Gelatin-based microspheres crosslinked with glutaraldehyde and rutin oriented to cosmetics

Graziola, Fabiana; Candido, Thalita Marcílio; Oliveira, Camila Areias de; Peres, Daniela D'Almeida; Issa, Michele Georges; Mota, Joana; Rosado, Catarina; Consiglieri, Vladi Olga; Kaneko, Telma Mary; Velasco, Maria Valéria Robles; Baby, André Rolim

doi:10.1590/S1984-82502016000400004

ABSTRACT

Glutaraldehyde (GTA) has been extensively used as a gelatin crosslinking agent, however, new natural ones have been suggested as more biocompatible. Polyphenols are possible candidates and the flavonols, such as rutin (RUT), also exhibit potential synergism with sunscreens and antioxidant agents used in cosmetics. In this work, gelatin microspheres (M0) were obtained and crosslinked with GTA 10 mM (MG) or RUT 10 mM (MR), dissolved in acetone:NaOH 0,01M (70:30 v/v). MG exhibited crosslinking extent of 54.4%. Gelatin, M0, MG and MR did not elicit any signs of skin damage, regarding the formation of erythema, the barrier function disruption and negative interference in the stratum corneum hydration. Oily dispersions containing M0, MG or MR, isolated or combined with benzophenone-3 or octyl methoxycinnamate, suggested that the microspheres, at a 5.0% w/w, had no additional chemical or physical photoprotective effect in vitro. Crosslinking with RUT had occurred, but in a lower degree than GTA. Microspheres had not improved sun protection parameters, although, non-treated gelatin interfered positively with the SPF for both UV filters. The in vivo studies demonstrated that these materials had very good skin compatibility.

Uniterms:
Protection solar/tests; Gelatin/microspheres/safety testing; Glutaraldehyde/safety testing; Flavonoids/Rutin/use in cosmetics; Natural products/use in cosmetics.

INTRODUCTION

Microspheres are microparticles in which a substance of interest is homogeneously dispersed within a polymer or a wax matrix, forming a monolithic system in which it is not possible to identify a distinct nucleus (Bresolin, Filho, 2003BRESOLIN, T.M.B.; CECHINEL FILHO, V. Ciências farmacêuticas: contribuição ao desenvolvimento de novos fármacos e medicamentos. Itajaí: Editora da Universidade do Vale do Itajaí, 2003. ). Gelatin is a biodegradable natural polymer that can be used to produce microparticles. However, due to the aqueous solubility and limited mechanical and thermal properties of gelatin microparticles, improvements, such as crosslinking reactions, are necessary in order to provide the use in long term applications (Bigi et al., 2002BIGI, A.; COJAZZI, G; PANZAVOLTA, S.; RUBINI, K.; ROVERI, N. Stabilization of gelatin films by crosslinking with genipin. Biomaterials , v.23, n.24, p.4827-32, 2002.; Hayashi, Tabata, 2011HAYASHI, K.; TABATA, Y. Preparation of stem cell aggregates with gelatin microspheres to enhance biological functions. Acta Biomater., v.7, n.7, 2797-2803, 2011.).

Crosslink reactions can be performed by chemical or physical medium and they cause structural changes that improve the gelatin mechanical strength and water resistance (Ratanavaraporn et al., 2010RATANAVARAPORN, J.; RANGKUPAN, R.; JEERATAWATCHAI, H.; KANOKPANONT, S.; DAMRONGSAKKUL, S. Influences of physical and chemical crosslinking techniques on electrospun type a and b gelatin fiber mats. Int. J. Biol. Macromol., v.47, n.4, p.431-438, 2010. ). Glutaraldehyde (GTA) is the most used aldehyde as chemical crosslinking, but its toxicity concerns and flaws in materials like heart valves, that triggers the search for new crosslinking substances (Catalina et al., 2013). Flavonoids are polyphenolic and aromatic substances constituted by 15 carbon atoms. They have a diphenylpropane skeleton (C₆C₃C₆) with two benzene rings bonded to a pyran ring. Due to such structure, flavonoids are characterized as intrinsic agents of protection against ultraviolet radiation (UV) by acting as chemical filters that absorb in this wavelength range (Bruneton, 1991BRUNETON, J. Elementos de Fitoquímica y de Farmacognosia. Zaragoza: Acribia, 1991. ; Baby et al., 2009BABY, A.R.; HAROUTIOUNIAN-FILHO, C.A.; SARRUF, F.D.; PINTO, C.A.S.O.; KANEKO, T.M.; VELASCO, M.V.R. Influence of urea, isopropanol and propylene glycol on rutin in vitro release from cosmetic semisolid systems estimated by factorial design. Drug Dev. Ind. Pharm., v.35, p.272-282, 2009.). Flavonoids are further divided into 13 classes according to the chemical structure, including flavonols (rutin, quercetin and mericitin). Because of its strong antioxidant activity, rutin is used in the prevention or treatment of venous or lymphatic insufficiency or capillary fragility and permeability, as well as, being used in the prevention of the damage caused by UV radiation (Velasco et al., 2008VELASCO, M.V.R.; SARRUF, F.D.; SALGADO-SANTOS, I.M.; HAROUTIOUNIAM-FILHO, C.A.; KANEKO, T.M.; BABY, A.R. Broad spectrum bioactive sunscreens. Int. J. Pharm., v.1/2, p.50-57, 2008.; Peres et al., 2016PERES, D.D.; OLIVEIRA, C.A.; COSTA, M.S.; TOKUNAGA, V.K.; MOTA, J.P.; ROSADO, C.; CONSIGLIERI, V.O.; KANEKO, T.M.; VELASCO, M.V.R.; BABY, A.R. Rutin increases critical wavelength of systems containing a single UV filter and with good skin compatibility. Skin Res. Technol., v.22, p.325-333, 2016.). Besides, flavonoids have been studied as a new alternative to chemical crosslinking agent for gelatin (Bigi et al., 2002BIGI, A.; COJAZZI, G; PANZAVOLTA, S.; RUBINI, K.; ROVERI, N. Stabilization of gelatin films by crosslinking with genipin. Biomaterials , v.23, n.24, p.4827-32, 2002.; Strauss, Gibson 2004STRAUSS, G.; GIBSON, S.M. Plant phenolics as cross-linkers of gelatin gels and gelatin-based coacervates for use as food ingredients. Food Hydrocolloid, v.18, n.1, p.81-89, 2004.).

