dental substrate via the dental composition after a step of photocuring the dental composition.

Accordingly, the present disclosure is directed to at least the following non-limiting embodiments:

Clause 1. In at least one embodiment the present disclosure includes a dental composition, comprising doped TiO2 nanoparticles, and a curable resin material, wherein the curable resin material comprises a polymer precursor component.

Clause 2. The dental composition of clause 1, wherein the doped TiO2 nanoparticles comprise at least one dopant selected from the group consisting of N (nitrogen), Ag (silver), F (fluorine), P (phosphorus), and PO4 (phosphate).

Clause 3. The dental composition of clause 1 or 2, wherein the doped TiO2 nanoparticles further comprise at least one second dopant selected from the group consisting of N, Ag, F, P, and PO4.

Clause 4. The dental composition of any one of clauses 1-3, comprising a volume to volume ratio of doped TiO2 nanoparticles to curable resin material in a range of 1% to 80% (v/v).

Clause 5. The dental composition of any one of clauses 1-4, comprising a volume to volume ratio of doped TiO2 nanoparticles to curable resin material in a range of 5% to 50% (v/v).

Clause 6. The dental composition of any one of clauses 1-5, comprising a volume to volume ratio of doped TiO2 nanoparticles to curable resin material in a range of 10% to 40% (v/v).

Clause 7. The dental composition of any one of clauses 1-6, wherein the polymer precursor component is photocurable.

Clause 8. The dental composition of any one of clauses 1-7, wherein the polymer precursor is selected from the group consisting of acrylates, methacrylates, dimethacrylates, epoxies, vinyls and thiols.

Clause 9. The dental composition of any one of clauses 1-8, wherein the polymer precursor is at least one selected from the group consisting of ethylenedimethacrylate (EDMA), bisphenol A glycidyl methacrylate (BisGMA), triethyleneglycol dimethacrylate (TEGDMA), 1,6-bis(methacryloxy-2-ethoxycarbonylamino)-2,4,4-trimethylhexane (UDMA), pyromellitic glycerol dimethacrylate (PMGDM), and 2-hydroxyethyl methacrylate (HEMA).

Clause 10. The dental composition of any one of clauses 1-9, further comprising at least one solvent.

Clause 11. The dental composition of any one of clauses 1-10, further comprising a solvent selected from the group consisting of water, ethanol, methanol, acetone, toluene, ethyl ether, cyclohexane, isopropanol, chloroform, ethyl acetate, hexane, and heptanes.

Clause 12. The dental composition of any one of clauses 1-11, further comprising a polymerization initiator.

Clause 13. The dental composition of any one of clauses 1-12, further comprising a filler.

Clause 14. The dental composition of any one of clauses 1-13, wherein the curable resin material is selected from the group consisting of dental resins, dental bonding agents, dental adhesives, dental cements, dental restoratives, dentals coatings, dental sealants, acrylic resins, and denture teeth.

Clause 15. The dental composition of any one of clauses 1-14, comprising bioactive and/or antibacterial activity in the absence of visible or ultraviolet light.

Clause 16. A kit for forming a dental composition, the kit comprising doped TiO2 nanoparticles, and a curable resin material, wherein the curable resin material comprises a polymer precursor component.

Clause 17. The kit of clause 16, wherein the doped TiO2 nanoparticles comprise at least one dopant selected from the group consisting of N (nitrogen), Ag (silver), F (fluorine), P (phosphorus), and PO4 (phosphate).

Clause 18. The kit of clause 16 or 17, wherein the doped TiO2 nanoparticles further comprise at least one second dopant selected from the group consisting of N, Ag, F, P, and PO4.

Clause 19. The kit of any one of clauses 16-18, comprising sufficient doped TiO2 nanoparticles and curable resin material such that the dental composition comprises a volume to volume ratio of doped TiO2 nanoparticles to curable resin material in a range of 1% to 80% (v/v).

Clause 20. The kit of any one of clauses 16-19, comprising sufficient doped TiO2 nanoparticles and curable resin material such that the dental composition comprises a volume to volume ratio of doped TiO2 nanoparticles to curable resin material in a range of 5% to 50% (v/v).

Clause 21. The kit of any one of clauses 16-20, comprising sufficient doped TiO2 nanoparticles and curable resin material such that the dental composition comprises a volume to volume ratio of doped TiO2 nanoparticles to curable resin material in a range of 10% to 40% (v/v).

Clause 22. The kit of any one of clauses 16-21, wherein the polymer precursor component is photocurable.

