Cytotoxicity and UV Light Absorption in Biopolymeric Membranes from Native Vegetation of Mexico

Sustainable processing from native vegetation such as agave, nopal and aloe, is mainly centered on the components of lignin, cellulose, and hemicellulose, defined generally as lignocellulosic. Cytotoxicity of lignocellulosic biopolymer membranes (LBMs) of mucilages of Opuntia ficus-indica, Aloe barbadensis Miller, fructans, and residual Agave tequilana Weber fibers at different concentrations (30, 50 and 70%), was evaluated in contact with human fibroblast cells (ATCC® PCS-201-010), cultured in vitro. Long and short LMBs were formed from the fibrous material. The interaction showed mild cytotoxicity according to ISO 10993-5: 2009. Cytotoxic activity demonstrated in the presence of fibroblasts implied a maximum cytotoxicity of close to 46% and a minimum of 7% in LBMs. UV light absorption results of the large fiber LMBs showed the highest prevention of passage of light, having a protective effect mechanism of delaying the response of hypersensitivity as a result of exposure to UV radiation. The morphology and structure were characterized using SEM, FT-IR, and image texture analysis. According to the LBMs reactivity measured, the feasible uses of these membranes can be suggested as materials for biomedical applications over a short period of time, with feasibility as a support to provide some beneficial solutions.


Introduction
Native vegetation is all plant species that materialize naturally in a particular habitat and provide essential habitat. These plants have evolved through time adapting to the soil, temperature, nutrients, and weather of their region, being naturally resilient because these are adapted to local conditions. A characteristic native vegetation of Mexico is the agave plant. However, Agavaceas in Mexico are characterized by the large-scale generation of residuals from alcoholic beverage production processes. Due to this, it is of great interest to re-use the subproducts. For each ton of bagasse of Agave tequilana Weber, 3.1% of fiber is obtained. In addition to this, Opuntia ficus-indica and Aloe barbadensis Miller, are both species from Mexico [1,2]. The Agave tequilana Weber fibers are mainly composed of cellulose are a specific model for the early recognition of possible cytotoxic effects of potential materials for the development of biocompatible components [20], these were used for cytotoxicity testing and information regarding any potential uncertainties with the tissue response [21]. For cytotoxicity tests ISO 10993-5: 2009 was developed, around the evaluation of materials and devices, regarding their usefulness as biocompatible materials. [22].
There is previous research in the use of natural fibers used as materials for the formation of biopolymeric materials. In a study conducted in Brazil, sisal and coconut fibers with an added emulsion were used as a matrix to produce composite soil. The results of the tests demonstrated that water absorption of sisal fibers is much greater than coconut fibers, depending on the orientation of the fibers within the matrix and their microstructure [23].
In other investigations, polymer compounds reinforced with natural fibers (bamboo, sisal, jute, etc.) have been obtained. These compounds have beneficial properties such as low density and less cost and solidity compared to synthetic compounds, which provides advantages for their use in commercial applications (automotive, buildings, and construction). The use of natural fibers as reinforcement for polymeric compounds introduces a positive effect in the mechanical behavior of polymers. Mohammed et al., 2015 evaluated the properties: mechanical, thermal, energy and moisture absorption. As well as the viscoelastic behaviors, degree of biodegradability of the fibers of the polymeric compounds reinforced with natural fibers by adding coupling agents [24].
In the case of cellulosic substrates, biocomposites were developed in two proportions of hyaluronic acid and cellulose, which showed a variety of morphological and structural changes, as well as biocompatibility results, suggesting their beneficial application in wound care devices [25]. On the other hand, researchers evaluated cellulose compounds in epithelial regeneration focusing on modifications such as topography, water content, and pore structure in combination with other polymers and found applications and positive effects in dermal applications [26].
This work consisted of performing the development and characterization of a method to re-use material manufactured from agave fiber and natural binders in order to provide the sustenance for a possible application of the membranes as support and use in skin care by carrying out a preliminary evaluation of the degree of cytotoxicity. Furthermore, the UV light absorption behavior and other properties such as Scanning Electron Microscope (SEM), stereoscopic microscopy, Fourier transform infrared spectroscopy (FT-IR), and image analysis were determined. The main advantages of this approach are the ease of fabrication, as cross-linking agents come from native vegetation. The preparation of these membranes demonstrates a promising alternative as a dressing material.