Chemical filters are substances that may be included in cosmetic formulations to protect the skin from damage caused by solar radiation. However, they can generate free radicals when exposed to sunlight and present problems related to photoallergenicity and skin irritation, as well as, photoinstability (Hanson, Gratton, Bardeen, 2006HANSON, K.M.; GRATTON, E.; BARDEEN, C.J. Sunscreen enhancement of uv-induced reactive oxygen species in the skin. Free Radical Biol. Med., v.41, n.8, p.1205-1212, 2006.). Such scenario has driven the search for alternatives to minimize or eliminate these effects and there is a tendency to develop photoprotective cosmetic formulations with reduced concentration of chemical filters, but with high protection against UVA and UVB radiation, preferentially, with multifunctional benefits. The research of new photostable molecules for use in sunscreens are still performed extensively and, currently, we notice growing interest for the development of sunscreens based on natural products (Schlumpf et al., 2004SCHLUMPF, M.; SCHMID, P.; DURRER, S.; CONSCIENCE, M.; MAERKEL, K.; HENSELER, M.; GRUETTER, M.; HERZOG, I.; REOLON, S.; CECCATELLI, R.; FAASS, O.; STUTZ, E.; JARRY, H.; WUTTKE, W.; LICHTENSTEIGER, W. Endocrine activity and developmental toxicity of cosmetic uv filters - an update. Toxicology, v.205, n.1-2, p.113-122, 2004.; Tanaka, Setsuko, Utsumi, 1963TANAKA, N.; SETSUKO, T.; UTSUMI, I. A new oral gelatinized sustained-release dosage form. J. Pharm. Sci., v.52, n.7, p.664-667, 1963.; Oliveira et al., 2016OLIVEIRA, C.A.; PERES, D.D.; GRAZIOLA, F.; BOU-CHACRA, N.A.; ARAUJO, G.L.B.; FLORIDO, A.C.; MOTA, J.P.; ROSADO, C.; VELASCO, M.V.R.; RODRIGUES, L.M.; FERNANDES, A.S.; BABY, A.R. Cutaneous biocompatible rutin-loaded gelatin-based nanoparticles increase SPF of the association of UVA and UVB filters. Eur. J. Pharm. Sci., v.81, p.1-9, 2016.).

In this research work, we investigated the use of the flavonoid rutin as an alternative to GTA for crosslinking gelatin microparticles. The good cutaneous compatibility of our samples was established by non-invasive methods and the physicochemical and functional properties of microparticles were determined to evaluate their applications as adjuvants for performance improvement of photoprotective dermocosmetic products.

MATERIAL AND METHODS

Obtainment of gelatin microspheres

Gelatin microspheres were obtained by emulsion polymerization method, using surfactant and solvent extraction (Tanaka, Setsuko, Utsumi, 1963TANAKA, N.; SETSUKO, T.; UTSUMI, I. A new oral gelatinized sustained-release dosage form. J. Pharm. Sci., v.52, n.7, p.664-667, 1963.; Ugwoke, Kinget, 1998UGWOKE, M.I.; KINGET, R. Influence of processing variables on the properties of gelatin microspheres prepared by the emulsification solvent extraction technique. J. Microencapsul., v.15, n.3, p.273-281, 1998.). Gelatin (bovine, food grade, bloom 180 and mesh 30) was purchased from NP^(r) (São Paulo, Brazil). An aqueous gelatin solution at 10.0% w/w (240.0 g) was transferred by dripping to a mixture of mineral oil (560.0 mL) and sorbitan monooleate (final concentration of 1.0% w/v) involving heating (55.0 °C) in a ceramic hot plate and mechanical agitation at 2400 rpm. The resulting emulsion was maintained under the conditions described previously for 15 min and then it was cooled to room temperature (25.0 °C) using water bath and 2400 rpm agitation. Then, to enable the gelation of the sample, the emulsion was cooled between 10.0 and 15.0 °C with an ice bath while stirring. After 30 min, acetone (400.0 mL), at of 5.0 °C, was added dropwise with a burette to the emulsion and the mixture was stirred for another 30 min, keeping the temperature at 10.0-15.0 °C, and then it was fractionated on 50.0 mL in plastic tubes to be centrifuged. After centrifugation (2 min, 3400 rpm, room temperature), the supernatant was discarded. To the amount of solid residue was added in an equal volume of acetone at 5.0 °C. The tubes were centrifuged again at 3400 rpm for 2 min. This procedure was repeated three times. After the last acetone washing, the solid residues were combined and dried at room temperature for at least 12 hours and the dry residue was sieved in 80 mesh sieve (0.177 mm opening).

Crosslinking of gelatin microspheres

The crosslinking medium was consisted of acetone: NaOH 0.01 M (70:30 v/v), in the proportion of 5.0 g of microspheres for each 100.0 mL of medium. The crosslinking agents were GTA (final concentration: 0.1% w/v, equivalent to 10.0 mM) and RUT (final concentration: 0.6% w/v, equivalent to 10.0 mM) and we accomplished the crosslinking process for 4 hours with magnetic stirring at maximum speed at room temperature. After, the crosslinking medium was removed and the crosslinked microspheres were washed 5 times with acetone and agitated for 15 min with magnetic stirring at maximum speed. Subsequently, the crosslinked microspheres were kept in an open beaker to allow air drying for, at least, 12 hours. The microspheres were sieved at 80 mesh sieve.

Appearance by scanning electron microscopy (SEM)

Morphology of gelatin, M0, MG and MR was assessed by SEM. Dry and aqueous samples of gelatin used for obtaining the microparticles were observed and the microparticles were observed in triplicate. The observation of the samples was performed in scanning electron microscope Quanta 600 FEG, FEI^(r) Company, (Hillsboro, OR, U.S.A.) in microscopic magnification of 150 to 50,000 times.

Determination of extent of crosslinking

There were added to 15.0 mL plastic tubes about 15.0 mg of each sample. Then, to each tube was added 1.0 mL of NaHCO₃ (4% w/v) and 1.0 mL of TNBS (0.5% w/v). The tubes were transferred to a bath and kept for 2 hours in this condition. After, the TNBS reaction was stopped by adding 3.0 mL of HCl (6.0 N) and the tubes were transferred to an ultrasonic bath, where they remained at 60.0°C for 90 min, to ensure complete dissolution of samples. Subsequently, there were added 5.0 mL of purified water to each tube. The resulting solution was diluted to 1:10 and subjected to spectrophotometric analysis, in triplicate, at 345.0 nm, using UV-VIS Spectrophotometer 600 Evolution^(r), Thermo Scientific (San Jose, CA, U.S.A.) (Sheu et al., 2001SHEU, M.T.; HUANG, J.C.; YEH, G.C.; HO, H.O. Characterization of collagen gel solutions and collagen matrices for cell culture. Biomaterials , v.22, n.13, p.1713-1719, 2001.).

A standard curve of L-leucine with concentration range from 0.0 to 3.0 mM was performed to measure free ɛ-amino groups in samples, which is equivalent to L-leucine groups (Gan, Cheng, Easa, 2009GAN, C.Y.; CHENG, L.H.; EASA, A.M. Assessment of cross-linking in combined cross-linked soy protein isolate gels by microbial transglutaminase and maillard reaction. J. Food Sci., v.74, n.2, p.141-146, 2009.). The extent of crosslinking was calculated as shown in Equation 1.

Determination of surface area

Measurements of surface area and porosity were performed in gas adsorption analyzer NOVA^(r) 2200E, Quantachrome Corporation (Boynton Beach, FL, U.S.A.). Samples were subjected to freezing in liquid nitrogen for 20 min and then analyzed with ultra-pure nitrogen. For each sample, the isotherms were constructed utilizing multipoint method by collecting 30 points of adsorption and 20 of desorption. Results were generated by NOVA^(r) P -Win 9.0 program.

Determination of true density

The determination of the true density of the samples was performed in a helium gas pycnometer, Ultrapycnometer^(r) 1000, Quantachrome Corporation. Approximately, 1.5 to 4.0 g of each sample was subjected to three successive measurements of volume and density and, ultimately, the average density was determined.

Determination of particle size distribution

The determination of particle size distribution was done in laser diffraction particle size analyzer CILAS^(r) 1090L (Orléans, France) by wet method. Sufficient amount of sample to obtain obscuration around 15% was dispersed in 50 mL of isopropyl alcohol and submitted to reading. Each sample was analyzed in triplicate in a range from 0.04 to 500 µM per 100 classes.

