Heat stable hyaluronic acid compositions for dermatological use

Description

BACKGROUND

Skin aging is a progressive phenomenon, occurs over time and can be affected by lifestyle factors, such as alcohol consumption, tobacco and sun exposure. Aging of the facial skin can be characterized by atrophy, slackening, and fattening. Atrophy corresponds to a massive reduction of the thickness of skin tissue. Slackening of the subcutaneous tissues leads to an excess of skin and ptosis and leads to the appearance of drooping cheeks and eye lids. Fattening refers to an increase in excess weight by swelling of the bottom of the face and neck. These changes are typically associated with dryness, loss of elasticity, and rough texture.

A variety of compounds can have an effect on the skin such as wrinkle reduction, antioxidant, haemostatic, vasoconstriction, anti-itching, anti-inflammatory and anti-irritant effects. For example, various vitamins as well and hyaluronic acid (HA) are known to have an effect on skin. Vitamin C is the L-enantiomer of ascorbate and has a well-described role in collagen development. Vitamin C is involved in the hydroxylation of collagen, which allows it to assume its triple-helix structure. Vitamin C is also known for its antioxidant effects and is well tolerated. HA is a natural polysaccharide. It is a polymer of disaccharides that are themselves composed of D-glucuronic acid and N-acetylglucosamine, linked to one another by alternating beta-1,4 and beta-1,3 glycosidic linkages. The polymers of this recurring unit may be from 10²and 10⁴kilo Daltons (kDa) in size, in vivo. Hyaluronic acid represents a natural constituent of the dermis, where it plays an important role in the hydration and elasticity of skin. There is a strong correlation between the water content in the skin and levels of HA in the dermal tissue. As skin ages, the amount and quality of HA in the skin is reduced. These changes lead to drying and wrinkling of the skin.

The use of HA in cosmetic and dermatological applications is known. HA is tolerated well and there is no immunogenicity associated with its use. The low incidence of side effects has lead to the use of HA for the treatment of wrinkles, fine lines, and scars. HA is subject to degradation through different pathways (e.g. enzymatic, temperature, free radicals), and therefore, its longevity in vivo is limited.

Disclosures of HA, vitamin C, and C-glycosides include U.S. patent application Ser. No. 12/393,884; U.S. Pat. No. 6,921,819 (a process for cross-linking solid hyaluronic acid (HA) by reacting it with a polyfunctional linker during hydration of the HA); U.S. Pat. No. 6,685,963 (acrylic particles of HA); U.S. publication 2006/0194758 (a method for making a hydrogel by cross linking high and low molecular weight sodium HAs); U.S. publication 2009/0036403 (cross-linking HA with a tetra functional PEG epoxide to provide “tunably” cross-linked HA); U.S. publication 2009/0143331 (a HA dermal filler with a degradation inhibitor, such as chondroitin sulphate, in order to provide a longer lasting filler); U.S. publication 2009/0143348 (HA combined with a steroid); and U.S. publication 2009/0155314 (HA combined with a botulinum toxin). Additionally, U.S. publications 2009/0148527, 2009/0093755, and 2009/0022808 disclose HA in microspheres, cross-linked with collagen, and coated with a protein, respectively. Further disclosures of HA include: WO 2009/034559 (a process for aesthetic and/or reparative treatment of the skin with compositions that contain at least one C-glycoside derivative); WO 2009/024719 (cosmetic and pharmaceutical compositions that contain HA and a C-glycoside derivative useful for filling recesses/depressions in the skin, restore volume of the body or the face, and to reduce the sign of aging); WO 2007/128923 (a method for preparing a biocompatible gel with controlled release of one or more active lipophilic and/or amphiphilic ingredients); U.S. publication 2009/0018102 (compositions containing HA and at least one retinoid or salt/derivative thereof in combination with an oligosaccharide and a HA degradation inhibitor, to treat wrinkles, lines fibroblast depletions and scars); U.S. Pat. No. 3,763,009 (a process for improving the oxidation resistance of ascorbic acid by subjecting a mixture of ascorbic acid, maltose and/or oligosaccharides to an enzyme derived from genera Aspergillus, Penicillium or others to enzymatically convert the mixture into ascorbic acid glucoside); U.S. Pat. No. 5,616,611 (a α-Glycosyl-L-ascorbic acid that exhibits no direct reducing activity, is stable, and is useful as a stabilizer, quality-improving agent, antioxidant, physiologically active agent, a UV-absorbant in pharmaceutical and cosmetic industries); U.S. Pat. No. 5,843,907 (the production and use of a crystalline 2-O-α-D-glucopyranosyl-L-ascorbic acid suitable for vitamin C enriching agents, food stuffs, pharmaceuticals, and cosmetics); and EP 0539196 (an industrial scale preparation of high purity 2-O-α-D-glucopyranosyl-L-ascorbic acid) and US publication 2002/0151711. Commercial products incorporating HA and/or vitamin C agents include: MESOGLOW® products, REVITACARE®, and NCTF® 135/135HA Mesotherapy products. Each of the above-cited references and printed publications are individually incorporated herein by reference in their entirety.

SUMMARY

Our invention includes a stable dermal filler formulation comprising a hyaluronic acid (HA) and at least one additional ingredient selected from the group consisting of a wrinkle reduction, antioxidant, haemostatic, vasoconstriction, anti-itching, anti-inflammatory and anti-irritant ingredient. Stability of the dermal filler formulation can be determined by subjecting the dermal filler formulation to a heat treatment selected from the group consisting of (a) steam sterilization (equivalently “autoclaving”) and (b) about 32 days at about 45° C., with substantial retention after the heat treatment of one or more of the dermal filler characteristics of being clear, homogenous, and cohesive, and without substantial degradation of the dermal filler formulation after the heat treatment. Preferably the steam sterilization is carried out at a temperature of at least about 120° C., as we have found that a high temperature steam sterilization reduces the sterilization time required while still providing all sterility requirements, without degradation of the dermal filler formulation occurring when the additional ingredients set forth herein are present in the formulation. More preferably, the steam sterilization is carried out at a temperature between about 130° C. and 135° C., because we found that such a particular high temperature steam sterilization not only further reduces the sterilization time required while still providing all sterility requirements but as well can be carried out with little or no degradation of the dermal filler formulation occurring. Preferably, the steam sterilization is carried out for between about one minute and about 10 minutes and more preferably for between about 1 minute and about 5 minutes.

Our invention also includes a steam sterilization stable dermal filler formulation comprising a hyaluronic acid (HA) and at least one additional ingredient selected from the group consisting of wrinkle reduction, antioxidant, haemostatic, vasoconstriction, anti-itching, anti-inflammatory and anti-irritant ingredients, wherein the formulation is substantially clear (i.e. little or no modification of the pre-heat [i.e. steam] treatment dermal filler formulation color occurs as compared to the color of the post heat treatment dermal filler formulation), homogenous, cohesive stable and not substantially degraded after steam sterilization. Degradation can be shown after steam sterilization by, for example, discoloration of the steam sterilized dermal filler formation and/or by a decrease in the homogeneity of the formulation or in other formulation rheological properties. Substantially clear means that on visual inspection the dermal filler formulation both before and after steam sterilization is not opaque. Substantially homogenous means the dermal filler formulation both before and after steam sterilization has the same consistency (eg well mixed throughout). Substantially monophasic means the dermal filler formulation both before and after steam sterilization comprises only one phase, meaning it is a gel with no particles. Substantially cohesive means the ability of the dermal filler formulation both before and after steam sterilization to retain its shape and resist deformation. Cohesiveness is affected by, among other factors, the molecular weight ratio of the initial free HA, the degree of crosslinking, the amount of residual free HA following crosslinking, and the pH of the dermal filler formulation. Moreover, a cohesive dermal filler formulation resists phase separation when tested according to the method disclosed by Example 1A herein.

Our dermal filler formulations are stable after steam sterilization (i.e. at a temperature between about 120° C. to 135° C. or greater). Additionally our dermal filler formulations have long term storage or shelf life stability as shown for example by maintenance of stability of the dermal filler formulations in an environment at about 45° C. for about 32 days (accelerated heat testing), which can be considered to show that stability will be maintained for about 1 to 3 years at room temperature; stability can be determined by substantial retention at room temperature of one or more of the dermal filler characteristics of being clear, homogenous, and cohesive, and without substantial degradation of the dermal filler formulation. Stability of our dermal filler formulations can be determined over a period of or about 25 days to about 35 days at a temperature of about 35° to 50° C. Preferably, as set forth above, the accelerated heat stability testing is carried out for about 32 days at about 45° C. Substantially stable after the accelerated heat (stability) testing carried out as set forth above, or substantially stable after autoclaving or after steam sterilization of the dermal filler formulation, means the dermal filler formulation retains (as being resistant to degradation) at least 80% and preferably at least 90% and most preferably at least about 95% of at least one of its measured characteristics of transparency, pH, extrusion force, rheological characteristics, hyaluronic acid (HA) concentration, sterility, osmolarity, and same additional ingredient concentration. In our dermal filler formulation the HA is preferably cross-linked and the HA can be present in an amount of about 1 to about 40 mg/mL.

An additional ingredient in our dermal filler formulation can be a vitamin B, C or E and the additional ingredient can be present in an amount of about 0.001% to about 10% w/w, and preferably be present in an amount of from about 0.1% to about 3% w/w. Important, the additional ingredient can provide the dermal filler formulation with improved rheological properties resulting in less extrusion force required for administration compared to an HA gel formulation without the additional constituent.

Our invention also includes a method for treating a dermal condition such as fine lines, wrinkles, fibroblast depletions, and/or scars of a patient by administering to the patient an effective amount of a steam sterilization stable dermal filler formulation comprising a hyaluronic acid (HA) and at least one additional ingredient selected from the group consisting of wrinkle reduction, antioxidant, haemostatic, vasoconstriction, anti-itching, anti-inflammatory and anti-irritant ingredients, wherein the formulation is clear, homogenous, cohesive, stable and not degraded after steam sterilization and wherein the appearance of the fine lines, wrinkles, fibroblast depletions, or scars is diminished. The administration can be by sub dermal, intra-dermal or subcutaneous injected (i.e. local injection administration) into a facial skin of the subject.

Our invention also includes a steam sterilization stable dermal filler formulation comprising a hyaluronic acid and at least one additional ingredient selected from the group consisting of AA2G and dexpanthenol, wherein the stability of the dermal filler formulation is significantly increased by the additional ingredient—as shown by the dermal filler formulation having a Δ Tan δ 1 Hz<−0.05.

DRAWINGS

FIG. 1 is a representation of the structure of an ascorbyl-2-glucoside, also known as AA2G™ (Hayashibara Co., Japan).

FIG. 2 is a graph showing the synthesis of pro-collagen (% control) for control, gel+lidocaine 0.3%, AA2G™ 0.6% in phosphate buffer, and gel+AA2G™ 0.6%+lidocaine 0.3%.

FIG. 3 is a graph showing the extrusion force over time (3 yr equivalent at 25° C.) in compositions: control, AA2G™ plus lidocaine, and AA2G™ plus lidocaine and TPGS.

FIG. 4 is a graph showing the pH over time (3 yr equivalent at 25° C.) in compositions: control, AA2G™ plus lidocaine, and AA2G™ plus lidocaine and TPGS.

FIG. 5 is a graph of tan delta 1 Hz over time (3 yr equivalent at 25° C.) in compositions: control, AA2G™ plus lidocaine, and AA2G™ plus lidocaine and TPGS.

FIG. 6 is an HPLC analysis (C18 column, eluent: sodium phosphate buffer (pH=2.2)/2-propanol 10%, 0.7 ml/min; detection at 260 nm) of AA2G™, lidocaine, and IPA (coeluent) after autoclaving (3 yr equivalent at 25° C.).

FIG. 7 is a graph comparing antioxidant properties in compositions: control versus JUVEDERM® Ultra with lidocaine AA2G™, and JUVEDERM® Ultra with lidocaine.

DESCRIPTION

Our invention is based on the discovery that a steam sterilization stable HA based dermal filler can be prepared with an additional ingredient (that is besides the HA present in the formation) which is a wrinkle reduction, antioxidant, haemostatic, vasoconstriction, anti-itching, anti-inflammatory and/or anti-irritant ingredient. An HA dermal filler within the scope of our invention (“the dermal filler formulation”) is (autoclaving) steam sterilization stable and as demonstrated stability after about 32 days at about 45° C. The formulation does not exhibit any degradation as shown by the pre and post autoclaved formulations both being clear, homogenous, and cohesive.

The dermal filler formulation can also exhibit greater stability than an HA gel formulation without the additional constituent. Without wishing to be bound by theory it may be that the matrix of the cross-linked HA used in our formulation sequesters, renders non-reactive and thereby prevents the additional ingredient (as set forth for example in Examples 4-6, 10-11, 13, 15-16, 20, 24, and 25-29, supra) from degrading and causes degradation of the dermal filler formulation during steam sterilization. Additionally, the additional ingredient can be hydrophilic and provides protection to the HA from degradation during steam sterilization and/or after administration of the dermal filler formulation to a patient. Without wishing to be bound by theory, the incorporation of an additional ingredient in the dermal filler formulation may inhibit free-radical scavenging at the injection/implant site, thereby prolonging dermal filler duration after patient administration. After steam sterilization the additional ingredient can upon administration (as by subdermal injection) be released from the dermal filler formulation for cosmetic or therapeutic effect.

Autoclave stable or steam sterilization stable as used herein means a dermal filler formulation that is resistant to degradation such that the formulation retains at least one, and preferably all, of the following aspects after steam sterilization: transparent or clear appearance pH, extrusion force and/or rheological characteristics, hyaluronic acid (HA) concentration, osmolarity, and same additional ingredient concentration.

High molecular weight HA as used herein describes a HA material having a molecular weight of at least about 1.0 million Daltons (mw≥10⁶Da or 1 MDa) to about 4.0 MDa. For example, the high molecular weight HA in the present compositions may have a molecular weight of about 2.0 MDa. In another example, the high molecular weight HA may have a molecular weight of about 2.8 MDa.

Low molecular weight HA as used herein describes a HA material having a molecular weight of less than about 1.0 MDa. Low molecular weight HA can have a molecular weight of between about 200,000 Da (0.2 MDa) to less than about 1.0 MDa, for example, between about 300,000 Da (0.3 M Da) to about 750,000 Da. (0.75 MDa).