Clause 23. The kit of any one of clauses 16-22, wherein the polymer precursor is selected from the group consisting of acrylates, methacrylates, dimethacrylates, epoxies, vinyls and thiols.

Clause 24. The kit of any one of clauses 16-23, wherein the polymer precursor is at least one selected from the group consisting of ethylenedimethacrylate (EDMA), bisphenol A glycidyl methacrylate (BisGMA), triethyleneglycol dimethacrylate (TEGDMA), 1,6-bis(methacryloxy-2-ethoxycarbonylamino)-2,4,4-trimethylhexane (UDMA), pyromellitic glycerol dimethacrylate (PMGDM), and 2-hydroxyethyl methacrylate (HEMA).

Clause 25. The kit of any one of clauses 16-24, further comprising at least one solvent.

Clause 26. The kit of any one of clauses 16-25, further comprising a solvent selected from the group consisting of water, ethanol, methanol, acetone, toluene, ethyl ether, cyclohexane, isopropanol, chloroform, ethyl acetate, hexane, and heptanes.

Clause 27. The kit of any one of clauses 16-26, further comprising a polymerization initiator for combining with the doped TiO2 nanoparticles, and curable resin material.

Clause 28. The kit of any one of clauses 16-27, further comprising a filler for combining with the doped TiO2 nanoparticles, and curable resin material.

Clause 29. The kit of any one of clauses 16-28, wherein the curable resin material is selected from the group consisting of dental resins, dental bonding agents, dental adhesives, dental cements, dental restoratives, dentals coatings, dental sealants, acrylic resins, and denture teeth.

Clause 30. The kit of any one of clauses 16-29, wherein the dental composition has bioactive and/or antibacterial activity in the absence of visible or ultraviolet light.

Clause 31. A hardened dental article formed from the dental composition of any one of clauses 1-15, after the dental composition has been photocured.

Clause 32. An in vivo dental process, comprising: applying a dental composition to a dental surface, the dental composition comprising doped TiO2 nanoparticles, and a curable resin material, wherein the curable resin material comprises a polymer precursor component; and causing the dental composition to be bonded to the dental surface by photocuring the dental composition.

Clause 33. The dental process of clause 32, wherein the dental surface is at least one of a dental restorative and a dental substrate.

Clause 34. The dental process of clause 32 or 33, wherein the doped TiO2 nanoparticles comprise at least one dopant selected from the group consisting of N (nitrogen), Ag (silver), F (fluorine), P (phosphorus), and PO4 (phosphate).

Clause 35. The dental process of any one of clauses 32-34, wherein the doped TiO2 nanoparticles further comprise at least one second dopant selected from the group consisting of N, Ag, F, P, and PO4.

Clause 36. The dental process of any one of clauses 32-35, wherein the dental composition comprises a volume to volume ratio of doped TiO2 nanoparticles to curable resin material in a range of 1% to 80% (v/v).

Clause 37. The dental process of any one of clauses 32-36, wherein the dental composition comprises a volume to volume ratio of doped TiO2 nanoparticles to curable resin material in a range of 5% to 50% (v/v).

Clause 38. The dental process of any one of clauses 32-37, wherein the dental composition comprises a volume to volume ratio of doped TiO2 nanoparticles to curable resin material in a range of 10% to 40% (v/v).

Clause 39. The dental process of any one of clauses 32-38, wherein the polymer precursor component is photocurable.

Clause 40. The dental process of any one of clauses 32-39, wherein the polymer precursor is selected from the group consisting of acrylates, methacrylates, dimethacrylates, epoxies, vinyls and thiols.

Clause 41. The dental process of any one of clauses 32-40, wherein the polymer precursor is at least one selected from the group consisting of ethylenedimethacrylate (EDMA), bisphenol A glycidyl methacrylate (BisGMA), triethyleneglycol dimethacrylate (TEGDMA), 1,6-bis(methacryloxy-2-ethoxycarbonylamino)-2,4,4-trimethylhexane (UDMA), pyromellitic glycerol dimethacrylate (PMGDM), and 2-hydroxyethyl methacrylate (HEMA).

Clause 42. The dental process of any one of clauses 32-41, wherein the dental composition further comprises at least one solvent.

Clause 43. The dental process of any one of clauses 32-42, further comprising a solvent selected from the group consisting of water, ethanol, methanol, acetone, toluene, ethyl ether, cyclohexane, isopropanol, chloroform, ethyl acetate, hexane, and heptanes.