In vivo cutaneous compatibility assays

Cutaneous compatibility was performed with 12 male and female volunteers, after informed oral and written consent. The procedures were in accordance with the ethical standards of the local responsible committee on human experimentation (Comissão de Ética da ULHT, Lisbon, Portugal) and with the Helsinki Declaration. Epicutaneous patches (Finn Chambers^(r), Epitest) were applied in the volar forearms of the volunteers for 24 h. Each patch had 5 chambers, containing each of the samples (gelatin, M0, MG and MR) at 10% w/v in purified water, as well as, purified water as the negative control. Non-invasive measurements were conducted in each tested site: stratum corneum (SC) hydration was assessed with a Corneometer^(r) CM825 (CK Electronics GmbH); skin barrier was probed with a Tewameter^(r) TM 300 (CK Electronics GmbH). A Chroma Meter CR-300 (Minolta Camera, Japan) was used to quantify a possible increase in erythema by the parameter a* that reflects the red chromaticity. All measurements were performed in triplicate and using the CIE Lab system. The basal values were determined before patch application, and further measurements were made at 24 hours, 2 hours after its removal. To minimize the effect of inter-individual variability, the results were analyzed as the ratio between the values obtained after patch application and the basal values (Oliveira et al., 2015OLIVEIRA, C.A.; PERES, D.D.; RUGNO, C.M.; KOJIMA, M.; PINTO, C.A.S.O.; CONSIGLIERI, V.O.; KANEKO, T.M.; ROSADO, C.; MOTA, J.; VELASCO, M.V.R.; BABY, A.R. Functional photostability and cutaneous compatibility of bioactive UVA sun care products. J. Photoch. Photobio. B, v.148, p.154-159, 2015.; Peres et al., 2016PERES, D.D.; OLIVEIRA, C.A.; COSTA, M.S.; TOKUNAGA, V.K.; MOTA, J.P.; ROSADO, C.; CONSIGLIERI, V.O.; KANEKO, T.M.; VELASCO, M.V.R.; BABY, A.R. Rutin increases critical wavelength of systems containing a single UV filter and with good skin compatibility. Skin Res. Technol., v.22, p.325-333, 2016.).

In vitro efficacy determination

Fifteen dispersions (formulations) were prepared with mineral oil, and mineral oil (and) polyethylene (Crodabase^(r) SQ). There were added to dispersions: gelatin, M0, MG, MR, benzophenone-3 (BZ3) and octyl methoxycinnamate (OCT), alone or in combination, in order to obtain the sunscreen activity in vitro. Formulations followed the proportions shown in Table I.

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TABLE I
Composition of the dispersions (%w/w)

For functional in vitro characterization of the samples, it was used diffuse reflectance spectrophotometer, equipped with integrating sphere, UV Transmittance Analyzer, Labsphere^(r) UV-2000S (North Sutton). In order to mimic the surface properties of human epidermis, it was used a quartz plate substrate coated with Transpore^(r) tape (Springsteen et al., 1999SPRINGSTEEN, A.; YUREK, R.; FRAZIER, M.; CARR, K.F. In vitro measurement of sun protection factor of sunscreens by diffuse transmittance. Anal. Chim. Acta, v.380, n.2-3, p.155-164, 1999.; Velasco et al., 2008VELASCO, M.V.R.; SARRUF, F.D.; SALGADO-SANTOS, I.M.; HAROUTIOUNIAM-FILHO, C.A.; KANEKO, T.M.; BABY, A.R. Broad spectrum bioactive sunscreens. Int. J. Pharm., v.1/2, p.50-57, 2008.)where human volunteers are subjected to potentially damaging and carcinogenic doses of ultraviolet radiation, has been the method of choice by regulatory agencies for determining the efficacy of sunscreens to protect humans from both sunburn (solar erythema.

Aliquots of the samples, accurately 0.75 mg/cm², were applied uniformly in the form of film, in a circular motion on the surface of the substrate. The records of spectrophotometric absorbance values were performed in the wavelength range between 290.0 and 400.0 nm, rate of progression of 1.0 nm. The analysis was performed in triplicates for obtaining in vitro SPF (Springsteen et al., 1999SPRINGSTEEN, A.; YUREK, R.; FRAZIER, M.; CARR, K.F. In vitro measurement of sun protection factor of sunscreens by diffuse transmittance. Anal. Chim. Acta, v.380, n.2-3, p.155-164, 1999.; Velasco et al., 2008VELASCO, M.V.R.; SARRUF, F.D.; SALGADO-SANTOS, I.M.; HAROUTIOUNIAM-FILHO, C.A.; KANEKO, T.M.; BABY, A.R. Broad spectrum bioactive sunscreens. Int. J. Pharm., v.1/2, p.50-57, 2008.; Silva et al., 2013SILVA, D.G.; SARRUF, F.D.; OLIVEIRA, L.C.D.; ARÊAS, E.P.G.; KANEKO, T.M.; CONSIGLIERI, V.O.; VELASCO, M.V.R.; BABY, A.R. Influence of particle size on appearance and in vitro efficacy of sunscreens. Braz. J. Pharm. Sci., v.49, n.2, p.251-261, 2013. ).

Analysis of results

Statistical analysis was performed using a Minitab (Version 16) software, with a significance level of 5.0% (α = 0.05). Data were treated using one-way ANOVA followed by Tukey test for multiple comparisons.

RESULTS AND DISCUSSION

Aspect of microspheres and yield of the processes of preparation and crosslinking

Protein-based microspheres were developed with gelatin, a raw material that offers low cost, biocompatibility, biodegradability, low antigenicity and potential application in several dermocosmetic products (Nahar et al., 2008NAHAR, M.; MISHRA, D.; DUBEY, V.; JAIN, N.K. Development, characterization, and toxicity evaluation of amphotericin b-loaded gelatin nanoparticles. Nanomed-Nanotechnol., v.4, n.3, p.252-261, 2008.). The gelatin microspheres were slightly yellowish fine powder, unlike the coarse yellowish powder aspect of the gelatin, as raw material. After the crosslinking process, the powder aspect changed to slightly beige, when the GTA was the crosslinking agent and, to greenish yellow, when the RUT was the crosslinking agent.

The loss of, approximately, 25% in the process of obtaining microspheres can be mainly explained by the separation and removal of the low molecular weight gelatin in the supernatant of the emulsion when adding acetone, which is an agent that precipitates high molecular weight gelatin (Nahar et al., 2008NAHAR, M.; MISHRA, D.; DUBEY, V.; JAIN, N.K. Development, characterization, and toxicity evaluation of amphotericin b-loaded gelatin nanoparticles. Nanomed-Nanotechnol., v.4, n.3, p.252-261, 2008.). The loss observed between 15 and 18% in the crosslinking process of the microspheres can be explained mainly by the process of separation, by sieving and washes with acetone (Table II).

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TABLE II
Microspheres process yield

Scanning electron microscopy

It was observed that the gelatin used to obtain microspheres showed amorphous granules larger than 100 micron size (Figure 1). In increase of 5,000 times, it was possible to observe in detail the texture of gelatin suggesting compact and dense structure.

FIGURE 1
SEM photomicrographs of gelatin (raw material) at a magnification of 150x (a), 5,000 x (b) and 650x (c).