Degree of crosslinking as used herein refers to the intermolecular junctions joining the individual HA polymer molecules, or monomer chains, into a permanent structure, or as disclosed herein the soft tissue filler composition. Moreover, degree of crosslinking for purposes of the present disclosure is further defined as the percent weight ratio of the crosslinking agent to HA-monomeric units within the crosslinked portion of the HA based composition. It is measured by the weight ratio of HA monomers to crosslinker (HA monomers:crosslinker).

Free HA as used herein refers to individual HA polymer molecules that are not crosslinked to, or very lightly crosslinked to (very low degree of crosslinking) the highly crosslinked (higher degree of crosslinking) macromolecular structure making up the soft tissue filler composition. Free HA generally remains water soluble. Free HA can alternatively be defined as the “uncrosslinked,” or lightly crosslinked component of the macromolecular structure making up the soft tissue filler composition disclosed herein.

The presence of an additional ingredient in the dermal filler formulation can provide a stability and longevity that is not exhibited in a dermal filler formulation containing HA without the additional ingredient. The disclosed formulations after steam sterilization are homogenous, uncolored, clear, cohesive gel. Our invention includes methods for treating dermatological conditions, such as fine lines, wrinkles, fibroblast depletions, and/or scars afflicting a subject by administering to a patient an effective amount of the dermal filler formulation. The patient can be any mammal, preferably a human of any age, gender or race. Although typically a subject experiencing the signs of aging skin is an adult, subjects experiencing premature aging or other skin conditions suitable for treatment (for example, a scar) with the HA gel formulation can be treated as well.

Our dermal filler formulation comprise HA which is preferably at least partly cross-linked and can contain some not cross-linked HA. Although any pharmaceutically or cosmetically acceptable HA can be used in the disclosed compositions and formulations, in certain embodiments, the preferred HA utilized includes those sold as JUVEDERM®, JUVEDERM® 30, JUVEDERM® Ultra Plus, JUVEDERM® Ultra injectable gel (Allergan Inc, Irvine, Calif.). In certain embodiments, the formulation comprises a HA gel matrix and an additional constituent. HA is a known hydrogel. The gel can be injectable, bioresorbable, monophasic, or biphasic. In some embodiments, the additional constituent can be directly incorporated into the HA gel. In other embodiments, in order to increase affinity with the medium or increase stability, modification of the molecule by derivatization or encapsulation of the constituent can be performed, as described above. For instance, certain oily molecules cannot be introduced directly into a hydrophilic matrix, and lead to a heterogeneous product. Derivatization of the molecule by grafting hydrophilic moieties is required to increase homogeneity of the gel. In some embodiments, the gel composition can include a biocompatible or biodegradable vessel.

The HA gel can be made by any known, suitable methods. Cross-linked HA gels typically have high viscosity and require considerable force to extrude through a fine needle. Uncross-linked HA is often used as a lubricant to facilitate the extrusion process. However, especially in HA dermal fillers and implants, uncross-linked HA does not contribute to the persistence of the final product in vivo. The formulations exhibit increased stability compared to formulations containing HA without the additional constituent. Stability is determined by assessing the homogeneity, color, and clarity, pH, and rheological properties of the gel formulation. The formulations disclosed herein are considered stable if they remain homogenous, colorless, and/or clear, and exhibit stable pH and rheology. The disclosed formulations remain stable for at least about 6 months, at least about 1 year, at least about 2 years or at least about 3 years.

A cross-linking agent can be used to cross-link the HA according to the present disclosure. The cross-linking agent may be any agent known to be suitable for cross-linking HA and its derivatives via hydroxyl groups. Suitable cross-linking agents include but are not limited to, 1,4-butanediol diglycidyl ether, 1,4-bis(2,3-epoxypropoxy)butane, and/or 1,4-bisglycidyloxybutane (commonly known as BDDE), 1,2-bis(2,3-epoxypropoxy)ethylene, and 1-(2,3-epoxypropyl)-2,3-epoxycyclohexane. The use of more than one cross-linking agent or a different cross-linking agent is included from the scope of the present disclosure.

Dermal fillers can be used to treat moderate to severe facial wrinkles and folds such as nasolabial folds (those lines that extend from the nose to the corners of the mouth). In one embodiment, a dermal filler can be a gel implant formulation that includes HA and an additional constituent. The formulations disclosed herein can further include additional cosmetic agents that supplement and improve the appearance of skin. The cosmetic active ingredients may include, but are not limited to, antioxidants, vitamins, tension agents, and moisturizers.

The formulations disclosed herein can be injected with a syringe into the mid to deep dermis of the face. The dermis is the subsurface skin layer that contains connective tissue, nerve endings, and blood vessels. The formulations, when administered as dermal fillers can improve skin appearance by lifting and adding volume to the wrinkles and folds in the treatment area. Further, in certain embodiments, improvement can be seen due to increased collagen production that results from administration of the formulation.

As used herein, “cosmetic” is an adjective referring to improving the appearance of a surface or covering defects. Typically, cosmetic compositions can be used to improve aesthetic rather than functional aspects of a surface. Most commonly, cosmetic compositions are formulated for application as a health and beauty treatment or for affecting personal appearance of the body, for example, keratinous surfaces such as skin, hair, nails, and the like.

As used herein, “formulation” and “composition” may be used interchangeably and refer to a combination of elements that is presented together for a given purpose. Such terms are well known to those of ordinary skill in the art.

Examples of additional ingredients (agents) which can be included in the present dermal filler formulations are anti-itch, anti-cellulite, anti-scarring, and anti-inflammatory agents, anesthetics, anti-irritants, vasoconstrictors, vasodilators, as well as agents to prevent/stop bleeding, and improve/remove pigmentation, moisturizers, desquamating agents, tensioning agents, anti-acne agents. Anti-itch agents can include methyl sulphonyl methane, sodium bicarbonate, calamine, allantoin, kaolin, peppermint, tea tree oil, camphor, menthol, hydrocortisone and combinations thereof. Anti-cellulite agents can include forskolin, xanthine compounds such as, but not limited to, caffeine, theophylline, theobromine, and aminophylline, and combinations thereof. Anesthetic agents can include lidocaine, benzocaine, butamben, dibucaine, oxybuprocaine, pramoxine, proparacaine, proxymetacaine, tetracaine, and combinations thereof. Anti-scarring agents can include IFN-.gamma., fluorouracil, poly(lactic-co-glycolic acid), methylated polyethylene glycol, polylactic acid, polyethylene glycol and combinations thereof. Anti-inflammatory agents can include dexamethasone, prednisolone, corticosterone, budesonide, estrogen, sulfasalazine, mesalamine, cetirizine, diphenhydramine, antipyrine, methyl salicylate, loratadine, and derivatives and combinations thereof. Additionally, active agents such as epinephrine, thymidine, cytidine, uridine, antiypyrin, aminocaproic acid, tranexamic acid, eucalyptol, allantoin, glycerin, and sodium selenite, can be included. The disclosed dermal filler formulations can further comprise degradation inhibitors. Degradation inhibitors, include but are not limited to, glycosaminoglycans (e.g., heparin, heparin sulfate, dermatan sulfate, chondroitin sulfate, o-sulfated HA, linamarin, glucosamine, and amygdalin), antioxidants (e.g. ascorbic acid, melatonin, vitamin C, vitamin E, sodium selenite, glutathion, retinoic acid, coenzyme, beta-carotene, allopurinol, mannitol, caffeic acid, caffeine, polyphenol, theobromine, catechin), proteins (e.g., serum hyaluronidase inhibitor), and fatty acids (e.g. saturated C₁₀to C₂₂fatty acids), vitamin B and complex, and combinations thereof as noted, in certain embodiments, the additional ingredient can be an antioxidant. In certain embodiments, the antioxidant comprises a vitamin C such as ascorbyl-2-glucoside (available as AA2G™, Hayashibara Co., Japan) (FIG. 1), and/or a vitamin E such as d-alpha-tocopheryl polyethylene glycol 1000 succinate (TPGS). Anti-irritants can include thymol, bisabolol. Healing agents can include allantoin, eucalyptol, chitosane, cytidine, thimidine, uridine, lanoline. Anti-bleeding: epinephrine, norepinephrine, phenylephrine, synephrine, naphazoline, aminocaproic acid, tranexamic acid, ethamsylate, vitamin K. Collagen promoters can include retinol, peptide sequences. Additionally, active ingredients (agents) such as epinephrine, thymidine, cytidine, uridine, antipyrine, aminocaproic acid, eucalyptol, sodium selenite, can be included.

In some embodiments, the HA is present at a concentration of about 1 to about 40 mg/mL, or about 10 to about 40 mg/mL, or about 20 to about 30 mg/mL. In certain embodiments, the HA is present in a concentration of about 20 to about 25 mg/mL. In certain embodiments, the HA is present at a concentration of 24 mg/mL. The additional constituent can be present in an amount of about 0.001 to about 10% w/w, or from about 0.001 to about 5% w/w, or from 0.3 to about 3% w/w.

In certain embodiments, the disclosure provides a dermal filler comprising (a) about 90 wt %, or about 95 wt %, or about 100 wt % of a high molecular weight (about 1 million to about 3 million Daltons) HA; and (b) 0 wt %, or about 5 wt %, or about 10 wt % of a low molecular weight (less than 1 million Daltons) HA. In certain embodiments, the HA is present in the dermal filler at a concentration of about 10 to about 24 mg HA/mL dermal filler and the HA is about 4% to about 11% cross-linked. In certain embodiments, the cross linker is 4-butane diol diglycidyl ether (BDDE). The dermal filler can further comprise about 0.1 wt % or 0.6 wt %, or 1.0 wt % of an ascorbyl-2-glucoside, such as AA2G™ (Hayashibara, Japan). In a preferred embodiment, 0.6 wt % AA2G™ (i.e., 6 mg AA2G™/g HA) is utilized and renders a concentration of 2.1012 mM AA2G™.

Topical formulations of AA2G™ are known. However, there are no subdermally administered formulations of AA2G™ available, which is likely due to the fact that a topical AA2G™ is not thought to lend itself to an injectable formulation. The disclosure provides the first injectable formulation of AA2G™ that is efficacious, compatible, and stable over time.

The disclosed compositions are also well suited for mesotherapy. Mesotherapy is a non-surgical cosmetic treatment technique involving intra-epidermal, intra-dermal, and/or subcutaneous injection of an agent (micronutrients, vitamins, mineral salts, etc). The compositions are administered in the form of small multiple droplets into the epidermis, dermo-epidermal junction, and/or the dermis.

The formulations of the disclosure can be injected utilizing needles with a diameter of about 0.26 to about 0.4 mm and a length ranging from about 4 to about 14 mm. Alternately, the needles can be 21 to 32 G and have a length of about 4 mm to about 70 mm. Preferably, the needle is a single-use needle. The needle can be combined with a syringe, catheter, and/or a pistol (for example, a hydropneumatic-compression pistol).

The formulations can be administered once or over several sessions with the subject spaced apart by a few days, or weeks. For instance, the subject can be administered a formulation every 1, 2, 3, 4, 5, 6, 7, days or every 1, 2, 3, or 4, weeks. The administration can be on a monthly or bi-monthly basis. Further, the formulation can be administered every 3, 6, 9, or 12 months.

Our dermal filler formulation can optionally include one or more agents such as, without limitation, emulsifying agents, wetting agents, sweetening or flavoring agents, tonicity adjusters, preservatives, buffers antioxidants and flavonoids. Tonicity adjustors useful in a pharmaceutical composition of the present disclosure include, but are not limited to, salts such as sodium acetate, sodium chloride, potassium chloride, mannitol or glycerin and other pharmaceutically acceptable tonicity adjusters. Preservatives useful in the dermal filler formulation described herein include, without limitation, benzalkonium chloride, chlorobutanol, thimerosal, phenyl mercuric acetate, and phenyl mercuric nitrate. Various buffers and means for adjusting pH can be used to prepare the dermal filler formulation, including but not limited to, acetate buffers, citrate buffers, phosphate buffers and borate buffers. Similarly, antioxidants useful in the dermal filler formulation include for example, sodium metabisulfite, sodium thiosulfate, acetylcysteine, butylated hydroxyanisole and butylated hydroxytoluene. Flavonoids are compounds found in plants that are well known to have diverse beneficial biochemical and antioxidant effects. Subcategories of flavonoids include: flavones, flavonols, flavanones and flavanonols. Examples of flavonoids include: luteolin, apigenin, tangeritin, quercetin, kaempferol, myricetin, fisetin, isorhamnetin, pachypodol, rhamnazin, hesperetin, naringenin, eriodictyol, homoeriodictyol, taxifolin, dihydroquercetin, dihydrokaempferol, tannic acid, tannins, condensed tannins, and hydrolysable tannins. It is understood that these and other substances known in the art can be included in the dermal filler formulations disclosed herein. The pH of the disclosed dermal filler formulations can be about 5.0 to about 8.0, or about 6.5 to about 7.5. In certain embodiments, the pH of the formulation is about 7.0 to about 7.4 or about 7.1 to about 7.3.

A dermal filler formulation must be capable of withstanding sterilization which is a strict requirement before the product can be sold (the product must be sterile). Sterilization can be carried out by steam sterilization, filtration, microfiltration, gamma radiation, ETO light or by a combination of these methods. It is known that a dermal filler can be steam sterilized (autoclaved) without degradation of physical properties, but when a dermal filler formulation contains an additional labile ingredient (such as an anti-oxidant, wrinkle reduction, haemostatic, vasoconstriction, anti-itching, anti-inflammatory, and/or anti-irritant ingredient, such as a vitamin, vitamin derivative or analgesic compound) the entire dermal filler formulation or at least the additional (heat labile) ingredient is sterilized by a non-heat treatment such as by a filtration sterilization method. Thus, the known dermal filler product (“Revitacare”) is sold in two separate vials or containers, one vial containing the HA (which is autoclave sterilized)) and the second vial containing any additional ingredients (the second vial contents are sterilized by filtration). Another known dermal filler product NCTF®135 HA is sold in a single container holding both HA and any additional ingredients, all having been sterilized by microfiltration. It is an important aspect of our invention that we mix the HA and the additional ingredients and then autoclave the completed dermal filler formulation with maintenance of gel properties (i.e. non-degraded and storage stable formulation). Additionally we have discovered dermal filler formulations that exhibit retention of stability after being treated (accelerated heat test environment) to about 45° C. for about 30 days, or at least about 60 days, or at least about 90 days with no degradation of physical properties.

To reiterate an important aspect of our invention and a significant distinction over known dermal fillers is that our dermal filler formulations are prepared by: (1) mixing the HA and the additional ingredient(s), and then; (2) autoclaving (no filtration sterilization of any component) the complete dermal filler formulation with; (3) maintenance of the desired gel properties (no degradation of any dermal filler constituent or ingredient, and stable).