Obtaining Fibrous Material
The fibrous material contained in the stem (32.9 brix degrees) was extracted by cutting from the seven-year-old crop of Agave tequilana Weber in the Laboratory of Permaculture and Eco design of Nano-microfibers, with coordinates 19 • 30 52.7" N, 99 • 07 45.2" W, in Mexico City. It underwent a crushing machine process with slow kinetics by passing through mechanical rippers at a temperature of 80 • C and a constant pressure of 300 MPa for 6 h. It was then washed with water at room temperature until the last wash was neutral (no sugars).
This was dried in a tray dryer at a temperature of 60 • C for 24 h until a relative humidity content of 5% was obtained. Half of the dry product was milled in a mechanical Pulvex ® (mill of grains) blade mill until the size of the fibers was reduced to between 1 and 4 cm in length, which are called long fibers (FL). The other half were subjected to a further grinding, passing the fiber through a sieve (N. 150) until a particle size between 10 and 15 µm was obtained. They were then heated on stove at 37 • C for 24 h until a relative humidity content of 5% was obtained, and they are named curt fibers (FC). Vegetative material from the five-year harvest of Opuntia ficus-indica from the laboratory of permaculture and eco design of nano microfibers, with coordinates 19 • 30 52.7" N, 99 • 07 45.2" W, in Mexico City was used. Cladodes were selected, homogeneous in size (between 40 and 55 cm in length) and age. The spines were removed, cut into pieces, and then crushed in an industrial blender and homogenized in aqueous medium at a 1:5 ratio in a mixer with rotating blades for 3 min. The mixture was subjected to a heating process for 20 min at 85 • C at approximately 3500 rpm (pH 4-4.5). This mixture was filtered through an N.150 sieve to later be centrifuged (Beckman, Avanti J-25) at 4000 rpm for 15 min. The dowels, which are along its edges, were removed before cutting the leaves. The leaves were washed with distilled water to remove dirt from the environment. The epidermis was carefully separated from the parenchyma using a scalpel. This pulp was washed with distilled water and then it was crushed in an industrial blender and homogenized in aqueous medium at a ratio of 1:5 in a mixer with rotating blades for 3 min. The mixture was subjected to a heating process for 20 min at 85 • C at approximately 3500 rpm (pH 4-4.5). This mixture was filtered through an N.150 sieve to later be centrifuged (Beckman, Avanti J-25) at 4000 rpm for 15 min.

Obtaining Fructans
Agave fructans were extracted using a pilot modular system for the extraction of agave fructans (Patent No. MX/E/2015/087857, "Modular system and process to obtain several products from agave fructans") designed by CeProBi researchers. Through this system, a liquid extract with a high content of fructans was obtained, which was subsequently dehydrated by spray drying, with a rotary disk dryer, whose inlet and outlet temperature was 200 and 70 • C, respectively, for 24 h, until the moisture content was 5%.