The gelatin microspheres obtained in this research work showed heterogeneity spherical shape and size (Figure 2). This observation confirmed the variation description of the particle size obtained by emulsion polymerization method using a surfactant and solvent extraction (Rabanel et al., 2009RABANEL, J.M.; BANQUY, X.; ZOUAOUI, H.; MOKHTAR, M.; HILDGEN, P. Progress technology in microencapsulation methods for cell therapy. Biotechnol. Progr., v.25, n.4, p.946-963, 2009.).

FIGURE 2
SEM photomicrographs of M0 (a), MG (b) and MR (c) at a magnification of 3,000x, 25,000x and 50,000x.

With a magnification of 50,000 times, it was possible to observe that the surface of all microspheres had a slight roughness, suggesting that crosslinking had no impact on surface morphology. This finding is contrary to that described by Choy et al. (2008CHOY, Y.B.; CHENG, F.; CHOI, H.; KIM, K.K. Monodisperse gelatin microspheres as a drug delivery vehicle: release profile and effect of crosslinking density. Macromol. Biosci., v.8, n.8, p.758-765, 2008.), who observed expressive wrinkles on the surface of MG and described by Patel et al. (2006PATEL, M.; JAIN, S.K.; YADAV, A.K.; GOGNA, D.; AGRAWAL, G.P., Preparation and characterization of oxybenzone-loaded gelatin microspheres for enhancement of sunscreening efficacy. Drug Deliv., v.13, n.5, p.323-330, 2006.), who obtained microspheres with smooth surface (Choy et al., 2008CHOY, Y.B.; CHENG, F.; CHOI, H.; KIM, K.K. Monodisperse gelatin microspheres as a drug delivery vehicle: release profile and effect of crosslinking density. Macromol. Biosci., v.8, n.8, p.758-765, 2008.). The use of NaOH and acetone, as a medium of crosslinking, may have led to differences in relation to the literature. The presence of agglomerates was greater in MG and MR than in M0.

Extent of crosslinking

The extent of crosslinking was determined by measuring the absorbance of the chromophore formed in the reaction of the free ɛ-amino groups of M0, MG and MR with 2,4,6-trinitrobenzenesulfonic acid (TNBS) with modifications (Sheu et al., 2001SHEU, M.T.; HUANG, J.C.; YEH, G.C.; HO, H.O. Characterization of collagen gel solutions and collagen matrices for cell culture. Biomaterials , v.22, n.13, p.1713-1719, 2001.). The extent of crosslinking was calculated in relation to non-crosslinked samples.

Reaction extent for gelatin and M0 were equal, demonstrating that the obtaining process of the microspheres had no impact on crosslinking of the free amino groups on the gelatin. Comparing to M0, the process of MG crosslinking resulted in the reduction of free amino groups with extent of 54.4%. This value indicated that the free amino groups were successfully crosslinked when treated for 4h, under agitation in room temperature in a NaOH 0.01M and acetone solution containing GTA 10 mM (0.1%). As exposed, this crosslinking occurred faster than the reaction described by Bigi et al. (2001BIGI, A.; COJAZZI, G; PANZAVOLTA, S.; RUBINI, K.; ROVERI, N. Mechanical and thermal properties of gelatin films at different degrees of glutaraldehyde crosslinking. Biomaterials, v.22, n.8, p.763-68, 2001.) that registered an extent of crosslinking of 60.0% in gelatin films treated with 7.4 phosphate buffer containing GTA 0.05% for 24 hours at room temperature (samples were remained in rest). Regarding the values obtained with RUT reaction, it was observed that MR extent of crosslinking occurred quite discreetly (14.4%).

Surface area, Porosity and True Density

Table III presents the results of surface area, pore volume, pore size and true density for gelatin, M0, MG and MR. Surface area and pore volume of MG were significantly lower than the values obtained for M0 and MR. However, this occurrence brought no changes to surface morphology of microspheres that can be identified by the SEM photomicrographs. The amount of pore sizes for all samples was in the range of mesoporosity classification (20-500 nm) (Teixeira, Coutinho, Gomes, 2001TEIXEIRA, V.G.; COUTINHO, F.M.B., GOMES, A.S. Principais métodos de caracterização da porosidade de resinas à base de divinilbenzeno. Quim. Nova, v.24, n.6, p.808-818, 2001.). No significant differences in this parameter were observed amongst M0, MG and MR. Values of true density for all samples showed no significant variations. This fact indicated that crosslinking with GTA influenced the results of surface area and pore volume, but it had no effect on true density of the powder.

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TABLE III
Surface area, volume and pore sizes, true density, diameters of 10%, 50%, 90% and average diameter by laser diffraction of gelatin and gelatin microspheres

Particle size distribution and particle diameters

The particle size distribution is presented in Figure 3. MR presented the smaller particle size distribution amplitude than M0 and MG. Diameter values at 10, 50, 90% and average diameter of gelatin, M0, MG and MR are presented in Table II.

FIGURE 3
Particle size distribution by laser diffraction of gelatin (a), M0 (b), MG (c) and MR (d).

Results presented that average diameters were higher in groups subjected to crosslinking (MG and MR), although, this value was only consistent with that one observed for surface area regarding the MG, which showed that the increase in particle diameter implied in its surface area reduction. Also, it has been reported that GTA is an effective crosslinker agent that provides stability and shape to gelatin microspheres by forming a network structure from the GTA aldehyde groups and the gelatin amino groups undergoing Schiff base reaction (Karthikeyan et al., 2013KARTHIKEYAN, S.; RAJENDRA PRASAD, N.; GANAMANI, A.; BALAMURUGAN, E. Anticancer activity of resveratrol-loaded gelatin nanoparticles on NCI-H460 non-small cell lung cancer cells. Biomed. Prev. Nutr., v.3, n.1, p.64-73, 2013.).

These results may indicate that, during the microspheres obtaining process, the washes with acetone, aiming at removing any oil residual, promoted deagglomeration of the particles, although, the crosslinking agents and some oily remained residual contributed to the highest average diameter for MG and MR.

In vitro cutaneous compatibility assays

According to the in vivo cutaneous biophysical properties established before (basal values) and 24 hours subsequently to the patch test, aqueous dispersions at 10.0% w/v of gelatin (non-treated raw material), M0, MG and MR did not elicit any signs of skin damage, regarding the formation of erythema (skin redness), disruption of the barrier function (increase in transepidermal water loss) and negative interference in the SC hydration, in comparison with the negative control (purified water). For all the variables, the ratio between the values after the patch application and the basal values was, hence, close to 1 (Figure 4). The ratio was used to decrease the inter-individual variability impact (Oliveira et al., 2015OLIVEIRA, C.A.; PERES, D.D.; RUGNO, C.M.; KOJIMA, M.; PINTO, C.A.S.O.; CONSIGLIERI, V.O.; KANEKO, T.M.; ROSADO, C.; MOTA, J.; VELASCO, M.V.R.; BABY, A.R. Functional photostability and cutaneous compatibility of bioactive UVA sun care products. J. Photoch. Photobio. B, v.148, p.154-159, 2015.).

FIGURE 4
In vivo cutaneous compatibility assays established by non-invasive methods (TEWL: transepidermal water loss; skin redness; and SC hydration: stratum corneum. M0: uncrosslinked gelatin microspheres; MG: gelatin microspheres crosslinked with GTA; MR: gelatin microspheres crosslinked with RUT.

Photoprotective activity in vitro: SPF and protection against UVA

Table IV presents the results of photoprotective efficacy in vitro for dispersions containing gelatin, M0, MG, MR, and/or UV filters, alone or in combination.