EXAMPLES

In the Examples below autoclaving means steam sterilization carried out at a temperature between about 130° C. to about 135° C. for between about one minute and about 10 minutes.

Example 1A
Method for Determining Gel Cohesivity

For purposes of example only and not to be considered as limiting the present invention in any way, the following tests may be performed in order to evidence or quantify cohesivity of a HA-based gel composition.

First, 0.2 g or 0.4 g of a gel composition to be tested is placed in a glass syringe. Next, 0.2 g or more of phosphate buffer is added to the syringe and the mixture is thoroughly mixed for about 1 hour to obtain a homogenous mixture. Then, the homogenized mixture is centrifuged for 5 min at 2000 tr/min to remove the air bubbles and to allow the decantation of any particles. The syringe is then held in a vertical position and one drop of eosin colorant is deposited at the surface of the gel by means of a syringe and an 18G needle. After 10 min, the dye has slowly diffused through the gel.

After dilution of the gel, homogenization and decantation, a relatively low cohesivity gel shows a phase separation (an upper diluted less viscous phase without particles and a lower one composed of decanted particles that are visible with the naked eye or under microscope). Under the same conditions, a highly cohesive gel shows substantially no phase separation, and the dye is prevented from diffusing into the cohesive formulation. A relatively less cohesive gel, on the other hand, shows a clear phase separation.

Example 1
Properties of Formulations of NaHA and Water Soluble Molecules are Tested

The active ingredient was incorporated into a NaHA matrix and autoclaved. The properties of the gel, aspect (i.e., color/clarity/homogeneity) and extrusion force were analyzed after sterilization at 3 years equivalent at room temperature. Table 1 shows that all formulations were clear, homogenous, and uncolored at the 3-year mark. The extrusion forces after autoclaving and at 3 years equivalent at room temperature are shown as well. In conclusion, the incorporation of the molecules has no impact on gel properties and ingredient structure.

TABLE 1

Extrusion
Extrusion

force
force

(N)
(N)

Content

after
3 years~room

Ingredient
(%)
Aspect
autoclaving
T ° C.

Allantoin
0.3
Clear
PASSED
PASSED

0.5
Homogeneous
PASSED
PASSED

Cytidine
0.5
Uncolored
PASSED
PASSED

1

PASSED
PASSED

Thymidine
0.5

PASSED
PASSED

1

PASSED
PASSED

Uridine
0.5

PASSED
PASSED

1

PASSED
PASSED

Antipyrin
0.5

PASSED
PASSED

1

PASSED
PASSED

Aminocaproic acid
0.5

PASSED
PASSED

1

PASSED
PASSED

Tranexamic acid
0.5

PASSED
PASSED

Eucalyptol
0.5

PASSED
PASSED

Sodium selenite
0.1

PASSED
PASSED

Glycerin
0.5

PASSED
PASSED

Acceptance criteria: “Passed” means that the change of extrusion force (ΔF) was less than two Newtons (<2 N). In other words the measured ΔF of the extrusion force of the HA gel with the specified ingredients minus the extrusion force of the HA gel without the added ingredients was <2 N.

Example 2
Preparation of NaHA Gel Containing Vitamin C

Ascorbic acid (1% w/w) was incorporated into a NaHA matrix. (JUVEDERM® FORMA). The pH was adjusted to about 7 and composition was autoclaved. The gel obtained was clear, yellow and degraded.

Example 3
Alternative Preparation of NAHA Gel Containing Vitamin C

Magnesium Ascorbyl Phosphate (MAP) (0.6%, 1 or 2% w/w) was incorporated in a NaHA matrix (JUVEDERM® Ultra). The pH was adjusted to about 7 and the compositions were autoclaved. All gels obtained were uncolored and clear. The gel properties after autoclaving are shown in Table 2. Extrusion force acceptance criteria: Conform with NaHA matrix specifications.

TABLE 2

After

autoclaving

Extrusion

force

Formulation
(N)

JUVEDERM ® Ultra + 0.6% MAP
PASSED

JUVEDERM ® Ultra + 1% MAP
PASSED

JUVEDERM ® Ultra + 2% MAP
PASSED

Rheology data of the gel containing 2% MAP after autoclaving is shown in Table 3. Rheological properties are followed as a function of time using a controlled stress rheometer according to the following method: frequency sweep from 0.05 to 10 Hz with 0.8% controlled strain. A degradation of the gel was observed by rheology. TAN δ×HZ is a rheological characterisation which shows the ratio of viscous modulus to elastic modulus. It shows the degradation of the gel.

Δ Tan δ1 Hz=(Tan δ1 Hz formulation)−(Tan δ1 Hz NaHA matrix)

Acceptance criterion: Δ Tan δ 1 Hz<0.1

TABLE 3

Δ Tan δ

Formulation
1 Hz

JUVEDERM ® Ultra + 2% MAP
0.344

Example 4
Alternative Preparation of NAHA Gel Containing Vitamin C

Sodium Ascorbyl Phosphate (SAP) (0.6%, 1% and 2% w/w) was incorporated in an NaHA matrix (JUVEDERM® Ultra). The pH was adjusted to about 7 and the composition was autoclaved. All gels obtained were uncolored and clear. The gel properties after autoclaving are shown in Table 4.

TABLE 4

After

autoclaving

Extrusion

force

Formulation
(N)

JUVEDERM ® Ultra + 0.6% SAP
PASSED

JUVEDERM ® Ultra + 1% SAP
PASSED

JUVEDERM ® Ultra + 2% SAP
PASSED

Rheology data of the gel containing 2% SAP after autoclaving is shown in Table 5. No degradation of the gel was observed by rheology.

TABLE 5

Formulation
Δ Tan δ 1 Hz

JUVEDERM ® Ultra + 2% SAP
0.089

Example 5
Alternative Preparation of NaHA Gel Containing Vitamin C

Ascorbic acid 2-Glucoside (AA2G™) at a concentration of 0.6%, 1% and 2% w/w was incorporated in an NaHA matrix (JUVEDERM® Ultra Plus). The pH was adjusted to about 7 and the composition was autoclaved. All gels obtained were uncolored and clear. The gel properties after autoclaving are shown in Table 6.

TABLE 6

After

autoclaving

Extrusion

force

Formulation
(N)

JUVEDERM ® Ultra Plus + 0.6% AA-2G
PASSED

JUVEDERM ® Ultra Plus + 1% AA-2G
PASSED

JUVEDERM ® Ultra Plus + 2% AA-2G
PASSED

The gels containing 0.6%, 1% and 2% were stable (pH, injection force) after autoclaving. Rheology data of the gels containing 0.6%, 1% and 2% w/w AA2G™ after autoclaving is shown in Table 7. No degradation of the gel was observed by rheology at each AA2G™ concentration.

TABLE 7

Formulation
Δ Tan δ 1 Hz

JUVEDERM ® Ultra Plus + 0.6% AA2G ™
−0.010

JUVEDERM ® Ultra Plus + 1% AA2G ™
−0.014

JUVEDERM ® Ultra Plus + 2% AA2G ™
−0.016

Rheological studies showed an slightly increase of the stability of the gel in the presence of the additive.

Example 6
Effect of Vitamin C on Aspect and Stability of the Gel

The shelf-life at 45° C. during 32 days was tested for the formulations prepared in example 5 and the NaHA matrix JUVEDERM® Ultra Plus. Rheology data of the gels containing 0.6%, 1% and 2% of AA2G™ are shown in Table 8.

TABLE 8

Formulation
Δ Tan δ 1 Hz

JUVEDERM ® Ultra Plus + 0.6% AA2G ™
−0.050

JUVEDERM ® Ultra Plus + 1% AA2G ™
−0.045

JUVEDERM ® Ultra Plus + 2% AA2G ™
−0.059

The gels containing ascorbyl glucoside maintained their properties after autoclaving and over a period of 32 days at 45° C. Surprising Rheological studies showed an increase of the stability of the gel in the presence of the additive.

Example 7
Preparation of NaHA Gel Containing Vitamin E

Tocopheryl Acetate (0.5% w/w) was incorporated into a NaHA matrix. (JUVEDERM® 30) and autoclaved. The gel obtained was unclear, white.

Example 8
Alternative Preparation of NaHA Gel Containing Vitamin E

Sodium Tocopheryl Phosphate (STP), at 0.4%, 1.2% w/w, was incorporated in a NaHA matrix (JUVEDERM® FORMA) and autoclaved. The gel obtained was not clear (white).

Example 9
Alternative Preparation of NaHA Gel Containing Vitamin E

Polyoxyethanyl-α-tocopheryl sebacate (0.7% w/w) was incorporated in a NaHA matrix (JUVEDERM® Ultra Plus) and autoclaved. The gel obtained was clear, but heterogenous.

Example 10
Alternative Preparation of NaHA Gel Containing Vitamin E

Tocopherol polyethylene glycol 1000 succinate (TPGS) was incorporated in varying concentrations (1%, 3.5% and 7% w/w) in a NAHA matrix (JUVEDERM® FORMA) and autoclaved. “JUVEDERM® FORMA” means the Juvederm formulation was used. All gels obtained were uncolored and clear. The gel properties after autoclaving are shown in Table 9.

TABLE 9

Extrusion

force

Formulation
(N)

JUVEDERM ® FORMA + 1% TPGS
PASSED

JUVEDERM ® FORMA + 3.5% TPGS
PASSED

JUVEDERM ® FORMA + 7% TPGS
PASSED

Rheology data of the gels containing 1%, 3.5% and 7% TPGS after autoclaving is shown in Table 10. No degradation of the gel was observed by rheology at each TPGS concentration.

TABLE 10

Formulation
Δ Tan δ 1 Hz

JUVEDERM ® FORMA + 1% TPGS
0.008

JUVEDERM ® FORMA + 3.5% TPGS
−0.007

JUVEDERM ® FORMA + 7% TPGS
−0.011

These rheological studies showed the stability of the dermal filler formulation with a particular additional ingredient.

Example 11
Stability of Formulations Containing Additional Ingredients

The stability of various formulations was tested. The ingredients shown in Table 11 were incorporated into a NaHA matrix, and autoclaved. The degradation of the formulations after autoclaving is shows in Table 11 and after 48 days at 45° C. in Table 12. The stability of extrusion force, pH, and degradation are shown over time in FIGS. 3, 4, and 5, respectively. HPLC analysis (C18 column; eluent: sodium phosphate buffer (pH 2.2), 2-propanol 10%, 0.7 ml/min; detection at 260 nm) confirmed the ingredients after autoclaving and 3-year shelf-life are shown in FIG. 6.

TABLE 11

Δ Tan δ 1 Hz

After
45° C.,

autoclaving
48 days

JUVEDERM ® Ultra Plus +
0.059
0.020

AA2G ™ 0.6% + Lidocaine 0.3%

JUVEDERM ® Ultra Plus +
0.016
0.007

AA2G ™ 0.6% + TPGS 1.5% +

lidocaine 0.3%

Example 12
AA2G™ Promotes Collagen Synthesis

Human skin fibroblasts were cultured in a 12 wells plate. At confluence, 100 μL of each compound (Juvederm® FORMA with 0.3% lidocaine, Juvederm® FORMA+AA2G™ 0.6%+Lidocaine 0.3% and Phosphate Buffer with 0.6% AA2G) was deposited in a culture insert (porosity of 0.4 μm), which was itself laid on the fibroblast monolayers. In parallel, a control without treatment was performed. Cultures were incubated for 72 hours and each experimental condition was conducted done in triplicate. At the end of incubation, cell viability was verified by microscopic observation and MTT reduction assay. Pro-collagen I secretion was measured using ELISA kit. The presence of 0.6% AA2G™ in a hyaluronic acid gel containing 0.3% lidocaine increased pro-collagen synthesis by a factor 3 (+292%), whereas JUVEDERM® gel with 0.3% lidocaïne showed an increase of 40% of the pro-collagen secretion (see FIG. 2).

Example 13
AA2G™ Protects NaHA from Oxidative Degradation

The effect of AA2G™ on NaHA oxidative degradation was studied. Oxidation testing was used as it allows testing of the resistance of a NaHA matrix to free radicals. Degradation by free radicals was simulated on a rheometer (Haake Rheostress 600) by addition of 1/7 ratio of H₂O₂30% on the surface of a spread gel measured with a controlled stress rheometer according to the following method: frequency of 1 Hz with 0.8% controlled strain, during 3600 s at 35° C. The time value is taken at 5 Pa/s.

Further, a comparison of antioxidant properties for JUVEDERM® Ultra with AA2G™ 0.6%/Lidocaine 0.3% formulation (15 800 s) versus NaHA matrix JUVEDERM® Ultra with Lidocaine (4 942 s) showed that the gel containing AA2G™ and lidocaine is more stable with respect to free radical activity (see FIG. 7). AA2G™ protected against oxidative degradation by a factor of 3.

Example 14
Implantation Study

A gel containing AA2G™ at 0.6% (=6 mg/g=2.10⁻²mM) was implanted in the deep dermis and subcutaneous tissues in rats. Histological evaluation at 1 week showed some mononuclear cells (lymphocytes and plasmocytes) around the implants in all implantation sites (test and control). They were also associated with macrophages. The gel containing AA2G™ appeared to be less inflammatory. The irritation index in test samples (AA2G™+NaHA) was 9.9 compared to 12.3 in controls (NaHA only). Table 12 shows the histological results at 1 week, 1 month, and 3 months. The irritation score of AA2G™ gel are (for each implantation time) lower than control (gel without AA2G™)

TABLE 12

NAHA + AA2G + Lido

Biocompatibility ISO 10993

Cytotoxicity
✓ (non cytotoxic)

Irritation
✓ (non irritant)

Sensitization
✓ (non sensitizing)

Implantation Test

1 week
✓ (no skin reaction)

3 weeks
✓ (no skin reaction)

3 months
✓ (no skin reaction)

Example 15
Incorporation of Dexpanthenol in NaHA Gel Formulations

Dexpanthenol was incorporated into a NaHA matrix JUVEDERM® Ultra Plus with Lidocaine (with 0.3% w/w lidocaine) with a content of 1 w/w. The gel was autoclaved. The gel obtained was clear and uncolored before and after autoclaving. The gel properties after autoclaving are shown in Table 13.