Clause 44. The dental process of any one of clauses 32-43, wherein the dental composition further comprises a polymerization initiator.

Clause 45. The dental process of any one of clauses 32-44, wherein the dental composition further comprises a filler.

Clause 46. The dental process of any one of clauses 32-45, wherein the curable resin material is selected from the group consisting of dental resins, dental bonding agents, dental adhesives, dental cements, dental restoratives, dentals coatings, dental sealants, acrylic resins, and denture teeth.

Clause 47. The dental process of any one of clauses 32-46, wherein after curing, the dental composition has bioactive and/or antibacterial activity in the absence of visible or ultraviolet light.

Clause 48. The dental process of any one of clauses 32-47, wherein the dental surface has been acid-etched prior to the application of the dental composition thereon.

While the present disclosure has been described herein in connection with certain embodiments so that aspects thereof may be more fully understood and appreciated, it is not intended that the present disclosure be limited to these particular embodiments. On the contrary, it is intended that all alternatives, modifications and equivalents are included within the scope of the present disclosure as defined herein. Thus the examples described above, which include particular embodiments, will serve to illustrate the practice of the inventive concepts of the present disclosure, it being understood that the particulars shown are by way of example and for purposes of illustrative discussion of particular embodiments only and are presented in the cause of providing what is believed to be the most useful and readily understood description of procedures as well as of the principles and conceptual aspects of the present disclosure. Changes may be made in the formulation of the various compositions described herein, the methods described herein or in the steps or the sequence of steps of the methods described herein without departing from the spirit and scope of the present disclosure. Further, while various embodiments of the present disclosure have been described in claims herein below, it is not intended that the present disclosure be limited to these particular claims.

US11857651B2. Compositions with doped titanium dioxide nanoparticles and methods of use (2024-01-02). The Board of Regents of the University of Oklahoma [US]. Inventors: Fernando Luis Esteban Florez [US], Sharukh Soli Khajotia [US], Adam Justin Rondinone [US].
Full text: Click here
Patent 2024
2-hydroxyethyl methacrylate Acetone Acids Acrylates Acrylic Resins Anti-Bacterial Agents Bacteria Biofilms Bioluminescent Measurements Bisphenol A-Glycidyl Methacrylate chemical composition Chlorhexidine Chloroform Cyclohexane Dental Caries Dental Cements Dental Resins Dentures Epoxy Resins Ethanol ethyl acetate Ethyl Ether Fluorides Fluorine Focused Ion Beam Scanning Electron Microscopy Glycerin Head Heptanes Hexanes Homo sapiens Isopropyl Alcohol JM 10 Light Light, Visible Luciferases Luminescence Methacrylates Methanol Microscopy Mouth Diseases Nitrogen OptiBond SOLO Phosphates Phosphorus Pit and Fissure Sealants Polymerization Polymers Polyvinyl Chloride Radiotherapy Resins, Plant Scanning Electron Microscopy Sclerosis Scotchbond Silver Solvents Streptococcus mutans Sulfhydryl Compounds T.E.R.M. composite resin titanium dioxide Toluene Tooth triethylene glycoldimethacrylate Ultraviolet Rays Vision
5
Perylene Red Pigment Dispersion
Not available on PMC !

Example 7

6 parts of the hydroxy-containing acrylic resin (R-2) (solids content: 3.3 parts), 35 parts of Paliogen Maroon L3920 (trade name, a perylene red pigment, produced by BASF A.G.), and 60 parts of deionized water were placed in a stirring vessel; and homogeneously mixed, followed by further adding 2-(dimethylamino) ethanol to adjust the pH to 7.5. The obtained mixture was placed in a 225-ml resin bottle; and 130 parts of zirconia beads (size: 1.5 mm) were added thereto, followed by hermetically sealing the bottle. The pigment was dispersed for 120 minutes with a shaking-type paint mixer. After the pigment was dispersed, the zirconia beads were filtered through a 100-mesh metallic gauze and removed, thereby obtaining a red pigment dispersion (P-2) with a solids content of 66%.

US11865576B2. Layered body (2024-01-09). KANSAI PAINT CO., LTD. [JP]. Inventors: Ikumi Ono [JP], Nobuhiko Narita [JP], Hirokazu Okazaki [JP].
Full text: Click here
Patent 2024
Acrylic Resins Blood Vessel Ethanol Metals Parts, Body Perylene Pigmentation Resins, Plant zirconium oxide

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