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TABLE IV
Photoprotective efficacy in vitro for dispersions containing gelatin and gelatin microspheres, and UV filters alone or in combination. Values were expressed as mean ± standard deviation (n = 3)

SPF values for dispersions containing gelatin (dispersion B), M0 (dispersion C), MG (dispersion D) or MR (dispersion E) were equal to base dispersion (dispersion A), that presented value close to 1.0 (no anti-UVB efficacy). All dispersions containing OCT and gelatin or microspheres (dispersions L, M, N and O) presented SPF values equal to or greater than 4.0. However, regarding to dispersions containing BZ3 and gelatin or microspheres, only the one containing gelatin (dispersion G) presented SPF values equal to or greater than 4.0.

The dispersions containing gelatin and BZ3 or OCT (dispersions G and L) had higher SPF values than the dispersions containing only one of these UV filters (dispersions F and K), suggesting that the gelatin, as raw material, when combined with filters, showed good film formation and/or absorption in the UVB region that contributed with the SPF improvement (dispersions G and L) and, interestingly, M0 did not achieve an enhanced performance as the gelatin, even though, there was not the use of crosslinking agent.

According to our results, it may be suggested that M0, MG and MR performed discreetly film formation and with similar profile among them. It was supposed that the microspheres could develop a booster SPF activity by dispersing the UV radiation, considering the more rigid spherical structures achieved by the reaction with GTA and RUT, or by absorbing the UVB and UVA radiation, regarding the presence of the flavonoid. It is also allowed to suppose that the polymorph aspect of the gelatin, as raw-material, could have influenced the film formation more efficiently considering the arrangement of the irregular shape gelatin particles, that structured a thicker film, since the gelatin is not soluble at the oily vehicle adopted in this research. Still considering this property, the effect of MR could have been inhibited by two mechanisms: (i) rutin was inaccessible to absorb the UV radiation since it was bound to the gelatin through the crosslinking reaction; and (ii) rutin was not sufficient soluble at the oily vehicle, than it was not adequately free for exerting its UV absorbing property. Rutin is a natural compound that does not possess the tendency to permeate across the skin and it is a notable antioxidant that has been studied as sunscreen adjuvant with promising results. For example, our research group observed that an O/W emulsion containing 0.1% rutin in association with 3.5% octyl methoxycinnamate and 1.0% benzophenone-3 developed a significant improvement of the in vitro sun protective properties in comparison with a similar preparation without the flavonoid (Baby et al., 2008BABY, A.R.; HAROUTIOUNIAN-FILHO, C.A.; SARRUF, F.D.; TAVANTE-JÚNIOR, C.R.; PINTO, C.A.S.O.; ZAGUE, V.; ARÊAS, E.P.G.; KANEKO, T.M.; VELASCO, M.V.R. Estabilidade e estudo de penetração cutânea in vitro da rutina veiculada em uma emulsão cosmética através de um modelo de biomembrana alternativo. Rev.Bras.Ciênc.Farm.v.44, p.233-248, 2008.; de Oliveira et al., 2015OLIVEIRA, C.A.; PERES, D.D.; RUGNO, C.M.; KOJIMA, M.; PINTO, C.A.S.O.; CONSIGLIERI, V.O.; KANEKO, T.M.; ROSADO, C.; MOTA, J.; VELASCO, M.V.R.; BABY, A.R. Functional photostability and cutaneous compatibility of bioactive UVA sun care products. J. Photoch. Photobio. B, v.148, p.154-159, 2015.). Oliveira et al. (2015)OLIVEIRA, C.A.; PERES, D.D.; RUGNO, C.M.; KOJIMA, M.; PINTO, C.A.S.O.; CONSIGLIERI, V.O.; KANEKO, T.M.; ROSADO, C.; MOTA, J.; VELASCO, M.V.R.; BABY, A.R. Functional photostability and cutaneous compatibility of bioactive UVA sun care products. J. Photoch. Photobio. B, v.148, p.154-159, 2015. additionally described the positive interaction of 0.1% rutin and 6.0% BZ3 in an O/W emulsion. Authors observed that the flavonoid contributed with the elevation of the in vitro SPF of 24 to 33. It is noteworthy to mention that the gelatin, M0, MG and MR concentrations were not suitable enough to interfere more positively with the efficacy parameters of sun protection.

Regarding λ_C (critical wavelength, nm), only dispersions without filters (dispersions A, B, C, D and E) presented values of λ_C greater than 370 nm. However, the average SPF values were approximately 1.0, indicating low protection against UVB radiation. The UVA/UVB ratio of dispersions containing OCT (dispersions K, L, M, N and O) was the lowest of all dispersions and it can be explained by UVB action, that is assigned to this chemical UV filter. Dispersions without filters showed no significant absorbance, indicating that gelatin and isolated microparticles did not develop substantial photoprotective action. In mixtures containing BZ3 and/or OCT, it was observed that there were no changes in the peak profiles due to the presence of gelatin or M0, MG or MR.

CONCLUSION

Physicochemical properties of MG and MR indicated that crosslinking method was more effective when the crosslinking agent was GTA and suggested that crosslinking occurred with RUT, however, to a lesser extent that would reinforce further researches to establish optimal conditions for the use of rutin as a potential substituent for GTA. The SPF analysis of dispersions containing M0, MG or MR, isolated or combined with chemical UV filters (benzophenone-3 and octyl methoxycinnamate) suggested that the microspheres (M0, MG or MR), at a 5.0% w/w, had no additional chemical or physical photoprotective effect in vitro, and showed no influence on the estimated efficacy when combined with UV filters, that implies in formulation adjustments such as increasing of the gelatin microsphere concentrations and, as well as, use of new classes of UV filters. The in vivo studies demonstrated that these materials had very good skin compatibility.

ACKNOWLEDGMENT

Authors are greatly thankful to The State of São Paulo Foundation - FAPESP - (2012/04435-9 and 2012/19972-0). Authors thank Prof. Humberto Gomes Ferraz for his valuable support regarding the analysis of particle size distribution, surface area, pore volume, pore size and true density. Authors also thank Prof. Carlota de Oliveira Rangel-Yagui and Prof. Tânia Santos de Almeida for their kind supports.