TABLE 13

After autoclaving

Extrusion

Formulation
force (N)
Δ Tan δ 1 Hz

JUVEDERM ®Ultra Plus with
PASSED
0.026

Lidocaine (0.3%) + Dexpanthenol 1%

Example 16
Effect of the Incorporation of Dexpanthenol in NAHA Gel Formulations

The shelf-life at 45° C. during 30 days was tested of the formulations prepared in example 15 and the NaHA matrix JUVEDERM® Ultra Plus XC. The gel was clear, uncolored. Rheology data of the gels containing dexpanthenol 1% w/w and lidocaine 0.3% w/w are shown in Table 14.

TABLE 14

After 30 days at 45° C.

Formulation
Δ Tan δ 1 Hz

JUVEDERM ®Ultra Plus with
−0.071

Lidocaine (0.3%) + Dexpanthenol 1%

Rheological studies showed an increase of the stability of the gel in the presence of the additive.

Example 17
Incorporation of Epinephrine in NaHA Gel Formulations

Epinephrine was incorporated into a NaHA matrix (JUVEDERM® Ultra Plus) with a 10 ppm epinephrine bitartrate. The gel was autoclaved. The gel obtained was clear and uncolored before and after autoclaving. The gel (dermal filler formulation) properties after autoclaving are shown in Table 15.

TABLE 15

After autoclaving

Extrusion

Formulation
force (N)
Δ Tan δ 1 Hz

JUVEDERM ® Ultra Plus +
PASSED
0.165

epinephrine bitartrate 10 ppm

Degradation of the gel was observed by rheological analysis.

Example 18
Incorporation of Epinephrine in NaHA Gel Formulations

Epinephrine was incorporated into a NaHA matrix (JUVEDERM® Ultra Plus) with 0.3% lidocaine and 10 ppm epinephrine bitartrate. The gel was autoclaved. The gel obtained was clear and colored after autoclaving. The gel properties after autoclaving are shown in Table 16.

TABLE 16

After autoclaving

Extrusion

Formulation
force (N)
Δ Tan δ 1 Hz

JUVEDERM ®Ultra Plus + Lidocaine
PASSED
0.092

0.3% + epinephrine bitartrate 10 ppm

A slight degradation of the gel was observed by rheological analysis.

Example 19
Effect of Additional Ingredient on the Stability of Gel Containing Epinephrine and Lidocaine

The shelf-life at 45° C. during 60 days was tested of the formulations prepared in Example 18 and the NaHA matrix JUVEDERM® Ultra Plus. The gel was clear, slightly colored. Rheology data of the gels containing epinephrine bitartrate (10 ppm), lidocaine (0.3% w/w) is shown in Table 17.

TABLE 17

After 60 days at 45° C.

Formulation
Δ Tan δ 1 Hz

JUVEDERM ®Ultra Plus + Lidocaine
0.185

0.3% + epinephrine bitartrate 10 ppm

After a stability of 60 days at 45° C., the gel containing epinephrine and lidocaine was unstable.

Example 20
Incorporation of Epinephrine in NaHA Gel Formulations Containing an Antioxidant

Epinephrine was incorporated into a NaHA matrix (JUVEDERM® Ultra Plus) with epinephrine bitartrate (10 ppm) and mannitol (0.9 or 4.5% w/w). The gels were autoclaved. The gel with 4.5% mannitol was clear and uncolored before and after autoclaving whereas with 0.9% mannitol was slightly colored. The gel properties after autoclaving is shown in Table 18.

TABLE 18

After autoclaving

Extrusion

Formulation
force (N)
Δ Tan δ 1 Hz

JUVEDERM ® Ultra Plus + epinephrine
PASSED
0.047

bitartrate 10 ppm + mannitol 0.9%

JUVEDERM ® Ultra Plus + epinephrine
PASSED
0.015

bitartrate 10 ppm + mannitol 4.5%

No degradation was observed for either of the dermal filler formulations tested.

Example 21
Effect of Additional Ingredient on the Stability of Gel Containing Epinephrine and an Antioxidant

The shelf-life at 45° C. during 60 days was tested of the formulations prepared in example 20 and the NaHA matrix JUVEDERM® Ultra Plus. The gels were clear, slightly colored. Rheology data of the gels containing epinephrine bitartrate (10 ppm) and mannitol (0.9 or 4.5% w/w) is shown in Table 19.

TABLE 19

After 60 days at 45° C.

Formulation
Δ Tan δ 1 Hz

JUVEDERM ® Ultra Plus + epinephrine
0.061

bitartrate 10 ppm + mannitol 0.9%

JUVEDERM ® Ultra Plus + epinephrine
0.006

bitartrate 10 ppm + mannitol 4.5%

After a stability of days at 45° C., both gels containing epinephrine, lidocaine and mannitol were stable. The composition containing 4.5% mannitol was more stable.

Example 22
Incorporation of Epinephrine in NaHA Gel Formulations Containing Lidocaine and Antioxidant

Epinephrine was incorporated into a NaHA matrix (JUVEDERM® Forma) with epinephrine bitartrate (20 ppm), lidocaine (0.3% w/w) and mannitol (4.5% w/w). The gel was autoclaved. The gel obtained was clear slightly colored after autoclaving. The gel properties after autoclaving are shown in Table 20.

TABLE 20

After autoclaving

Extrusion

Formulation
force (N)
Δ Tan δ 1 Hz

JUVEDERM ® Forma + Lidocaine
PASSED
0.026

0.3% + epinephrine bitartrate 20

ppm + mannitol 4.5%

No degradation was observed.

Example 23
Effect of Additional Ingredient on the Stability of Gel Containing Epinephrine, Lidocaine and an Antioxidant

The shelf-life at 45° C. during 60 days was tested of the formulations prepared in example 22 and the NaHA matrix JUVEDERM® Forma. The gel was clear, slightly colored. Rheology data of the gel containing epinephrine bitartrate (20 ppm), lidocaine (0.3% w/w) and mannitol (4.5% w/w) is shown in Table 21.

TABLE 21

After 60 days at 45° C.

Formulation
Δ Tan δ 1 Hz

JUVEDERM ® Forma + epinephrine
−0.030

bitartrate 20 ppm + mannitol 4.5%

The gel (dermal filler formulation) was stable after 60 days at 45° C.

Example 24
Incorporation of Synephrine in NaHA Gel Formulations Containing Lidocaine and Antioxidant

Synephrine was incorporated into a NaHA matrix Juvederm Ultra Plus with Lidocaine (with 0.3% w/w lidocaine) with a content of 100 ppm of synephrine. The gel was autoclaved. The gel obtained was clear and uncolored before and after autoclaving. The gel properties after autoclaving is shown in Table 22.

TABLE 22

After autoclaving

Extrusion

Formulation
force (N)
Δ Tan δ 1 Hz

JUVEDERM ®with lidocaine
PASSED
−0.006

(0.3%) + synephrine 100 ppm

Example 25
Effect of Additional Ingredient on the Stability of Gel Containing Synephrine and Lidocaine

The shelf-life at 45° C. during 60 days was tested of the formulations prepared in example 24 and the NaHA matrix JUVEDERM® Ultra Plus with Lidocaine. The gels was clear, uncolored. Rheology data of the gel containing synephrine 100 ppm and lidocaine 0.3% w/w is shown in Table 23.

TABLE 23

After 60 days at 45° C.

Formulation
Δ Tan δ 1 Hz

JUVEDERM ®Ultra Plus with lidocaine
−0.028

(0.3%) + synephrine 100 ppm

This rheological study showed maintenance of the stability of the gel (dermal filler formulation) in the presence of the particular additional ingredient (additive) shown.

Example 26
Incorporation of Phenylephrine in NaHA Gel Formulations Containing Lidocaine

Phenylephrine was incorporated into a matrix JUVEDERM® Ultra Plus with Lidocaine (with 0.3% w/w lidocaine) with a content of 100 ppm phenylephrine. The gel was autoclaved. The gel obtained was clear and uncolored before and after autoclaving. The gel properties after autoclaving are shown in Table 24.

TABLE 24

After autoclaving

Extrusion

Formulation
force (N)
Δ Tan δ 1 Hz

JUVEDERM ® Ultra Plus with Lidocaine
PASSED
−0.002

0.3% + Phenylephrine 100 ppm

Example 27
Effect of Additional Ingredient on the Stability of Gel Containing Phenylephrine and Lidocaine

The shelf-life at 45° C. during 60 days was tested of the formulations prepared in example 26 and the NaHA matrix JUVEDERM® Ultra Plus with Lidocaine. The gel was clear, uncolored. Rheology data of the gel containing phenylephrine 100 ppm and lidocaine 0.3% w/w are shown in Table 25.

TABLE 25

After 60 days at 45° C.

Formulation
Δ Tan δ 1 Hz

JUVEDERM ® Ultra Plus with Lidocaine
−0.017

(0.3%) + Phenylephrine 100 ppm

This rheological study showed maintenance of the stability of the gel (dermal filler formulation) in the presence of the particular additional ingredient (additive) shown.

Example 28
Incorporation of Naphazoline in NaHA Gel Formulations Containing Lidocaine and Antioxidant

Naphazoline was incorporated into a matrix Juvederm Ultra Plus with Lidocaine (with 0.3% w/w lidocaine) with a content of 100 ppm. The gel was autoclaved. The gel obtained was clear and uncolored before and after autoclaving. The gel properties after autoclaving are shown in Table 26.

TABLE 26

After autoclaving

Extrusion

Formulation
force (N)
Δ Tan δ 1 Hz

JUVEDERM ® Ultra Plus with Lidocaine
PASSED
−0.003

(0.3%) + Naphazoline 100 ppm

Example 29
Effect of Additional Ingredient on the Stability of Gel Containing Naphazoline and Lidocaine

The shelf-life at 45° C. over 60 days was tested of the formulations prepared in example 28 and the NaHA matrix JUVEDERM® Ultra Plus with Lidocaine. The gel was clear, uncolored. Rheology data of the gel containing naphazoline 100 ppm and lidocaine 0.3% w/w is shown in Table 27.

TABLE 27

After 60 days at 45° C.

Formulation
Δ Tan δ 1 Hz

JUVEDERM ® Ultra Plus with Lidocaine
−0.008

0.3% + Naphazoline 100 ppm

Example 30
Treatment Example

A woman, age 37, presents with fine lines around her eyes and deeper wrinkles on the sides of her mouth. She receives injections of a formulation of Example 10. She receives the injections in the fine lines and in the wrinkles once a week for 3 weeks and notices a visible improvement in the appearance of her skin.

Example 31
Alternate Treatment Example

A 59 year old man presents with wrinkles between his eyebrows and in the nasolabial folds. He receives injections of the dermal filler formulation of Example 11, every 3 months. A visible improvement in the wrinkles is seen.

Example 32
Alternate Treatment Example

A 35 year old woman presents with fine lines across her forehead. She receives injections of the dermal filler formulation of Example 15, once a week for two weeks, and notices an improvement in the appearance of the skin on her forehead.

Example 33
Alternate Treatment Example

A woman, age 44, presents with uneven texture on her right cheek resulting from a loss of collagen due to aging. She receives injections of the dermal formulation of Example 20 (using the 4.5% mannitol dermal filler formulation), in her cheek to build up the areas where the collagen has been lost. A visible improvement is seen in the texture of the skin on her cheek after 3 series of injections over a 2 week period of time.

Example 34
Alternate Treatment Example

A 35 year old man presents with a deep wrinkle across his chin and fine lines on the sides of his eyes. He receives the dermal filler formulation of Example 26 along the sides of his eyes. He receives 2 series of injections in his chin, spaced 1 week apart. The fine lines and wrinkle are visibly diminished after treatment.

Example 35
Alternate Treatment Example

A woman, age 62, presents with wrinkles across her forehead, on the sides of her eyes, in the nasolabial folds, and a scar on her chin. She receives injections of the dermal filler formulation of Example 29 each week for one month. After the injections, the appearance of the wrinkles and the scar is visibly diminished.

Our results above show that at least each of the two additional ingredients AA2G and dexpanthenol significantly increased the stability of the dermal filler formulation (HA gel), as shown by the dermal filler formulation having a Δ Tan δ 1 Hz<−0.05.

With regard to dexpanthenol: panthenol is the alcohol analog of pantothenic acid (vitamin B5), and is thus the provitamin of B5 which in vivo is oxidized to pantothenate. Panthenol is a highly viscous transparent liquid at room temperature, but salts of pantothenic acid (for example sodium pantothenate) are powders (typically white). Panthenol is soluble in water, alcohol and propylene glycol, soluble in ether and chloroform, and slightly soluble in glycerin. Panthenol has two D and L enantiomers with only the D enantiomer (D-panthenol, also called dexpanthenol) being biologically active, however both the D and L forms have moisturizing properties. For topical cosmetic use panthenol has been used in the D form and as a racemic mixture of D and L (DL-panthenol). Thus topical dexpanthenol cream (sold under the generic name “panthoderm”) is made by mixing with an emollient and has been used for relieving dry skin, preventing and treating sore nipples during breast-feeding, and promoting healing of burns and poorly-healing wounds.

Unless otherwise indicated, all numbers expressing quantities of ingredients, properties such as molecular weight, reaction conditions, and so forth used in the specification and claims are to be understood as being modified in all instances by the term “about.” Accordingly, unless indicated to the contrary, the numerical parameters set forth in the specification and attached claims are approximations that may vary depending upon the desired properties sought to be obtained by the present invention. At the very least, and not as an attempt to limit the application of the doctrine of equivalents to the scope of the claims, each numerical parameter should at least be construed in light of the number of reported significant digits and by applying ordinary rounding techniques. Notwithstanding that the numerical ranges and parameters setting forth the broad scope of the invention are approximations, the numerical values set forth in the specific examples are reported as precisely as possible. Any numerical value, however, inherently contains certain errors necessarily resulting from the standard deviation found in their respective testing measurements.

The terms “a,” “an,” “the” and similar referents used in the context of describing the invention (especially in the context of the following claims) are to be construed to cover both the singular and the plural, unless otherwise indicated herein or clearly contradicted by context. Recitation of ranges of values herein is merely intended to serve as a shorthand method of referring individually to each separate value falling within the range. Unless otherwise indicated herein, each individual value is incorporated into the specification as if it were individually recited herein. All methods described herein can be performed in any suitable order unless otherwise indicated herein or otherwise clearly contradicted by context. The use of any and all examples, or exemplary language (e.g., “such as”) provided herein is intended merely to better illuminate the invention and does not pose a limitation on the scope of the invention otherwise claimed. No language in the specification should be construed as indicating any non-claimed element essential to the practice of the invention.