Obtaining Lignocellulosic Biopolymer Membranes
Lignocellulosic biopolymer membranes (LBMs) were prepared with different compositions of the fibrous material. To define the concentrations of the fibrous material, a sweep from 5 to 90% of the concentration was performed in the UV radiation absorption processes, defining significant differences at 30, 50 and 70% of fibrous material at the different wavelengths.
For the conformation of the LBMs (Table 1), mixtures were made with Opuntia ficus-indica mucilage; Aloe barbadensis Miller mucilage as binder and emulsifier agents [27]; fructans were added as stabilizer, humectant, and gelling agents [28]; and fibrous material (FL and FC), that give different characteristics to the porous surface [29]. The mixture was kept under constant magnetic stirring while heating to 80 • C for 10 min. The suspension was emptied into Petri dishes and dried at 60 • C for 48 h in an oven (VWR Scientific Products) to obtain different LBMs, with an average thickness of 0.3422 mm. For the cytotoxic evaluation, a cell line of normal primary dermal fibroblast was used: human, neonatal (HDFn) ATCC ® PCS-201-010. The cell line was provided by the stem cell biology laboratory of the Faculty of Medicine of the Autonomous University of the State of Morelos, México. The cells were cultured, according to the ISO 10993-5:2009 protocol, in 2 mL of DMEM culture medium, which contains glucose, L-glutamine, sodium pyruvate, sodium bicarbonate, and sterile-filtered liquid, in 24-well plates at a density of 10,000 cells/cm 2 . Human fibroblast cultures were propagated to obtain a semi-confluent density of 80% (4 days of culture). Subsequently, a sample of LBMs, previously bored to 6 mm Ø and sterilized with ultraviolet (UV) light for 30 min on each side, were isolated from moisture and covered with foil until used. They was deposited in Transwell-COL collagen-coated polytetrafluoroethylene (PTFE) inserts with 0.4 µm pore size and 6.5 mm diameter ( Figure 1). The test was carried out in triplicate. For the cytotoxic evaluation, a cell line of normal primary dermal fibroblast was used: human, neonatal (HDFn) ATCC ® PCS-201-010. The cell line was provided by the stem cell biology laboratory of the Faculty of Medicine of the Autonomous University of the State of Morelos, México. The cells were cultured, according to the ISO 10993-5:2009 protocol, in 2 mL of DMEM culture medium, which contains glucose, L-glutamine, sodium pyruvate, sodium bicarbonate, and sterile-filtered liquid, in 24-well plates at a density of 10,000 cells/cm 2 . Human fibroblast cultures were propagated to obtain a semi-confluent density of 80% (4 days of culture). Subsequently, a sample of LBMs, previously bored to 6 mm Ø and sterilized with ultraviolet (UV) light for 30 min on each side, were isolated from moisture and covered with foil until used. They was deposited in Transwell-COL collagen-coated polytetrafluoroethylene (PTFE) inserts with 0.4 µm pore size and 6.5 mm diameter ( Figure 1). The test was carried out in triplicate.

Cytotoxicity Test
The first evaluation was after 24 h of culture, allowing the adherence with the six different LBMs of 30 (FC30), 50 (FC50), and 70% (FC70) long fiber and 30 (FL30), 50 (FL50) and 70% (FL70) short fiber in indirect contact using a transwell insert holder, so they did not have direct contact with the cells. Along with the addition of membranes and in order to have a positive control of oxidative stress, three culture wells with only cell culture medium were also subdued. The control group consisted of cells in culture medium, with normal growth to the same semi-confluent density and without exposition to the membranes. The cell densities used in each 24-well plate were the suggested: 10,000 in indirect contact using a transwell insert holder, so they did not have direct contact with the cells. Along with the addition of membranes and in order to have a positive control of oxidative stress, three culture wells with only cell culture medium were also subdued. The control group consisted of cells in culture medium, with normal growth to the same semi-confluent density and without exposition to the membranes. The cell densities used in each 24-well plate were the suggested: 10,000 cells/cm 2 cells). The test was carried out in triplicate. Membranes were removed one by one with dissecting forceps, and once this process was completed, cell cultures were fixed with 10% trichloroacetic acid for 1 h, followed by washing five times with distilled water at 4 • C, and dried at room temperature for 12 h.

Staining with Sulphordamine B (SRB)
Staining with SRB is a determination of the total protein content by staining with SRB (sulphordamine B), which is a bright pink aminoxantane dye with two S0 3 sulfonic groups, which under moderately acidic conditions increase their affinity for the basic amino acids of proteins, electrostatically and selectively fixing them [30]. After 24 h of applying the treatment on the cells, the culture medium was extracted. Subsequently, 100 µL of 10% trichloric acetic acid (TCA) solution was added to each well and incubated for one hour at 4 • C. After the incubation time, the TCA was discarded and each plate was washed five times with 500 µL of distilled water at 4 • C, and at the end of the washings, it was allowed to dry for 12 h. Next, 300 µL of SRB solution was added to each well by incubating it for 30 min at room temperature.
Subsequently, the dye was removed by five washes per plate with 300 µL of 1% acetic acid. Finally, 100 µL of 10 mM base TRIS solution, pH 10, was added. Finally, the 24-well plates were placed for the quantification absorbance in a spectrophotometer (Synergy 2 BioTek). The absorbance plate test compares the reader's optical density to wavelength measurements from 200 to 999 nm in 1-nm increments.
To avoid the appearance of false positives in this assay because of the SRB dye binding to the amino acid residues of the proteins, transwell inserts were used within the 24-well plate, which allows the exchange of molecules between the different LBMs and the culture medium, since they have pores with a diameter of 0.4 µm, and also prevents the remains of the material being evaluated from adhering to the surface of the culture plates, thus preventing the formation of false positives due to their staining.