REFERENCES

BABY, A.R.; HAROUTIOUNIAN-FILHO, C.A.; SARRUF, F.D.; TAVANTE-JÚNIOR, C.R.; PINTO, C.A.S.O.; ZAGUE, V.; ARÊAS, E.P.G.; KANEKO, T.M.; VELASCO, M.V.R. Estabilidade e estudo de penetração cutânea in vitro da rutina veiculada em uma emulsão cosmética através de um modelo de biomembrana alternativo. Rev.Bras.Ciênc.Farm.v.44, p.233-248, 2008.
BABY, A.R.; HAROUTIOUNIAN-FILHO, C.A.; SARRUF, F.D.; PINTO, C.A.S.O.; KANEKO, T.M.; VELASCO, M.V.R. Influence of urea, isopropanol and propylene glycol on rutin in vitro release from cosmetic semisolid systems estimated by factorial design. Drug Dev. Ind. Pharm., v.35, p.272-282, 2009.
BIGI, A.; COJAZZI, G; PANZAVOLTA, S.; RUBINI, K.; ROVERI, N. Mechanical and thermal properties of gelatin films at different degrees of glutaraldehyde crosslinking. Biomaterials, v.22, n.8, p.763-68, 2001.
BIGI, A.; COJAZZI, G; PANZAVOLTA, S.; RUBINI, K.; ROVERI, N. Stabilization of gelatin films by crosslinking with genipin. Biomaterials , v.23, n.24, p.4827-32, 2002.
BRESOLIN, T.M.B.; CECHINEL FILHO, V. Ciências farmacêuticas: contribuição ao desenvolvimento de novos fármacos e medicamentos. Itajaí: Editora da Universidade do Vale do Itajaí, 2003.
BRUNETON, J. Elementos de Fitoquímica y de Farmacognosia. Zaragoza: Acribia, 1991.
CATALINA, M.; ATTENBURROW, G.E.; COT, J.; COVINGTON, A.D.; ANTUNES, A.P.M. Influence of crosslinkers and crosslinking method on the properties of gelatin films extracted from leather solid waste. J. Appl. Polym. Sci, v.119, n.4, p.2105-2111, 2011.
CHOY, Y.B.; CHENG, F.; CHOI, H.; KIM, K.K. Monodisperse gelatin microspheres as a drug delivery vehicle: release profile and effect of crosslinking density. Macromol. Biosci, v.8, n.8, p.758-765, 2008.
GAN, C.Y.; CHENG, L.H.; EASA, A.M. Assessment of cross-linking in combined cross-linked soy protein isolate gels by microbial transglutaminase and maillard reaction. J. Food Sci, v.74, n.2, p.141-146, 2009.
HANSON, K.M.; GRATTON, E.; BARDEEN, C.J. Sunscreen enhancement of uv-induced reactive oxygen species in the skin. Free Radical Biol. Med, v.41, n.8, p.1205-1212, 2006.
HAYASHI, K.; TABATA, Y. Preparation of stem cell aggregates with gelatin microspheres to enhance biological functions. Acta Biomater, v.7, n.7, 2797-2803, 2011.
KARTHIKEYAN, S.; RAJENDRA PRASAD, N.; GANAMANI, A.; BALAMURUGAN, E. Anticancer activity of resveratrol-loaded gelatin nanoparticles on NCI-H460 non-small cell lung cancer cells. Biomed. Prev. Nutr, v.3, n.1, p.64-73, 2013.
NAHAR, M.; MISHRA, D.; DUBEY, V.; JAIN, N.K. Development, characterization, and toxicity evaluation of amphotericin b-loaded gelatin nanoparticles. Nanomed-Nanotechnol, v.4, n.3, p.252-261, 2008.
OLIVEIRA, C.A.; PERES, D.D.; GRAZIOLA, F.; BOU-CHACRA, N.A.; ARAUJO, G.L.B.; FLORIDO, A.C.; MOTA, J.P.; ROSADO, C.; VELASCO, M.V.R.; RODRIGUES, L.M.; FERNANDES, A.S.; BABY, A.R. Cutaneous biocompatible rutin-loaded gelatin-based nanoparticles increase SPF of the association of UVA and UVB filters. Eur. J. Pharm. Sci., v.81, p.1-9, 2016.
OLIVEIRA, C.A.; PERES, D.D.; RUGNO, C.M.; KOJIMA, M.; PINTO, C.A.S.O.; CONSIGLIERI, V.O.; KANEKO, T.M.; ROSADO, C.; MOTA, J.; VELASCO, M.V.R.; BABY, A.R. Functional photostability and cutaneous compatibility of bioactive UVA sun care products. J. Photoch. Photobio. B, v.148, p.154-159, 2015.
PATEL, M.; JAIN, S.K.; YADAV, A.K.; GOGNA, D.; AGRAWAL, G.P., Preparation and characterization of oxybenzone-loaded gelatin microspheres for enhancement of sunscreening efficacy. Drug Deliv., v.13, n.5, p.323-330, 2006.
PERES, D.D.; OLIVEIRA, C.A.; COSTA, M.S.; TOKUNAGA, V.K.; MOTA, J.P.; ROSADO, C.; CONSIGLIERI, V.O.; KANEKO, T.M.; VELASCO, M.V.R.; BABY, A.R. Rutin increases critical wavelength of systems containing a single UV filter and with good skin compatibility. Skin Res. Technol., v.22, p.325-333, 2016.
RABANEL, J.M.; BANQUY, X.; ZOUAOUI, H.; MOKHTAR, M.; HILDGEN, P. Progress technology in microencapsulation methods for cell therapy. Biotechnol. Progr, v.25, n.4, p.946-963, 2009.
RATANAVARAPORN, J.; RANGKUPAN, R.; JEERATAWATCHAI, H.; KANOKPANONT, S.; DAMRONGSAKKUL, S. Influences of physical and chemical crosslinking techniques on electrospun type a and b gelatin fiber mats. Int. J. Biol. Macromol, v.47, n.4, p.431-438, 2010.
SCHLUMPF, M.; SCHMID, P.; DURRER, S.; CONSCIENCE, M.; MAERKEL, K.; HENSELER, M.; GRUETTER, M.; HERZOG, I.; REOLON, S.; CECCATELLI, R.; FAASS, O.; STUTZ, E.; JARRY, H.; WUTTKE, W.; LICHTENSTEIGER, W. Endocrine activity and developmental toxicity of cosmetic uv filters - an update. Toxicology, v.205, n.1-2, p.113-122, 2004.
SHEU, M.T.; HUANG, J.C.; YEH, G.C.; HO, H.O. Characterization of collagen gel solutions and collagen matrices for cell culture. Biomaterials , v.22, n.13, p.1713-1719, 2001.
SILVA, D.G.; SARRUF, F.D.; OLIVEIRA, L.C.D.; ARÊAS, E.P.G.; KANEKO, T.M.; CONSIGLIERI, V.O.; VELASCO, M.V.R.; BABY, A.R. Influence of particle size on appearance and in vitro efficacy of sunscreens. Braz. J. Pharm. Sci, v.49, n.2, p.251-261, 2013.
SPRINGSTEEN, A.; YUREK, R.; FRAZIER, M.; CARR, K.F. In vitro measurement of sun protection factor of sunscreens by diffuse transmittance. Anal. Chim. Acta, v.380, n.2-3, p.155-164, 1999.
STRAUSS, G.; GIBSON, S.M. Plant phenolics as cross-linkers of gelatin gels and gelatin-based coacervates for use as food ingredients. Food Hydrocolloid, v.18, n.1, p.81-89, 2004.
TANAKA, N.; SETSUKO, T.; UTSUMI, I. A new oral gelatinized sustained-release dosage form. J. Pharm. Sci, v.52, n.7, p.664-667, 1963.
TEIXEIRA, V.G.; COUTINHO, F.M.B., GOMES, A.S. Principais métodos de caracterização da porosidade de resinas à base de divinilbenzeno. Quim. Nova, v.24, n.6, p.808-818, 2001.
UGWOKE, M.I.; KINGET, R. Influence of processing variables on the properties of gelatin microspheres prepared by the emulsification solvent extraction technique. J. Microencapsul., v.15, n.3, p.273-281, 1998.
VELASCO, M.V.R.; SARRUF, F.D.; SALGADO-SANTOS, I.M.; HAROUTIOUNIAM-FILHO, C.A.; KANEKO, T.M.; BABY, A.R. Broad spectrum bioactive sunscreens. Int. J. Pharm., v.1/2, p.50-57, 2008.