Groupings of alternative elements or embodiments of the invention disclosed herein are not to be construed as limitations. Each group member may be referred to and claimed individually or in any combination with other members of the group or other elements found herein. It is anticipated that one or more members of a group may be included in, or deleted from, a group for reasons of convenience and/or patentability. When any such inclusion or deletion occurs, the specification is deemed to contain the group as modified thus fulfilling the written description of all Markush groups used in the appended claims.

Certain embodiments of this invention are described herein, including the best mode known to the inventors for carrying out the invention. Of course, variations on these described embodiments will become apparent to those of ordinary skill in the art upon reading the foregoing description. The inventor expects skilled artisans to employ such variations as appropriate, and the inventors intend for the invention to be practiced otherwise than specifically described herein. Accordingly, this invention includes all modifications and equivalents of the subject matter recited in the claims appended hereto as permitted by applicable law. Moreover, any combination of the above-described elements in all possible variations thereof is encompassed by the invention unless otherwise indicated herein or otherwise clearly contradicted by context.

Specific embodiments disclosed herein may be further limited in the claims using consisting of or consisting essentially of language. When used in the claims, whether as filed or added per amendment, the transition term “consisting of” excludes any element, step, or ingredient not specified in the claims. The transition term “consisting essentially of” limits the scope of a claim to the specified materials or steps and those that do not materially affect the basic and novel characteristic(s). Embodiments of the invention so claimed are inherently or expressly described and enabled herein. Furthermore, numerous references have been made to patents and printed publications throughout this specification. Each of the above-cited references and printed publications are individually incorporated herein by reference in their entirety.

In closing, it is to be understood that the embodiments of the invention disclosed herein are illustrative of the principles of the present invention. Other modifications that may be employed are within the scope of the invention. Thus, by way of example, but not of limitation, alternative configurations of the present invention may be utilized in accordance with the teachings herein. Accordingly, the present invention is not limited to that precisely as shown and described. Specific embodiments disclosed herein may be further limited in the claims using consisting of or consisting essentially of language. When used in the claims, whether as filed or added per amendment, the transition term “consisting of” excludes any element, step, or ingredient not specified in the claims. The transition term “consisting essentially of” limits the scope of a claim to the specified materials or steps and those that do not materially affect the basic and novel characteristic(s). Embodiments of the invention so claimed are inherently or expressly described and enabled herein.

Claims

1. A steam sterilization-stable dermal filler formulation comprising a crosslinked hyaluronic acid (HA), ascorbyl-2-glucoside and an anesthetic agent, wherein the hyaluronic acid is crosslinked with 1,4-butanediol diglycidyl ether, 1,4-bis(2,3-epoxypropoxy)butane, 1,4-bisglycidyloxybutane, 1,2-bis(2,3-epoxypropoxy)ethylene, or 1-(2,3-epoxypropyl)-2,3-epoxycyclohexane.
2. The dermal filler formulation of claim 1, wherein the anesthetic agent is lidocaine.
3. The dermal filler formulation of claim 2, wherein the lidocaine is present in an amount of about 0.001% to about 10% w/w.
4. The dermal filler formulation of claim 2, wherein the lidocaine is present in an amount of about 0.001% to about 5% w/w.
5. The dermal filler formulation of claim 2, wherein the lidocaine is present in an amount of about 0.3% to about 3% w/w.
6. The dermal filler formulation of claim 2, wherein the lidocaine is present in an amount of 0.3% w/w.
7. The dermal filler formulation of claim 1, wherein the crosslinked HA is present in an amount of about 1 mg/mL to about 40 mg/mL.
8. The dermal filler formulation of claim 7, wherein the crosslinked HA is present in an amount of about 10 mg/mL to about 40 mg/mL.
9. The dermal filler formulation of claim 7, wherein the crosslinked HA is present in an amount of about 20 mg/mL to about 30 mg/mL.
10. The dermal filler formulation of claim 7, wherein the crosslinked HA is present in an amount of about 20 mg/mL to about 25 mg/mL.
11. The dermal filler formulation of claim 1, wherein the ascorbyl-2-glucoside is present in an amount of about 0.001% w/w to about 10% w/w.
12. The dermal filler formulation of claim 11, wherein the ascorbyl-2-glucoside is present in an amount of about 0.1% w/w to about 3.0% w/w.
13. The dermal filler formulation of claim 11, wherein the ascorbyl-2-glucoside is present in an amount of 1% w/w.
14. The dermal filler formulation of claim 11, wherein the ascorbyl-2-glucoside is present in an amount of 2% w/w.
15. The dermal filler formulation of claim 11, wherein the ascorbyl-2-glucoside is present in an amount of 0.6% w/w.
16. The dermal filler formulation of claim 1, wherein the steam-sterilization stability of the dermal filler formulation is determined by subjecting the dermal filler formulation to a steam sterilization treatment at between about 120° C. and about 135° C. for between about 1 minute and about 5 minutes, with substantial retention after the treatment of one or more of the dermal filler characteristics of being clear, homogenous and cohesive.
17. The dermal filler formulation of claim 16, wherein the HA is crosslinked with 1,4-butanediol diglycidyl ether, and the anesthetic agent is lidocaine.
18. The dermal filler formulation of claim 17, wherein the crosslinked HA is present in an amount of about 10 mg/mL to about 40 mg/mL.
19. The dermal filler formulation of claim 18, wherein the ascorbyl-2-glucoside is present in an amount of about 0.1% w/w to about 3.0% w/w, and the lidocaine is present in an amount of about 0.3% to about 3% w/w.

CROSS REFERENCE

This application is a continuation of U.S. patent application Ser. No. 15/825,465 filed on Nov. 29, 2017, which is a continuation of Ser. No. 15/099,016 filed on Apr. 14, 2016, which granted as U.S. Pat. No. 9,855,367 on Jun. 2, 2018, which is a continuation of U.S. patent application Ser. No. 13/675,993 filed Nov. 13, 2012, which granted as U.S. Pat. No. 9,333,160 on May 10, 2016, which is a continuation of U.S. patent application Ser. No. 12/714,377 filed Feb. 26, 2010, which is abandoned, which is a continuation-in-part of U.S. patent application Ser. No. 12/687,048 filed Jan. 13, 2010, which is abandoned, the entire content of each of which is incorporated herein by reference.

US Referenced Citations (358)