Viability
The viability of the cell culture exposed to the different LBMs, was compared against the control group. It was made using a Synergy 2 plate reader by recording absorbances. A reduction in the amount of protein in the sample results in a reduction in the number of living cells. This reduction is directly correlated with the amount of SRB formed by fluorescence. The viability [22] was determined and compared to the blank with the following equation: where: OD 570e is the average OD of the respective groups that were in contact with different LBMs. OD 570b is the average OD of all the wells of the control group. All values are final ODs after subtraction of background absorbance.
A tested LBM has cytotoxic potential when the cell culture viability decreases to <70% in comparison with the control group, which was set at 100% viability [22]. The average viability percentages were obtained for each concentration of fibrous material based on the outcomes of the three repetitions of each experiment [22]. The compared data were the cytotoxicity potentials obtained from different plate readings on the spectrophotometer and the fluorescence intensity by staining the cells. This established differences in response between the cell viability of each membrane, in the different samples evaluated, and determined if the methods provide comparable results in the viability of the exposed cells in the LBMs versus the viability of the cultures of cells of the control group.

Qualitative Evaluation
Culture wells were examined microscopically with fixed cells. Changes in general morphology, vacuolization, cell lysis, and LBM integrity were evaluated. The change in normal morphology was performed descriptively and numerically (Table 2), in accordance with the qualitative morphological classification of cytotoxicity in the standard [22]. Table 2. Degree of reactivity according to cell conditions.

Grade
Reactivity Cell Conditions 0 None Discrete intracytoplasmic granules, without cell lysis, without reduction of cell growth.

Slight
No more than 20% of the cells are round, freely bound and without intracytoplasmic granules, without changes in morphology; occasional lysed cells; a slight growth inhibition is observed.

Measured
No more than 50% of the cells are uniform, without intracytoplasmic granules, without extensive cell lysis; no more than 50% inhibition of observable growth.

Moderate
No more than 70% of the cell layers contain rounded cells or these are lysed; cell layers are not completely destroyed, but more than 50% growth inhibition is observed.

4
Severe Almost complete or complete destruction of cell layers.

Environmental Scanning Electron Microscopy
The surface of the obtained short and long LBMs was observed by means of environmental scanning electron microscopy (Zeiss, Evo LS10, Munich, Germany), to determine the distribution and conformation of the dressing.

Fourier Transform Infrared Spectroscopy
The functional groups of the short and long mixtures of the obtained LBMs were determined using ATR-FTIR. A Shimadzu spectrophotometer (IR Affinity model, Shimadzu, Japan), equipped with ATR (attenuated total reflection), was used with the following scanning parameters: zinc selenium crystal, % transmittance, number of scans: 100, 4 cm −1 resolution. The region that was used for the analysis was 500-4000 cm −1 . The dried and sterilized membranes were mounted on the equipment sample plate. From the transmittance spectra, it was possible to identify interactions between the used biopolymers.

Adsorption of Ultraviolet Radiation
The UV radiation adsorption of the different LMBs was determined using an EA30-Extech Lux meter (8-volt UVL-28 UV lamp). The amount of light transmitted on the different exposed membranes was quantified for about 2 s. The LBMs were exposed to different wavelengths, 254, 302, and 365 nm, covering the entire spectrum of UV light radiation, and the tests were performed in triplicate for each concentration. The lux meter detector was completely covered and the lamp was placed 24 cm away from the detector, inside a black box to eliminate external light.