Publication Dates

Publication in this collection
Dec 2016

History

Received
04 Jan 2016
Accepted
13 Sept 2016

This is an open-access article distributed under the terms of the Creative Commons Attribution License

[1] BABY, A.R.; HAROUTIOUNIAN-FILHO, C.A.; SARRUF, F.D.; TAVANTE-JÚNIOR, C.R.; PINTO, C.A.S.O.; ZAGUE, V.; ARÊAS, E.P.G.; KANEKO, T.M.; VELASCO, M.V.R. Estabilidade e estudo de penetração cutânea in vitro da rutina veiculada em uma emulsão cosmética através de um modelo de biomembrana alternativo. Rev.Bras.Ciênc.Farm.v.44, p.233-248, 2008.

[2] BABY, A.R.; HAROUTIOUNIAN-FILHO, C.A.; SARRUF, F.D.; PINTO, C.A.S.O.; KANEKO, T.M.; VELASCO, M.V.R. Influence of urea, isopropanol and propylene glycol on rutin in vitro release from cosmetic semisolid systems estimated by factorial design. Drug Dev. Ind. Pharm., v.35, p.272-282, 2009.

[3] BIGI, A.; COJAZZI, G; PANZAVOLTA, S.; RUBINI, K.; ROVERI, N. Mechanical and thermal properties of gelatin films at different degrees of glutaraldehyde crosslinking. Biomaterials, v.22, n.8, p.763-68, 2001.

[4] BIGI, A.; COJAZZI, G; PANZAVOLTA, S.; RUBINI, K.; ROVERI, N. Stabilization of gelatin films by crosslinking with genipin. Biomaterials , v.23, n.24, p.4827-32, 2002.

[5] BRESOLIN, T.M.B.; CECHINEL FILHO, V. Ciências farmacêuticas: contribuição ao desenvolvimento de novos fármacos e medicamentos. Itajaí: Editora da Universidade do Vale do Itajaí, 2003.

[6] BRUNETON, J. Elementos de Fitoquímica y de Farmacognosia. Zaragoza: Acribia, 1991.

[7] CATALINA, M.; ATTENBURROW, G.E.; COT, J.; COVINGTON, A.D.; ANTUNES, A.P.M. Influence of crosslinkers and crosslinking method on the properties of gelatin films extracted from leather solid waste. J. Appl. Polym. Sci, v.119, n.4, p.2105-2111, 2011.

[8] CHOY, Y.B.; CHENG, F.; CHOI, H.; KIM, K.K. Monodisperse gelatin microspheres as a drug delivery vehicle: release profile and effect of crosslinking density. Macromol. Biosci, v.8, n.8, p.758-765, 2008.

[9] GAN, C.Y.; CHENG, L.H.; EASA, A.M. Assessment of cross-linking in combined cross-linked soy protein isolate gels by microbial transglutaminase and maillard reaction. J. Food Sci, v.74, n.2, p.141-146, 2009.

[10] HANSON, K.M.; GRATTON, E.; BARDEEN, C.J. Sunscreen enhancement of uv-induced reactive oxygen species in the skin. Free Radical Biol. Med, v.41, n.8, p.1205-1212, 2006.

[11] HAYASHI, K.; TABATA, Y. Preparation of stem cell aggregates with gelatin microspheres to enhance biological functions. Acta Biomater, v.7, n.7, 2797-2803, 2011.

[12] KARTHIKEYAN, S.; RAJENDRA PRASAD, N.; GANAMANI, A.; BALAMURUGAN, E. Anticancer activity of resveratrol-loaded gelatin nanoparticles on NCI-H460 non-small cell lung cancer cells. Biomed. Prev. Nutr, v.3, n.1, p.64-73, 2013.

[13] NAHAR, M.; MISHRA, D.; DUBEY, V.; JAIN, N.K. Development, characterization, and toxicity evaluation of amphotericin b-loaded gelatin nanoparticles. Nanomed-Nanotechnol, v.4, n.3, p.252-261, 2008.

[14] OLIVEIRA, C.A.; PERES, D.D.; GRAZIOLA, F.; BOU-CHACRA, N.A.; ARAUJO, G.L.B.; FLORIDO, A.C.; MOTA, J.P.; ROSADO, C.; VELASCO, M.V.R.; RODRIGUES, L.M.; FERNANDES, A.S.; BABY, A.R. Cutaneous biocompatible rutin-loaded gelatin-based nanoparticles increase SPF of the association of UVA and UVB filters. Eur. J. Pharm. Sci., v.81, p.1-9, 2016.

[15] OLIVEIRA, C.A.; PERES, D.D.; RUGNO, C.M.; KOJIMA, M.; PINTO, C.A.S.O.; CONSIGLIERI, V.O.; KANEKO, T.M.; ROSADO, C.; MOTA, J.; VELASCO, M.V.R.; BABY, A.R. Functional photostability and cutaneous compatibility of bioactive UVA sun care products. J. Photoch. Photobio. B, v.148, p.154-159, 2015.

[16] PATEL, M.; JAIN, S.K.; YADAV, A.K.; GOGNA, D.; AGRAWAL, G.P., Preparation and characterization of oxybenzone-loaded gelatin microspheres for enhancement of sunscreening efficacy. Drug Deliv., v.13, n.5, p.323-330, 2006.

[17] PERES, D.D.; OLIVEIRA, C.A.; COSTA, M.S.; TOKUNAGA, V.K.; MOTA, J.P.; ROSADO, C.; CONSIGLIERI, V.O.; KANEKO, T.M.; VELASCO, M.V.R.; BABY, A.R. Rutin increases critical wavelength of systems containing a single UV filter and with good skin compatibility. Skin Res. Technol., v.22, p.325-333, 2016.

[18] RABANEL, J.M.; BANQUY, X.; ZOUAOUI, H.; MOKHTAR, M.; HILDGEN, P. Progress technology in microencapsulation methods for cell therapy. Biotechnol. Progr, v.25, n.4, p.946-963, 2009.

[19] RATANAVARAPORN, J.; RANGKUPAN, R.; JEERATAWATCHAI, H.; KANOKPANONT, S.; DAMRONGSAKKUL, S. Influences of physical and chemical crosslinking techniques on electrospun type a and b gelatin fiber mats. Int. J. Biol. Macromol, v.47, n.4, p.431-438, 2010.

[20] SCHLUMPF, M.; SCHMID, P.; DURRER, S.; CONSCIENCE, M.; MAERKEL, K.; HENSELER, M.; GRUETTER, M.; HERZOG, I.; REOLON, S.; CECCATELLI, R.; FAASS, O.; STUTZ, E.; JARRY, H.; WUTTKE, W.; LICHTENSTEIGER, W. Endocrine activity and developmental toxicity of cosmetic uv filters - an update. Toxicology, v.205, n.1-2, p.113-122, 2004.

[21] SHEU, M.T.; HUANG, J.C.; YEH, G.C.; HO, H.O. Characterization of collagen gel solutions and collagen matrices for cell culture. Biomaterials , v.22, n.13, p.1713-1719, 2001.

[22] SILVA, D.G.; SARRUF, F.D.; OLIVEIRA, L.C.D.; ARÊAS, E.P.G.; KANEKO, T.M.; CONSIGLIERI, V.O.; VELASCO, M.V.R.; BABY, A.R. Influence of particle size on appearance and in vitro efficacy of sunscreens. Braz. J. Pharm. Sci, v.49, n.2, p.251-261, 2013.