Number	Name	Date	Kind
2128827	Killian	Aug 1938	A
3548056	Eigen et al.	Dec 1970	A
3763009	Suzuki et al.	Oct 1973	A
3949073	Daniels et al.	Apr 1976	A
4060081	Yannas et al.	Nov 1977	A
4140537	Luck et al.	Feb 1979	A
4233360	Luck et al.	Nov 1980	A
4273705	Kato	Jun 1981	A
4279812	Cioca	Jul 1981	A
4424208	Wallace et al.	Jan 1984	A
4501306	Chu et al.	Feb 1985	A
4582640	Smestad et al.	Apr 1986	A
4582865	Balazs et al.	Apr 1986	A
4605691	Balazs et al.	Aug 1986	A
4636524	Balazs et al.	Jan 1987	A
4642117	Nguyen et al.	Feb 1987	A
4657553	Taylor	Apr 1987	A
4713448	Balazs et al.	Dec 1987	A
4716154	Malson et al.	Dec 1987	A
4772419	Malson et al.	Sep 1988	A
4803075	Wallace et al.	Feb 1989	A
4886787	De Belder et al.	Dec 1989	A
4896787	Delamour et al.	Jan 1990	A
5009013	Wiklund	Apr 1991	A
5084563	Sakai et al.	Jan 1992	A
5087446	Suzuki et al.	Feb 1992	A
5091171	Yu et al.	Feb 1992	A
5137723	Yamamoto et al.	Aug 1992	A
5143724	Leshchiner et al.	Sep 1992	A
5246698	Leshchiner et al.	Sep 1993	A
5252722	Mandai et al.	Oct 1993	A
5272136	Mandai et al.	Dec 1993	A
5278059	Sugimoto et al.	Jan 1994	A
5314874	Miyata et al.	May 1994	A
5328955	Rhee et al.	Jul 1994	A
5338420	Aga et al.	Aug 1994	A
5356883	Kuo et al.	Oct 1994	A
5399351	Leshchiner et al.	Mar 1995	A
5407812	Sakai et al.	Apr 1995	A
5428024	Chu et al.	Jun 1995	A
5432161	Sakai et al.	Jul 1995	A
5468850	Mandai et al.	Nov 1995	A
5508391	Sakai et al.	Apr 1996	A
5531716	Luzio et al.	Jul 1996	A
5545587	Sugimoto et al.	Aug 1996	A
5565519	Rhee et al.	Oct 1996	A
5571503	Mausner	Nov 1996	A
5614587	Rhee et al.	Mar 1997	A
5616568	Pouyani et al.	Apr 1997	A
5616611	Yamamato et al.	Apr 1997	A
5616689	Shenoy et al.	Apr 1997	A
5630923	Aga et al.	May 1997	A
5633001	Agerup	May 1997	A
5643464	Rhee et al.	Jul 1997	A
5676964	Della Valle et al.	Oct 1997	A
5750141	Roberts	May 1998	A
5759532	Galin et al.	Jun 1998	A
5767149	Yamamoto et al.	Jun 1998	A
5823671	Mitchell et al.	Oct 1998	A
5824333	Scopelianos et al.	Oct 1998	A
5827529	Ono et al.	Oct 1998	A
5843907	Sakai et al.	Dec 1998	A
5880107	Buenter	Mar 1999	A
5886042	Yu et al.	Mar 1999	A
5935164	Iverson	Aug 1999	A
5972326	Galin et al.	Oct 1999	A
5972385	Liu et al.	Oct 1999	A
5980930	Fenton et al.	Nov 1999	A
6013679	Kuo et al.	Jan 2000	A
6066325	Wallace et al.	May 2000	A
6129761	Hubbell	Oct 2000	A
6224857	Romeo et al.	May 2001	B1
6248905	Fujinami et al.	Jun 2001	B1
6319260	Yamamoto	Nov 2001	B1
6335035	Drizen et al.	Jan 2002	B1
6372494	Naughton et al.	Apr 2002	B1
6383218	Sourdille et al.	May 2002	B1
6383219	Telandro et al.	May 2002	B1
6418934	Chin	Jul 2002	B1
6444647	Robinson et al.	Sep 2002	B1
6495148	Abbiati	Dec 2002	B1
6521223	Calias et al.	Feb 2003	B1
6544503	Vanderhoff et al.	Apr 2003	B1
6576446	Yamasaki et al.	Jun 2003	B2
6627620	Nielsen	Sep 2003	B1
6630486	Royer	Oct 2003	B1
6685963	Taupin et al.	Feb 2004	B1
6716251	Asius et al.	Apr 2004	B1
6734298	Barbucci et al.	May 2004	B1
6767924	Yu et al.	Jul 2004	B2
6767928	Murphy et al.	Jul 2004	B1
6852255	Yang et al.	Feb 2005	B2
6893466	Trieu	May 2005	B2
6903199	Moon et al.	Jun 2005	B2
6921819	Piron et al.	Jul 2005	B2
6924273	Pierce	Aug 2005	B2
6939562	Spiro et al.	Sep 2005	B2
6979440	Shefer et al.	Dec 2005	B2
6991652	Burg	Jan 2006	B2
7015198	Orentreich	Mar 2006	B1
7119062	Alvis et al.	Oct 2006	B1
7129209	Rhee	Oct 2006	B2
7166570	Hunter et al.	Jan 2007	B2
7192984	Berg et al.	Mar 2007	B2
7196180	Aeschlimann et al.	Mar 2007	B2
7314636	Caseres et al.	Jan 2008	B2
7316822	Binette	Jan 2008	B2
7491709	Carey	Feb 2009	B2
7741476	Lebreton	Jun 2010	B2
7767452	Kleinsek	Aug 2010	B2
7799767	Lamberti et al.	Sep 2010	B2
7812049	Shanler et al.	Oct 2010	B2
7875296	Binette	Jan 2011	B2
7902171	Reinmueller et al.	Mar 2011	B2
8052990	Hermitte et al.	Nov 2011	B2
8053423	Lamberti et al.	Nov 2011	B2
8114898	Shanler et al.	Feb 2012	B2
8124120	Sadozai et al.	Feb 2012	B2
8137702	Binette et al.	Mar 2012	B2
8153591	Masters et al.	Apr 2012	B2
8288347	Collette et al.	Oct 2012	B2
8318695	Stroumpoulis et al.	Nov 2012	B2
8338375	Schroeder et al.	Dec 2012	B2
8338388	Lebreton	Dec 2012	B2
8357795	Lebreton	Jan 2013	B2
8394782	Strompoulis	Mar 2013	B2
8394783	Strompoulis	Mar 2013	B2
8394784	Stroumpoulis et al.	Mar 2013	B2
8455465	Molliard	Jun 2013	B2
8512752	Crescenzi et al.	Aug 2013	B2
8513216	Strompoulis	Aug 2013	B2
8524213	Leshchiner et al.	Sep 2013	B2
8563532	Lebreton	Oct 2013	B2
8575129	Bellini	Nov 2013	B2
8586562	Lebreton	Nov 2013	B2
8853184	Strompoulis	Oct 2014	B2
8946192	Gousse et al.	Feb 2015	B2
9333160	Gousse	May 2016	B2
9655991	Gousse	May 2017	B2
9662422	Pollock et al.	May 2017	B2
9855367	Gousse	Jan 2018	B2
10220113	Gousse	Mar 2019	B2
10449268	Gousse	Oct 2019	B2
20010039336	Miller et al.	Nov 2001	A1
20020102311	Gustavsson et al.	Aug 2002	A1
20020160109	Yeo et al.	Oct 2002	A1
20030031638	Joshi et al.	Feb 2003	A1
20030093157	Casares et al.	May 2003	A1
20030119985	Sehl et al.	Jun 2003	A1
20030148995	Piron et al.	Aug 2003	A1
20040032056	Vang et al.	Feb 2004	A1
20040101959	Marko et al.	May 2004	A1
20040127698	Tsai et al.	Jul 2004	A1
20040127699	Zhao et al.	Jul 2004	A1
20040199241	Gravett et al.	Oct 2004	A1
20040265389	Yui et al.	Dec 2004	A1
20050013729	Brown-Skrobot	Jan 2005	A1
20050025755	Hedrick et al.	Feb 2005	A1
20050101582	Lyons et al.	May 2005	A1
20050136122	Sadozai et al.	Jun 2005	A1
20050142152	Leshchiner et al.	Jun 2005	A1
20050165079	Shanler	Jul 2005	A1
20050181007	Hunter et al.	Aug 2005	A1
20050186261	Avelar et al.	Aug 2005	A1
20050186673	Geistlich et al.	Aug 2005	A1
20050226936	Agerup	Oct 2005	A1
20050227936	McSwiggen et al.	Oct 2005	A1
20050240147	Makower	Oct 2005	A1
20050271729	Wang	Dec 2005	A1
20050276830	DeJovin et al.	Dec 2005	A1
20050281880	Wang	Dec 2005	A1
20050287180	Chen	Dec 2005	A1
20060029578	Hoemann et al.	Feb 2006	A1
20060040894	Hunter	Feb 2006	A1
20060095137	Chung et al.	May 2006	A1
20060105022	Yokokawa et al.	May 2006	A1
20060122147	Wohlrab	Jun 2006	A1
20060141049	Lyons	Jun 2006	A1
20060147483	Chaouk et al.	Jul 2006	A1
20060189516	Yang et al.	Aug 2006	A1
20060194758	Lebreton	Aug 2006	A1
20060246137	Hermitte et al.	Nov 2006	A1
20060247722	Maschino	Nov 2006	A1
20060257488	Hubbard	Nov 2006	A1
20060264515	Dejovin et al.	Nov 2006	A1
20060286769	Tsuchiya et al.	Dec 2006	A1
20070026070	Vonwiller et al.	Feb 2007	A1
20070036745	Leshchiner et al.	Feb 2007	A1
20070066816	Tsai et al.	Mar 2007	A1
20070077292	Pinsky	Apr 2007	A1
20070082070	Stookey	Apr 2007	A1
20070104692	Quijano et al.	May 2007	A1
20070104693	Quijano et al.	May 2007	A1
20070203095	Sadozai et al.	Aug 2007	A1
20070212385	David	Sep 2007	A1
20070224247	Chudzik et al.	Sep 2007	A1
20070224278	Lyons et al.	Sep 2007	A1
20070298005	Marie-Josee	Dec 2007	A1
20080044476	Lyons et al.	Feb 2008	A1
20080050335	Faour et al.	Feb 2008	A1
20080057091	Abdellaoui et al.	Mar 2008	A1
20080089918	Lebreton	Apr 2008	A1
20080188416	Bernstein	Aug 2008	A1
20080193538	Kitazono et al.	Aug 2008	A1
20080200430	Bitterman et al.	Aug 2008	A1
20080207794	Wright et al.	Aug 2008	A1
20080241252	Lyons et al.	Oct 2008	A1
20080268051	Hughes et al.	Oct 2008	A1
20080268547	Avent	Oct 2008	A1
20080274946	Giampapa	Nov 2008	A1
20080279806	Cho	Nov 2008	A1
20080293637	Schroeder et al.	Nov 2008	A1
20080300681	Rigotti et al.	Dec 2008	A1
20090017091	Daniloff et al.	Jan 2009	A1
20090018102	Moutet et al.	Jan 2009	A1
20090022808	Champion et al.	Jan 2009	A1
20090028817	Niklason et al.	Jan 2009	A1
20090036403	Stroumpoulis et al.	Feb 2009	A1
20090042834	Karageozian	Feb 2009	A1
20090054638	Shelby	Feb 2009	A1
20090060852	DeJovin et al.	Mar 2009	A1
20090093755	Schroeder et al.	Apr 2009	A1
20090098177	Werkmeister et al.	Apr 2009	A1
20090110671	Miyata et al.	Apr 2009	A1
20090110736	Boutros	Apr 2009	A1
20090123547	Hill et al.	May 2009	A1
20090124552	Hill et al.	May 2009	A1
20090130027	Shanler et al.	May 2009	A1
20090143331	Stroumpoulis et al.	Jun 2009	A1
20090143348	Tezel et al.	Jun 2009	A1
20090148527	Robinson et al.	Jun 2009	A1
20090155314	Tezel et al.	Jun 2009	A1
20090155362	Longin et al.	Jun 2009	A1
20090162415	Huang et al.	Jun 2009	A1
20090169615	Pinsky	Jul 2009	A1
20090181104	Rigotti et al.	Jul 2009	A1
20090192533	Dlugos	Jul 2009	A1
20090192541	Ortiz	Jul 2009	A1
20090222065	Dlugos	Sep 2009	A1
20090263447	Asius et al.	Oct 2009	A1
20090291986	Puppas et al.	Nov 2009	A1
20090297632	Waugh	Dec 2009	A1
20090317376	Zukowska et al.	Dec 2009	A1
20100004198	Stroumpoulis et al.	Jan 2010	A1
20100028437	Lebreton	Feb 2010	A1
20100035838	Heber et al.	Feb 2010	A1
20100041788	Voigts et al.	Feb 2010	A1
20100098764	Stroumpoulis et al.	Apr 2010	A1
20100098794	Armand	Apr 2010	A1
20100099623	Schroeder et al.	Apr 2010	A1
20100111919	Abuzaina et al.	May 2010	A1
20100130502	DeJovin et al.	May 2010	A1
20100136070	Dobak et al.	Jun 2010	A1
20100160948	Rigotti et al.	Jun 2010	A1
20100161052	Rigotti et al.	Jun 2010	A1
20100168780	Rigotti et al.	Jul 2010	A1
20100226982	Malessa	Sep 2010	A1
20100226988	Lebreton	Sep 2010	A1
20100227867	DeJovin	Sep 2010	A1
20100247651	Kestler	Sep 2010	A1
20100249924	Powell et al.	Sep 2010	A1
20100255068	Stroumpoulis et al.	Oct 2010	A1
20100291171	Crescenzi et al.	Nov 2010	A1
20100316683	Piron et al.	Dec 2010	A1
20110008406	Altman et al.	Jan 2011	A1
20110008436	Altman et al.	Jan 2011	A1
20110008437	Altman et al.	Jan 2011	A1
20110014263	Altman et al.	Jan 2011	A1
20110014287	Altman et al.	Jan 2011	A1
20110020409	Altman et al.	Jan 2011	A1
20110034684	Yokokawa et al.	Feb 2011	A1
20110052695	Jiang et al.	Mar 2011	A1
20110070281	Altman	Mar 2011	A1
20110077737	Stroumpoulis et al.	Mar 2011	A1
20110091726	Shibuya et al.	Apr 2011	A1
20110097381	Altman	Apr 2011	A1
20110104800	Kensy et al.	May 2011	A1
20110111031	Jiang et al.	May 2011	A1
20110118206	Lebreton	May 2011	A1
20110150823	Huang	Jun 2011	A1
20110150846	Van Epps	Jun 2011	A1
20110171286	Cecile et al.	Jul 2011	A1
20110171310	Gousse	Jul 2011	A1
20110171311	Gousse et al.	Jul 2011	A1
20110172180	Gousse et al.	Jul 2011	A1
20110183001	Rosson	Jul 2011	A1
20110183406	Kensy	Jul 2011	A1
20110189292	Lebreton	Aug 2011	A1
20110194945	Kensy et al.	Aug 2011	A1
20110201571	Gavard	Aug 2011	A1
20110224164	Lebreton	Sep 2011	A1
20110224216	Andres	Sep 2011	A1
20110229574	Guillen et al.	Sep 2011	A1
20110286945	DeJovin et al.	Nov 2011	A1
20110288096	Graeber et al.	Nov 2011	A1
20110295238	Kensy et al.	Dec 2011	A1
20120010146	Han et al.	Jan 2012	A1
20120034462	Stroumpoulis et al.	Feb 2012	A1
20120045420	Van Epps et al.	Feb 2012	A1
20120071437	Stroumpoulis et al.	Mar 2012	A1
20120076868	Lamberti et al.	Mar 2012	A1
20120095206	Chen	Apr 2012	A1
20120100217	Green	Apr 2012	A1
20120100611	Kensy et al.	Apr 2012	A1
20120135937	Bertholon et al.	May 2012	A1
20120156265	Binette et al.	Jun 2012	A1
20120164098	Schroeder et al.	Jun 2012	A1
20120164116	Van Epps	Jun 2012	A1
20120165935	Van Epps	Jun 2012	A1
20120171265	Altman et al.	Jul 2012	A1
20120172317	Altman et al.	Jul 2012	A1
20120172328	Lebreton	Jul 2012	A1
20120172985	Altman et al.	Jul 2012	A1
20120189589	Van Epps et al.	Jul 2012	A1
20120189590	Van Epps et al.	Jul 2012	A1
20120189591	Van Epps et al.	Jul 2012	A1
20120189699	Stroumpoulis et al.	Jul 2012	A1
20120189708	Van Epps et al.	Jul 2012	A1
20120190644	D'este	Jul 2012	A1
20120207837	Powell et al.	Aug 2012	A1
20120208890	Gousse et al.	Aug 2012	A1
20120209381	Powell et al.	Aug 2012	A1
20120213852	Van Epps et al.	Aug 2012	A1
20120213853	Van Epps et al.	Aug 2012	A1
20120219627	Van Epps et al.	Aug 2012	A1
20120225842	Gousse et al.	Sep 2012	A1
20120232030	Gousse et al.	Sep 2012	A1
20120263686	Van Epps et al.	Oct 2012	A1
20120265297	Altman et al.	Oct 2012	A1
20120269777	Van Epps et al.	Oct 2012	A1
20120283428	Lee et al.	Nov 2012	A1
20120295870	Lebreton	Nov 2012	A1
20130023658	Stroumpoulis et al.	Jan 2013	A1
20130041038	Lebreton	Feb 2013	A1
20130041039	Lebreton	Feb 2013	A1
20130072453	Gousse et al.	Mar 2013	A1
20130096081	Njikang	Apr 2013	A1
20130116188	Pollock et al.	May 2013	A1
20130116190	Pollock et al.	May 2013	A1
20130116411	Pollock et al.	May 2013	A1
20130123210	Liu	May 2013	A1
20130129835	Pollock et al.	May 2013	A1
20130131011	Lebreton	May 2013	A1
20130131655	Rigotti et al.	May 2013	A1
20130136780	Tezel et al.	May 2013	A1
20130203696	Liu	Aug 2013	A1
20130203856	Cho, II	Aug 2013	A1
20130209532	Stroumpoulis et al.	Aug 2013	A1
20130210760	Liu	Aug 2013	A1
20130237615	Meunier	Sep 2013	A1
20130244943	Yu et al.	Sep 2013	A1
20130244970	Lebreton	Sep 2013	A1
20130274222	Horne	Oct 2013	A1
20130287758	Tozzi	Oct 2013	A1
20140011990	Lebreton	Jan 2014	A1
20140227235	Kim et al.	Aug 2014	A1
20160113855	Njikang	Apr 2016	A1
20170273886	Gousse	Sep 2017	A1

Foreign Referenced Citations (131)

Number	Date	Country
0949965	Jun 1974	CA
2805008	Jan 2012	CA
2786968	Feb 2018	CA
102548590	Jul 2012	CN
0273823	Jul 1988	EP
0416250	Mar 1991	EP
0416846	Mar 1991	EP
0555898	Oct 1993	EP
0648229	Apr 1995	EP
1247522	Oct 2002	EP
1398131	Mar 2004	EP
1419792	May 2004	EP
1115433	Dec 2004	EP
1532991	May 2005	EP
1726299	Nov 2006	EP
1932530	Jun 2008	EP
2236523	Jun 2010	EP
2435045	Apr 2012	EP
2435083	Apr 2012	EP
2484387	Aug 2012	EP
2207424	Jun 2014	EP
2523701	Sep 2016	EP
2733427	Oct 1996	FR
2752843	Mar 1998	FR
2920000	Feb 2009	FR
2924615	Jun 2009	FR
650153711	Nov 1980	JP
2001192336	Jul 2001	JP
2002-080501	Mar 2002	JP
2006523731	Oct 2006	JP
2007502645	Feb 2007	JP
2007063177	Mar 2007	JP
2007525541	Sep 2007	JP
2010511454	Apr 2010	JP
2010202522	Sep 2010	JP
2012508217	Apr 2012	JP
20110138765	Dec 2011	KR
20130018518	Feb 2013	KR
1986000079	Jan 1986	WO
1986000912	Feb 1986	WO
1992000105	Jan 1992	WO
1992020349	Nov 1992	WO
1996033751	Oct 1993	WO
1994001468	Jan 1994	WO
1994002517	Mar 1994	WO
1996033709	Oct 1996	WO
1997004012	Jun 1997	WO
1998035639	Aug 1998	WO
1998035640	Aug 1998	WO
1999-049878	Oct 1999	WO
2000001428	Jan 2000	WO
WO 0008061	Feb 2000	WO
WO 0046252	Aug 2000	WO
2001079342	Oct 2001	WO
2002005753	Jan 2002	WO
2002006350	Jan 2002	WO
2002009792	Feb 2002	WO
2003007782	Jan 2003	WO
2002017713	Mar 2003	WO
2004020473	Mar 2004	WO
2004022603	Mar 2004	WO
WO 2004067575	Aug 2004	WO
2004073759	Sep 2004	WO
2004092223	Oct 2004	WO
2005040224	Jun 2005	WO
WO 2005052035	Jun 2005	WO
2005067994	Jul 2005	WO
2005074913	Aug 2005	WO
2005112888	Dec 2005	WO
WO 2006015490	Feb 2006	WO
2006-031555	Mar 2006	WO
2006023645	Mar 2006	WO
WO 2006021644	Mar 2006	WO
WO 2006048671	May 2006	WO
2006067608	Jun 2006	WO
WO 2006056204	Jun 2006	WO
2006-102626	Sep 2006	WO
2007018124	Feb 2007	WO
2007070617	Jun 2007	WO
2007077399	Jul 2007	WO
2007128923	Nov 2007	WO
2007136738	Nov 2007	WO
2008-015249	Feb 2008	WO
2008034176	Mar 2008	WO
WO2008031525	Mar 2008	WO
WO 2008063569	May 2008	WO
2008068297	Jun 2008	WO
2008072230	Jun 2008	WO
2008077172	Jul 2008	WO
2008-098019	Aug 2008	WO
2008098019	Aug 2008	WO
2008139122	Nov 2008	WO
2008148967	Dec 2008	WO
2008157608	Dec 2008	WO
WO 2008148071	Dec 2008	WO
WO 2009003135	Dec 2008	WO
2009-005790	Jan 2009	WO
2009024719	Feb 2009	WO
2009026158	Feb 2009	WO
WO 2009024350	Feb 2009	WO
2009028764	Mar 2009	WO
2009034559	Mar 2009	WO
2009073437	Jun 2009	WO
2009082354	Jul 2009	WO
2010003797	Jan 2010	WO
WO 2010003104	Jan 2010	WO
2010-015901	Feb 2010	WO
2010015900	Feb 2010	WO
2010027471	Mar 2010	WO
2010028025	Mar 2010	WO
2010029344	Mar 2010	WO
WO 2010026299	Mar 2010	WO
2010038771	Apr 2010	WO
2010051641	May 2010	WO
2010052430	May 2010	WO
2010053918	May 2010	WO
2010061005	Jun 2010	WO
2010-136585	Dec 2010	WO
2010-136594	Dec 2010	WO
WO 2011023355	Mar 2011	WO
WO 2011072399	Jun 2011	WO
2011-086458	Jul 2011	WO
WO 2011135150	Nov 2011	WO
WO 2012008722	Jan 2012	WO
WO 2012077055	Jun 2012	WO
2012-104419	Aug 2012	WO
2012-113529	Aug 2012	WO
WO 2013015579	Jan 2013	WO
WO 2013036568	Mar 2013	WO
WO 2013067293	May 2013	WO
WO 2013086024	Jun 2013	WO