Image Texture Analysis
Stereoscopic surface microscopy can be analyzed as a set of rectangular images Nz (layers) with Nx pixels in the horizontal direction and Ny pixels in the vertical direction. The digital value of each pixel is quantified to Ng gray levels: Lx = {0, 1, . . . , Nx -1}, Ly = {0, 1, . . . , Ny -1}, and Lz = {0, 1, . . . , Nz -1} with domains X, Y, and Z. In addition, G {0, 1, . . . , Ng -1} is the set of Ng gray levels. The set Lx × Ly × Lz is the set of pixels of the images ordered by their column-row-layer designations. The images can be represented as a function that assigns some digital value in G to each pixel in Lx × Ly × Lz; I: Lx × Ly × Lz -G [31]. Therefore, an image can be represented as a function, which assigns various shades of gray for each pixel or set of pixels, and from this information you can characterize the texture of an image [32].
In a two-dimensional gray level histogram for a pair of pixels (reference pixel and neighbor), this matrix approximates the probability of joint distribution of a pair of pixels [33].
The texture is quantified by a set of continuous variables, which describes the local spatial arrangement of reflectance values. Texture measurements describe quantitatively the relationships among the Nz values of the neighboring pixels. The result is a continuous measurement of spatial information that can be used for further processing. Spatial relationships are not necessarily correlated with the spectral data for a given class, and the inclusion of a measure for them improves the accuracy of the classification [34].
The second angular momentum (SMA) or energy parameter measures the textural homogeneity of the image and is a parameter opposite to entropy. The contrast, which is also known as variance or inertia, is a measure of the local variations of the grayscale values of the image pixels. Entropy, which measures the disorder or randomness of the images and characterizes the texture of the image, is an indication of the complexity within the image. Therefore, complex images will have high entropy values [35].
Finally, the fractal dimension performs a description of irregular objects. This refers to the description of irregular geometry or fragmented forms of natural characteristics, as well as other complex objects that traditional Euclidean geometry cannot analyze [36]. It is an ideal tool to measure the roughness/texture of an image [37].
Image texture analysis (ATI) was used to characterize quantitatively the surface microstructure of different LBMs. Five study parameters were obtained: fractal dimension (DFT), energy (or second angular moment), contrast and entropy. All images obtained from microscopy (ESEM) were converted to grayscale images. Subsequently, algorithms of the gray level co-occurrence matrix (GLCM) and shifting differential box counting (SDBC) were applied to obtain texture parameters from grayscale images [38]. All image processing was performed using the Image J v1.34 software program. Five texture parameters were extracted from images obtained from microscopy techniques with the GLCM texture plug-in included in the Image J software program, as well as the SDBC plug-in for calculating the fractal dimension (DFT).
The values of the different parameters obtained were averaged with their respective standard deviations (average ± standard deviation), obtained from equations [30] for the texture parameters extracted from grayscale SEM images. Statistical values were obtained using one-way analysis of variance (ANOVA) followed by the multiple comparison test with Minitab v.15 statistical software. Significant differences were considered when p ≤ 0.05. The graphs and equations of the results were generated using SigmaPlot v.11 software (Systat Software Inc., San Jose, CA, USA).

Quantitative Evaluation
The data presented represent the average of three repetitions of LBMs cytotoxicity assays using the SRB method, and the error bars indicate the standard deviation ( Figure 2). The standard deviation remains with little dispersion in all samples and the cytotoxic effect is found in acceptable limits. If the viability is reduced to <70% of the control; it had a cytotoxic potential [22], with the exception of the SF30 membrane, with a cytotoxicity of 64.64%. All other samples showed values higher than 70% (Table 3). The different membranes showed a concentration-response relationship since cytotoxicity increased gradually with increasing concentration of the fibrous material. The result of the one-way ANOVA test shows ( Table 3) that there is no significant difference between the cell viability and the different treatment conformations at probability value (p > 0.05). Cytotoxicity evaluations performed in LBMs, for both LF and SF, at different concentrations were shown to have mild cytotoxic activity [22]. Using an average of the three evaluations of all the LBMs, an acceptable behavior of obtained results according to ISO: 10993-5:2009 is observed. A cytotoxic viability behavior of 64.64 and 77.65%, respectively, is observed in the sieved dressings FC30 and FL50. However, the SF70 sample reaches 93.52% cell viability-the lower the agavaceous load, the lower cell viability. On the other hand, the LBMs without screening have a downward Larger particles have a smaller surface area and lower porosity among the particles, in contrast to small particles that have a larger specific surface area with less porosity within it [39]. Since LBMs have a greater specific area with screened fibers, because of the particle size, they are provided with a better distribution, which leads to better cell growth.