[23] SPRINGSTEEN, A.; YUREK, R.; FRAZIER, M.; CARR, K.F. In vitro measurement of sun protection factor of sunscreens by diffuse transmittance. Anal. Chim. Acta, v.380, n.2-3, p.155-164, 1999.

[24] STRAUSS, G.; GIBSON, S.M. Plant phenolics as cross-linkers of gelatin gels and gelatin-based coacervates for use as food ingredients. Food Hydrocolloid, v.18, n.1, p.81-89, 2004.

[25] TANAKA, N.; SETSUKO, T.; UTSUMI, I. A new oral gelatinized sustained-release dosage form. J. Pharm. Sci, v.52, n.7, p.664-667, 1963.

[26] TEIXEIRA, V.G.; COUTINHO, F.M.B., GOMES, A.S. Principais métodos de caracterização da porosidade de resinas à base de divinilbenzeno. Quim. Nova, v.24, n.6, p.808-818, 2001.

[27] UGWOKE, M.I.; KINGET, R. Influence of processing variables on the properties of gelatin microspheres prepared by the emulsification solvent extraction technique. J. Microencapsul., v.15, n.3, p.273-281, 1998.

[28] VELASCO, M.V.R.; SARRUF, F.D.; SALGADO-SANTOS, I.M.; HAROUTIOUNIAM-FILHO, C.A.; KANEKO, T.M.; BABY, A.R. Broad spectrum bioactive sunscreens. Int. J. Pharm., v.1/2, p.50-57, 2008.

Process	Process yield (%)
Obtaining	74.8 ± 8.5
Crosslinking with glutaraldehyde	82.0 ± 13.3
Crosslinking with rutin	85.1 ± 9.1

Samples	Surface area (m²/g)	Pore size (nm)	Pore volume (x10^-3 cm³/g)	True density (g/cm³)	d (0.1)	d (0.5)	d (0.9)	Average diameter
Gelatin	0.8	2.6	1.1	1.4	104.5 ± 1.3	350.1 ± 0.1	467.1 ± 0.1	329.1 ± 0.2
M0	4.4 ^a ± 0.1	3.0 ^a ± 0.1	6.5 ^a ± 0.1	1.6 ^a ± 0.0	1.1 ^a ± 1.0	6.4 ^b ± 1.6	29.4 ^b ± 4.6	11.2 ^b ± 1.9
MG	1.8 ^b ± 0.4	3.4 ^a ± 0.1	3.4 ^b ± 0.1	1.6 ^a ± 0.1	2.7 ^a.b ± 0.3	18.1 ^a ± 2.0	52.1 ^a ± 2.0	23.6 ^a ± 1.6
MR	4.1 ^a ± 1.2	3.0 ^a ± 0.3	5.9 ^a ± 0.1	1.6 ^a ± 0.1	4.8 ^b ± 1.0	18.4 ^a ± 0.6	34.7 ^a ± 3.3	19.7 ^a ± 1.6

Dispersions	Sun protection fator (in vitro SPF)	λ_C (nm)	UVA / UVB ratio
A	1.0 ^a ± 0.1	378.6 ^a ± 9.6	0.8 ^a ± 0.2
B	1.1 ^a ± 0.2	383.0 ^a ± 10.0	0.8 ^a ± 0.3
C	1.0 ^a ± 0.0	377.5 ^a ± 20.0	0.8 ^a ± 0.4
D	1.0 ^a ± 0.0	386.0 ^a ± 6.6	0.8 ^a ± 0.3
E	1.0 ^a ± 0.0	374.6 ^a ± 12.4	0.6 ^a ± 0.2
F	2.8 ^b ± 0.3	354.7 ^b ± 1.2	0.5 ^b ± 0.0
G	4.1 ^c ± 0.5	354.5 ^b ± 1.9	0.5 ^b ± 0.0
H	3.7 ^b.c ± 0.3	356.1 ^b ± 1.7	0.5 ^b ± 0.0
I	3.3 ^b.c ± 0.3	354.9 ^b ± 0.5	0.5 ^b ± 0.0
J	3.8 ^b.c ± 0.5	356.3 ^b ± 0.7	0.5 ^b ± 0.0
K	6.4 ^d ± 0.4	328.3 ^d ± 2.2	0.1 ^d ± 0.0
L	8.4 ^e ± 1.0	327.3 ^d ± 2.9	0.1 ^d ± 0.0
M	6.8 ^d.e ± 0.6	328.7 ^d ± 3.4	0.1 ^d ± 0.0
N	7.7 ^d.e ± 0.3	327.6 ^d ± 2.1	0.1 ^d ± 0.0
O	7.3 ^d.e ± 0.8	328.0 ^d ± 3.7	0.1 ^d ± 0.0
P	10.1 ^f ± 4.1	351.3 ^f ± 1.7	0.3 ^f ± 0.0
Q	16.2 ^f ± 3.4	350.0 ^f ± 1.1	0.3 ^f ± 0.0
R	10.7 ^f ± 1.1	350.7 ^f ± 0.2	0.3 ^f ± 0.0
S	11.0 ^f ± 2.1	351.2 ^f ± 1.2	0.3 ^f ± 0.0
T	12.4 ^f ± 1.4	350.9 ^f ± 0.9	0.4 ^f ± 0.0

Brasil

Brasil

Gelatin-based microspheres crosslinked with glutaraldehyde and rutin oriented to cosmetics

ABSTRACT

INTRODUCTION

MATERIAL AND METHODS

Obtainment of gelatin microspheres

Crosslinking of gelatin microspheres

Appearance by scanning electron microscopy (SEM)

Determination of extent of crosslinking

Determination of surface area

Determination of true density

Determination of particle size distribution

In vivo cutaneous compatibility assays

In vitro efficacy determination

Analysis of results

RESULTS AND DISCUSSION

Aspect of microspheres and yield of the processes of preparation and crosslinking

Scanning electron microscopy

Extent of crosslinking

Surface area, Porosity and True Density

Particle size distribution and particle diameters

In vitro cutaneous compatibility assays

Photoprotective activity in vitro: SPF and protection against UVA

CONCLUSION

ACKNOWLEDGMENT

REFERENCES

Publication Dates

History

Components	% w/w
Components	A	B	C	D	E	F	G	H	I	J	K	L	M	N	O	P	Q	R	S	T
Mineral oil	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0	50,0
Crodabase^(r) SQ	45,0	45,0	45,0	45,0	45,0	44,0	39,0	39,0	39,0	39,0	42,5	37,5	37,5	37,5	37,5	36,5	31,5	31,5	31,5	31,5
Gelatin	-	5,0	-	-	-	-	5,0	-	-	-	-	5,0	-	-	-	-	5,0	-	-	-
M0	-	-	5,0	-	-	-	-	5,0	-	-	-	-	5,0	-	-	-	-	5,0	-	-
MG	-	-	-	5,0	-	-	-	-	5,0	-	-	-	-	5,0	-	-	-	-	5,0	-
MR	-	-	-	-	5,0	-	-	-	-	5,0	-	-	-	-	5,0	-	-	-	-	5,0
BZ3	-	-	-	-	-	6,0	6,0	6,0	6,0	6,0	-	-	-	-	-	6,0	6,0	6,0	6,0	6,0
OCT	-	-	-	-	-	-	-	-	-	-	7,5	7,5	7,5	7,5	7,5	7,5	7,5	7,5	7,5	7,5