Non-Patent Literature Citations (140)

Entry
Adams, Mark, An Analysis of Clinical Studies of the Use of Crosslinked Hyaluronan, Hylan, in the Treatment of Osteoarthritis, The Journal of Rheumatology, 1993, 16-18, 20 (39).
Aesthetic Buyers Guide, Juvederm Raises Standards, 2007, 1, 4-7; www.miinews.com.
Albano, Emanuele et al., Hydroxyethyl Radicals in Ethanol Hepatotoxicity, Frontiers in Bioscience, 1999, 533-540, 4.
Allemann, Inja Bogdan, Hyaluronic Acid Gel (Juvederm) Preparations in the Treatment of Facial Wrinkles and Folds, Clinical Interventions in Aging, 2008, 629-634, 3 (4).
American Society for Aesthetic Plastic Surgery, http://www.surgery.org/media/news-release/115-million-cosmetic-procedures-in-2006; Mar. 9, 2007.
Anatelli, Florencia et al, Amorphous Basophilic Deposit in the Superficial Dermis of the Lip in an 80 Year Old, Am J Dermatophathol, 2010, 306-309, 32(3).
Antunes, et al., Efficacy of Intrarectal Lidocaine Hydrochloride Gel for Pain Control in Patients Undergoing Transrectal Prostate Biopsy, International Brazilian Journal of Urology, Sep./Oct. 2004, 380-383, vol. 30, Issue 5, Brazilian Society of Urology.
Atanassoff, et al., The Effect of Intradermal Administration of Lidocaine and Morphine on the Response to Thermal Stimulation, Anesthesia and Analgesia, 1997, 1340-1343, vol. 84, Issue 6.
Basran, G.S. et al, Adrenoceptor-Agonist Inhibition of the Histamine-Induced Cutaneuos Response in Man, British Journal of Dermatology, 1982, 140-142, 107.
Baumann, et al., Comparison of Smooth-Gel Hyaluronic Acid Dermal Fillers with Cross-linked Bovine Collagen: A Multicenter, Double-Masked, Randomized, Within-Subject Study, Dermatologic Surgery, Dec. 2007, S128-S135, vol. 33, Suppl. 2, American Society of Dermatologic Surgery, Inc.
Beasley, Karen et al., Hyaluronic Acid Fillers: A Comprehensive Review, Facial Plastic Surgery, 2009, 86-94, 25 (2), Thieme Medical Publishers, Inc.
Beasley, Karen et al., Soft Tissue Augmentation Using a Two-Way Connector to Supplement Hyaluronic Acid Filler with 1% Lidocaine Hydrochloric Acid With Epinephrine 1:100000: Our Experience and Observations, Dermatol Surg, 2008, 524-526, 35.
Beer, Dermal Fillers and Combinations of Fillers for Facial Rejuvenation, Dermatologic Clinics, 2009, 427-432, 27 (4).
Belda, Jose et al., Hyaluronic Acid Combined With Mannitol to Improve Protection Against Free-Radical Endothelial Damage: Experimental Model, Journal of Cataract Refract Surg, 2005, 1213-1218, 31, Elsevier Inc.
Bircher, Andres et al., Delayed-type Hypersensitivity to Subcutaneous Lidocaine With Tolerance to Articaine: Confirmation by In Vivo and In Vitro Tests, Contact Dermatitis, 1996, 387-389, 34, Blackwell Publishing Ltd., Denmark.
Bluel, K. et al., Evaluation of Reconstituted Collagen Tape as a Model for Chemically Modified Soft Tissues, Biomat. Med. Dev. Art. Org., 1981, 37-46, 9 (1), Marcel Dekker, Inc.
Buck, Donald, Injectable Fillers For Facial Rejuvenation: A Review, Journal of Plastic, Reconstructive & Aesthetic Surgery, 2009, 11-18, 62, Elsevier.
Busso, Mariano et al, An Investigation of Changes in Physical Properties of Injectable Calcium Hydroxylapatite in a Carrier Gel When Mixed with Lidocaine and with Lidocaine/Epinephrine, Dermatol Surg, 2008, S16-S24, 34.
Capozzi, Angelo et al., Distant Migration of Silicone Gel From a Ruptured Breast Implant, Silicone Gel Migration, 1978, 302-3, 62 (2).
Carlin, G. et al., Effect of Anti-Inflammatory Drugs on Xanthine Oxidase and Xanthine Oxidase Induced Depolymerization of Hyaluronic Acid, Agents and Actions, 1985, 377-384, 16 (5), Birkhauser Verlag, Basel.
Carruthers, Alastair et al, Botulinum Toxin Type A: History and Current Cosmetic Use in the Upper Face, Semin Cutan Med Surg, 2001, 71-84, 20(2).
Carruthers, et al., The Science and Art of Dermal Fillers for Soft-Tissue Augmentation, Journal of Drugs in Dermatology, Apr. 2009, 335-350, vol. 8, Issue 4.
Carruthers, Jean et al, Volumizing the Glabella and Forehead, Dermatol Surg, 2010, 1905-1909, 36.
Cassidy, James et al, Epinephrine: Systemic Effects and Varying Concentrations in Local Anesthesia, Anesth Prog, 1986, 289-297, 33(6).
Champion, et al., Role of Target Geometry in Phagocytosis, Proc. National Academy of Sciences, 2006, 4930-4934, 103 (13), The National Academy of Sciences of the USA.
Chemical Abstract Registry, RN 220644-17-7, RN 39479-63-5, 1 Page, 2016.
Chin, et al., Allergic Hypersensitivity to Lidocaine Hydrochloride, International Journal of Dermatology, 1980, 147-148, vol. 19, International Society of Topical Dermatology, Inc.
Chvapil, Milos, Collagen Sponge: Theory and Practice of Medical Applications, J. Biomed. Mater. Res., 1977, 721-741, 11, John Wiley & Sons, Inc.
Clark, et al., The Influence of Triamcinolone Acetonide on Joint Stiffness in the Rat, The Journal of Bone and Joint Surgery, Oct. 1971, 1409-1414, 53A (7).
Cohen, Miriam et al., Organization and Adhesive Properties of the Hyaluronan Pericellular Coat of Chondrocytes and Epithelial Cells, Biophysical Journal, Sep. 2003, 1996-2005, 85, Biophysical Society.
Cui, Yu et al., The Comparison of Physicochemical Properties of Four Cross-linked Sodium Hyaluronate Gels With Different Cross-linking Agents, Advanced Materials Research, 2012, 1506-1512, 396-398.
Deland, Frank, Intrathecal Toxicity Studies with Benzyl Alcohol, Toxicology and Applied Pharmacology, 1973, 153-6, 25, Academic Press, Inc.
Desai, et al., Molecular Weight of Heparin Using 13C Nuclear Magnetic Resonance Spectroscopy, Journal of Pharm Sci., Feb. 1995, 212-215, 84 (2).
Egbert, L.D. et al, Reduction of Bleeding by the Addition of Vasoconstrictor Drugs to Local Anesthetics, Annals of Surgery, 1962, 20-24, 155.
Eyre, et al., Collagen Cross-Links, Top Curr Chem, 2005, 207-229, 247, Springer-Verlag, Berlin Heidelberg.
Fagien, Steven, Variable Reconstitution of Injectable Hyaluronic Acid With Local Anesthetic for Expanded Applications in Facial Aesthetic Enhancement, Dermatol Surg, 2010, 815-821, 36.
Falcone, et al., Crosslinked Hyaluronic Acid Dermal Fillers: A Comparison of Rheological Properties, Journal of Biomedical Materials Research, 2008, 264-271, 87 (1), Wiley InterScience.
Falcone, Samuel et al., Temporary Polysaccharide Dermal Fillers: A Model for Persistence Based on Physical Properties, Dermatologic Surgery, 2009, 1238-1243, 35 (8).
Farley, et al., Diluting Lidocaine and Mepivacaine in Balanced Salt Solution Reduces the Pain of Intradermal Injection, Regional Anesthesia, 1994, 48-51, 19 (1).
Folwaczny, C. et al, Influence of Prophylactic Local Administration of Epinephrine on Bleeding Complications After Polypectomy, Endoscopy, 1996, 31-33, 28.
Frati, Elena et al., Degradation of Hyaluronic Acid by Photosensitized Riboflavin In Vitro. Modulation of the Effect by Transition Metals, Radical Quenchers, and Metal Chelators, Free Radical Biology Medicine, 1996, 1139-1144, 22 (7).
Fujinaga, Masahiko et al., Reproductive and Teratogenic Effects of Lidocaine in Sprague-Dawley Rats, Anesthesiology, 1986, 626-632, 65.
Fukuda, et al., English machine translation of JP 2007-063177 A, Mar. 15, 2007, translated Feb. 9, 2012 JST, pp. 1-10.
Funt, David, Avoiding Malar Edema During Midface/Check Augmentation with Dermal Fillers, J Clin Aesthet Dermatol, Dec. 2011, 32-36, 4(12).
Gammaitoni, et al., Pharmacokinetics and Safety of Continuously Applied Lidocaine Patches 5%, Am J Health Syst Pharm, 2002, 2215-2220, 59.
Gassner, Holger et al, Addition of an Anesthetic Agent to Enhance the Predictability of the Effects of Botulinum Toxin Type A Injections: A Randomized Controlled Study, Mayo Clin Proc, 2000, 701-704, 75(7).
Ginshicel MH, Hydroxy Propyl Methyl Cellulose, Retrieved on Nov. 12, 2008 http://www.ginshicel.cn/MHPC.html, 2007, p. 1-3, 2 (3).
Gold, Use of Hyaluronic Acid Fillers for the Treatment of the Aging Face, Clinical Interventions in Aging, 2007, 369-376, 2 (3), Dove Medical Press Limited.
Goldberg, David, Breakthroughs in US dermal fillers for facial soft-tissue augmentation, Journal of Cosmetic and Laser Therapy, 2009, 240-247, 11, Informa UK Ltd.
Graefe, et al., Sensitive and Specific Photometric Determination of Mannitol, Clinical Chemistry and Laboratory Medicine, 2003, 1049-1055, 41 (8), Walter de Gruyter.
Grecomoro, G. et al., Intra-articular treatment with sodium hyaluronate in gonarthrosis: a controlled clinical trial versus placebo, Pharmatherapeutica, 1987, 137-141, 5 (2).
Grillo, Hermes et al., Thermal Reconstitution of Collagen From Solution and the Response to Its Heterologous Implantation, JSR, 1962, 69-82, 2 (1).
Hantash, Basil et al, A Pilot Study on the Effect of Epinephrine on Botulinum Toxin Treatment for Periorbital Rhytides, Dermatologic Surgery, 2007, 461-468, 33.
Hassan, HG et al., Effects of Adjuvants to Local Anaesthetics on Their Duration. III. Experimental Studies of Hyaluronic Acid, Acta Anaesthesiol Scand., 1985, 1, 29 (4).
Hayashibara, AA2G, Sep. 23, 2007, Retrieved on Jan. 17, 2012, http://web.archive.org/web/20070923072010/http://www.hayashibara-intl.com/cosmetics/aa2g.html.
Helary, Christophe et al., Concentrated Collagen Hydrogels as Dermal Substitutes, Biomaterials, 2010, 481-490, 31.
Helliwell, Philip, Use of an objective measure of articular stiffness to record changes in finger joints after intra-articular injection of corticosteroid, Annals of Rheumatic Diseases, 1997, 71-73, 56.
Hertzberger-Ten, Cate et al., Intra-articular steroids in pauciarticular juvenile chronic arthritis, type 1, European Journal of Pediatrics, 1991, 170-172, 150.
Hetherington, NJ et al., Potential for Patient Harm from Intrathecal Administration of Preserved Solutions, Med J Aust., 2000, 1, 173(3).
Hong, Samin et al, Effect of Prophylactic Brimonidine Instillation on Bleeding During Strabismus Surgery in Adults, Am J Ophthalmol, 2007, 469-470, 144.
Hurst, E., Adhesive Arachnoiditis and Vascular Blockage Caused by Detergents and Other Chemical Irritants: An Experimental Study, J Path. Bact., 1955, 167, 70.
Intramed (Pty) Ltd, Intramed Mannitol 20% m/v Infusion, Package Insert, Jan. 1979, 4 pages, 12-214/8-94, ZA.
Jones, Adrian et al, Intra-articular Hyaluronic Acid Compared to Intra-articular Triamcinolone Hexacetonide in Inflammatory Knee Osteoarthritis, Osteoarthritis and Cartilage, 1995, 269-273, 3.
Jones, Derek, Semipermanent and Permanent Injectable Fillers, Dermatol Clin, 2009, 433-444, 27.
Kablik, et al., Comparative Physical Properties of Hyaluronic Acid Dermal Fillers, Dermatology Surgery, 2009, 302-312, 35, Wiley Periodicals, Inc.
Klein, A., Skin Filling Collagen and Other Injectables of the Skin, Fundamentals of Cosmetic Surgery, 2001, 491-508, 3 (19).
Kopp, et al., The Short-term Effect of Intra-articular Injections of Sodium Hyaluronate and Corticosteroid on Temporomandibular Joint Pain and Dysfunction, Journal of Oral and Maxillofacial Surgery, 1985, 429-435, 43.
Kulicke, Werner-Michael et al., Visco-Elastic Properties of Sodium Hyaluronate Solutions, Institute for Technical and Macromolecular Chemistry, 2008, 585-587, DE.
Laeschke, Klaus, Biocompatibility of Microparticles Into Soft Tissue Fillers, Semin Cutan Med Surg, 2004, 214-217, 23.
Lamar, PD et al., Antifibrosis Effect of Novel Gels in Anterior Ciliary Sclerotomy (ACS), 2002, 1 Page, The Association for Research in Vision and Ophthalmology, Inc.
Levy, Jaime et al., Lidocaine Hypersensitivity After Subconjunctival Injection, Can J Ophthalmol, 2006, 204-206, 41.
Lindgren, Bjorn et al, Inhibitory Effects of Clonidine on Allergic Reactions in Guinea-Pig Skin, European Journal of Pharmacology, 1987, 339-343, 134.
Lindvall, Sven et al., Influence of Various Compounds on the Degradation of Hyaluronic Acid by a Myeloperoxidase System, Chemico-Biological Interactions, 1994, 1-12, 90.
Lundeberg, T. et al, Epinephrine Reduces the Severity of Catheter-Induced Urethral Inflammation By Action at the α2-Adrenoceptors, British Journal of Urology, 1993, 349-352, 72.
Lupo, Mary, Hyaluronic Acid Fillers in Facial Rejuvenation, Seminars in Cutaneous Medicine and Surgery, 2006, 122-126, 25.
Mackley, Christine et al., Delayed-Type Hypersensitivity to Lidocaine, Arch Dermatol, 2003, 343-346, 139.
Mancinelli, Laviero et al., Intramuscular High-dose Triamcinolone Acetonide in the Treatment of Severe Chronic Asthma, West J Med, 1997, 322-329, 167 (5).
Maniglia-Ferreira, Claudlo et al, Clinical Evaluation of the Use of Three Anesthetics in Endodontics, Acta Odontol Latinoam, 2009, 21-26, 22(1).
Martin, Donna et al, Fine Rhytides Treated with Porcine Collagen-Derived Filler Mixed with Anesthetic, Dermatol Surg, 2010, 270-272, 36(2).
Matsumoto, Alan et al., Reducing the Discomfort of Lidocaine Administration Through pH Buffering, Journal of Vascular and Interventional Radiology, 1994, 171-175, 5 (1).
McCarty, Daniel et al., Inflammatory Reaction after Intrasynovial Injection of Microcrystalline Adrenocorticosteroid Esters, Arthritis and Rheumatism, 1964, 359-367, 7 (4).
McCleland, Marcee et al., Evaluation of Artecoll Polymethylmethacrylate Implant for Soft-Tissue Augmentation: Biocompatibility and Chemical Characterization, Plastic & Reconstructive Surgery, 1997, 1466-1474, 100 (6).
McCracken, Hyaluronic Acid Gel (Restylane) Filler for Facial Rhytids: Lessons Learned From American Society of Ophthalmic Plastic and Reconstructive Surgery Member Treatment of 286 Patients, Ophthalmic Plastic and Reconstructive Surgery, 2006, 188-191, 22 (3).
McPherson, John et al., Development and Biochemical Characterization of Injectable Collagen, Journal of Dermatol Surg Oncol, 1988, 13-20, 14 (Suppl 1) 7.
Menon, Harikumar et al, Low Dose of Hyaluronidase to Treat Over Correction by HA Filler—A Case Report, Journal of Plastic, Reconstructive & Aesthetic Surgery, 2010, e416-e417, 63.
Millay, Donna et al., Vasoconstrictors in Facial Plastic Surgery, Arch Otolaryngol Head Neck Surg., 1991, 160-163, 117.
Naoum, Christos et al, Dermal Filler Materials and Botulin Toxin, International Journal of Dermatology, 2001, 609-621, 40.
Orvisky, E. et al., High-molecular-weight Hyaluronan—a Valuable Tool in Testing the Antioxidative Activity of Amphiphilic Drugs Stobadine and Vinpocetine, Journal of Pharm. Biomed. Anal., 1997, 419-424, 16.
Osmitrol (generic name Mannitol), Official FDA Information, side effects and uses, http://www.drugs.com/pro/osmitrol.html, 2010, 10 Pages.
Palmon, Sally et al, The Effect of Needle Gauge and Lidocaine pH on Pain During Intradermal Injection, Anesth Analg, 1998, 379-381, 86.
Park, et al., Biological Characterization of EDC-Crosslinked Collagen-Hyaluronic Acid Matrix in Dermal Tissue Restoration, Biomaterials, 2003, 1631-1641, 24, Elsevier.
Park, et al., Characterization of Porous Collagen/Hyaluronic Acid Scaffold Modified by 1-Ethyl-3-(3-Dimethylaminopropyl) Carbodiimide Cross-Linking, Biomaterials, 2002, 1205-1212, 23, Elsevier.
Phenylephrine. Open Drug Data and Drug Target Database 2013; http://www.drugbank.ca/drugsIDB00388. Accessed May 6, 2013.
Powell, Michael, Stability of Lidocaine in Aqueous Solution: Effect of Temperature, pH, Buffer, and Metal Ions on Amide Hydrolysis, Pharmaceutical Research, 1987, 42-45, 4 (1).
Prestwich, Glenn, Evaluating Drug Efficacy and Toxicology in Three Dimensions: Using Synthetic Extracellular Matrices in Drug Discovery, Accounts of Chemical Research, Jan. 2008, 139-148, 41(1).
Rehakova, Milena et al., Properties of Collagen and Hyaluronic Acid Composite Materials and Their Modification By Chemical Crosslinking, Journal of Biomedical Materials Research, 1996, 369-372, 30, US.
Remington's Pharmaceutical Sciences, 1980, 16th Edition, Mack Publishing Company, Easton, Pennsylvania.
Romero-Sandoval, Alfonso et al, Clonidine Reduces Hypersensitivity and Alters the Balance of Pro- and Anti-Inflammatory Leukocytes After Local Injection at the Site of Inflammatory Neuritis, Brain Behav Immun, Jul. 2007, 569-580, 21(5).
Rosenblatt, J. et al., Chain Rigidity and Diffusional Release in Biopolymer Gels, Controlled Release Society, 1993, 264-265, 20.
Rosenblatt, J. et al., The Effect of Collagen Fiber Size Distribution on the Release Rate of Proteins From Collagen Matrices by Diffusion, J Controlled Release, 1989, 195-203, 9, Elsevier Science Publishers B.V.
Sannino, A. et al., Crosslinking of Cellulose Derivatives and Hyaluronic Acid With Water-Soluble Carbodiimide, Polymer, 2005, 11206-11212, 46.
SCULPTRA® Aesthetic (injectable poly-L-lactic acid) Directions for Use, Product Insert, Jul. 2009, 12 Pages, Dermik Laboratories.
Segall, A.I. et al, Stability of Vitamin C Derivatives in Topical Formulations Containing Lipoic Acid, Vitamins A and E, International Journal of Cosmetic Science, 2008, 453-458, 30.
Segura, Tatiana et al., Crosslinked Hyaluronic Acid Hydrogels: A Strategy to Functionalize and Pattern, Biomaterials, 2005, 359-371, 26 (4).
Selvi, Enrico et al., Arthritis Induced by Corticosteroid Crystals, The Journal of Rheumatology, 2004, 622, 31 (3).
Serban, et al., Modular Extracellular Matrices: Solutions for the Puzzle, Methods, 2008, 93-98, 45 (1).
Shoroghi, Mehrdad et al, Effect of Different Epinephrine Concentrations on Local Bleeding and Hemodynamics During Dermatologic Surgery, Acta Dermatovenerol Croat, 2008, 209-214, 16(4).
Shu, et al., In Situ Crosslinkable Hyaluronan Hydrogels for Tissue Engineering, Biomaterials, 2004, 1339-1348, 25, Elsevier.
Shu, Xiao et al, Synthesis and evaluation of injectable, in situ crosslinkable synthetic extracellular matrices for tissue engineering, Journal of Biomedical Materials Research, 2006, 902-912, 79A.
Silver, Frederick et al., Physical Properties of Hyaluronic Acid and Hydroxypropylmethylcellulose in Solution: Evaluation of Coating Ability, Journal of Applied Biomaterials, 1994, 89-98, 5.
Skardal, Aleksander et al., Bioprinting Vessel-Like Constructs Using Hyaluronan Hydrogels Crosslinked With Tetrahedral Polyethylene Glycol Tetracrylates, Biomaterials, 2010, 6173-6181, 31.
Smith, Kevin et al., Five Percent Lidocaine Cream Applied Simultaneously to the Skin and Mucosa of the Lips Creates Excellent Anesthesia for Filler Injections, Dermatol Surg, 2005, 1635-1637, 31.
Tezel, Ahmet et al., The science of hyaluronic acid dermal fillers, Journal of Cosmetic and Laser Therapy, 2008, 35-42, 10.
Visiol, TRB Chemedica Ophthalmic Line, Product Info, May 2014, p. 1-2, Geneva, CH.
Visiol, Viscoelstic Gel for Use in Ocular Surgery, http://www.trbchemedica.com/index.php/option=com_content&tas, 2010, 1 Page.
Vivawoman, Sodium Ascorbyl Phosphate: A Stable Vitamin C, Nov. 3, 2010, 13 Pages, http://www.vivawoman.net/2010/11/sodium-ascrobyl-phosphate-a-stable-vitamin-c/.
Wahl, Gregor, European Evaluation of a New Hyaluronic Acid Filler Incorporating Lidocaine, Journal of Cosmetic Dermatology, 2008, 298-303, 7.
Waraszkiewicz, Sigmund et al., Stability-Indicating High-Performance Liquid Chromatographic Analysis of Lidocaine Hydrochloride and Lidocaine Hydrochloride with Epinephrine Injectable Solutions, Journal of Pharmaceutical Sciences, 1981, 1215-1218, 70 (11).
Weidmann, Michael, New Hyaluronic Acid Filler for Subdermal and Long-lasting Volume Restoration of the Face, European Dermatology, 2009, 65-68.
Xia, Yun et al., Comparison of Effects of Lidocaine Hydrochloride, Buffered Lidocaine, Diphenhydramine, and Normal Saline After Intradermal Injection, Journal of Clinical Anesthesia, 2002, 339-343, 14.
Yeom, Junseok et al., Effect of Cross-Linking Reagents for Hyaluronic Acid Hydrogel Dermal Fillers on Tissue Augmentation and Regeneration, Bioconjugate Chemistry, 2010, 240-247, 21, American Chemical Society.
Yoshimura, Kotaro et al., Cell-Assisted Lipotransfer for Cosmetic Breast Augmentation: Supportive Use of Adipose-Derived Stem/Stromal Cells, Aesth. Plast. Surg., 2008, 48-55, 32.
Yui, Nobuhiko et al., Inflammation Responsive Degradation of Crosslinked Hyaluronic Acid Gels, Journal of Controlled Release, 1992, 105-116, 26.
Yui, Nobuhiko et al., Photo-Responsive Degradation of Heterogeneous Hydrogels Comprising Crosslinked Hyaluronic Acid and Lipid Microspheres for Temporal Drug Delivery, Journal of Controlled Release, 1993, 141-145, 26.
Yun, Yang H. et al., Hyaluronan Microspheres for Sustained Gene Delivery and Site-Specific Targeting, Biomaterials, 2004, 147-157, 25, US.
Zulian, F. et al., Triamcinolone Acetonide and Hexacetonide Intra-Articular Treatment of Symmetrical Joints in Juvenile Idiopathic Arthritis: A Double-Blind Trial, Rheumatology, 2004, 1288-1291, 43.
Pierre, et al., “Basics of Dermal Filler Rheology,” Dermatol Surg, 2015, vol. 41, pp. S120-S126.
Juvederm Volux, Product Insert, Jul. 26, 2018, 65 pages.
Boulle et al., “Lip Augmentation and Contour Correction with a Ribose Cross-linked Collagen Dermal Filler,” Journal of Drugs in Dermatology, Mar. 2009, vol. 8, Issue 3, 8 pages.
Calderon et al., “Type II Collagen-Hyaluronan Hydrogel—A Step Towards a Scaffold for Intervertebral Disc Tissue Engineering,” European Cells and Materials, 2010, vol. 20, pp. 134-148.
Crosslinking Technical Handbook, Termo Scientific, Apr. 2009, pp. 1-48.
Davidenko et al., “Collagen-hyaluronic acid scaffolds for adipose tissue engineering,” Acta Biomaterialia, 2010, vol. 8, pp. 3957-3968.
Gomis et al., “Effects of Different Molecular Weight Elastoviscous Hyaluronan Solutions on Articular Nociceptive Afferents,” Arthritis and Rheumatism, Jan. 2004, vol. 50, No. 1, pp. 314-326.
Kim et al., “Gallotannin Isolated from Euphorbia Species, 1, 2, 6-Tri-O-galloyl-b-D-allose, Decreases Nitric Oxide Production through Inhibition of Nuclear Factor-K>B and Downstream Inducible Nitric Oxide Synthase Expression in Macrophages,” Jun. 2009, Biological and Pharmaceutical Bulletin, vol. 32, No. 6, pp. 1053-1056.
Nadim et al., “Improvement of polyphenol properties upon glucosylation in a UV-induced skin cell ageing model,” International Journal of Cosmetic Science, Sep. 2014, vol. 36, No. 6, pp. 579-587.
Gallic Acid, National Center for Biotechnology Information, PubChem Compound Database, CID=370, 2018, https://pubchem.ncbi.nim.nih.gov/compound/370, 1 page.
Caffeic Acid, National Center for Biotechnology Information, PubChem Compound Database, CID=689043, 2018, https://pubchem.ncbi.nim.nih.gov/compound/689043, 1 page.
Park et al., “In vitro evaluation of conjugated Hyaluronic acid with Ascorbic Acid,” Journal of Bone and Joint Surgery, British vol. 92-B, 2010, 1 page abstract.
Tomihata et al., “Crosslinking of Hyaluronic Acid with Water-Soluable Carbodiimide,” J. Biomed Mater Res, Feb. 1997, vol. 37, No. 2, pp. 243-251.
Wang et al., “Development of hyaluronic acid-based scaffolds for brain tissue engineering,” Acta Biomaterialia, 2009, pp. 2371-2384.

Related Publications (1)

	Number	Date	Country
	20190192732 A1	Jun 2019	US

Continuations (4)

	Number	Date	Country
Parent	15825465	Nov 2017	US
Child	16290274		US
Parent	15099016	Apr 2016	US
Child	15825465		US
Parent	13675993	Nov 2012	US
Child	15099016		US
Parent	12714377	Feb 2010	US
Child	13675993		US

Continuation in Parts (1)

	Number	Date	Country
Parent	12687048	Jan 2010	US
Child	12714377		US

Heat stable hyaluronic acid compositions for dermatological use

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