Qualitative Evaluation
The morphology change is shown descriptively and numerically (Table 4), according to the qualitative morphological classification of cytotoxicity of extracts (Table 2) [22]. Figure 3 shows the micrographs with an inverted microscope (Nikon eclipse ts100, Tokyo, Japan) at 10× magnification of the different fibroblast culture media evaluations of all the LBMs.    The different membranes showed a concentration-response relationship since cytotoxicity increased gradually with increasing concentration of the fibrous material. The result of the one-way ANOVA test shows ( Table 3) that there is no significant difference between the cell viability and the different treatment conformations at probability value (p > 0.05).
Cytotoxicity evaluations performed in LBMs, for both LF and SF, at different concentrations were shown to have mild cytotoxic activity [22]. Using an average of the three evaluations of all the LBMs, an acceptable behavior of obtained results according to ISO: 10993-5:2009 is observed. A cytotoxic viability behavior of 64.64 and 77.65%, respectively, is observed in the sieved dressings FC30 and FL50. However, the SF70 sample reaches 93.52% cell viability-the lower the agavaceous load, the lower cell viability. On the other hand, the LBMs without screening have a downward behavior with FL30, FL50, and FL70, showing a cell viability of 93.18, 85.66, and 71.09%, respectively. The lower the agavaceous load, the greater the cell viability, which could indicate that the screening process could reduce the concentration of some types of toxic contaminant (Figure 2).
Larger particles have a smaller surface area and lower porosity among the particles, in contrast to small particles that have a larger specific surface area with less porosity within it [39]. Since LBMs have a greater specific area with screened fibers, because of the particle size, they are provided with a better distribution, which leads to better cell growth.

Qualitative Evaluation
The morphology change is shown descriptively and numerically (Table 4), according to the qualitative morphological classification of cytotoxicity of extracts (Table 2) [22]. Figure 3 shows the micrographs with an inverted microscope (Nikon eclipse ts100, Tokyo, Japan) at 10× magnification of the different fibroblast culture media evaluations of all the LBMs. Table 4. Morphological conditions of cell cultures.

Grade
Reactivity Cell Conditions

Slight
No more than 20% of the cells are round, freely bound and without intracytoplasmic granules, without changes in morphology; occasional lysed cells; a slight growth inhibition is observed.

Environmental Scanning Electron Microscopy
In Figure 4, the surfaces of the different screened and unscreened LBMs are shown at 30,50,70% fibrous material, respectively. It is evident that membranes show completely different surface morphologies. ESEM micrographs of the longitudinal sections of the LBMs show the conformation between natural binders and lignocellulosic materials (fiber matrix), forming porous structures.  Figure 5 shows the FTIR spectra of different LBMs where the detection of phenol-OH corroborates the presence of the conjugation in the molecular structure of the components of the LBMs, attributing to them the absorption potential of UV radiation.  Figure 5 shows the FTIR spectra of different LBMs where the detection of phenol-OH corroborates the presence of the conjugation in the molecular structure of the components of the LBMs, attributing to them the absorption potential of UV radiation.

Fourier Transform Infrared Spectroscopy
An analysis of the spectra was performed and identified chemical groups in different frequency ranges are shown in Table 5. Appl. Sci. 2020, 10, x FOR PEER REVIEW 12 of 21 An analysis of the spectra was performed and identified chemical groups in different frequency ranges are shown in Table 5.

Adsorption of Ultraviolet Radiation
UV absorption profiles at different wavelengths. The percentage of UV light absorbance in FL membranes was between 51.56% and 82.45%. The FL70 membrane had the highest value. The absorbance activities of the LBM FC had absorbances between 29.43% and 52.01%. The lowest value was shown by the FC 30% mixture.
LBMs with long fibrous material exhibited better UV light absorbance, indicating better material distribution compared to LBMs with FC material. It is observed that membranes with a higher content of fibrous material can prevent the passage of UV light towards the lux meter, which increases the absorbance intensity.
The different membranes showed a concentration-response relationship since the UV absorbance increased gradually with increasing concentration of the fibrous material. The result of the one-way ANOVA test shows that there is no significant difference among different wavelengths, but in the conformation, they are significantly different at p-value (p > 0.05), as is shown in Table 6.

Image Texture Analysis
The texture of the images was analyzed by studying the spatial dependence of the pixel values represented by a coincidence matrix Pd, θ with entry in Pd, θ (i, j) is the frequency or relative distance for two pixels (d) in the direction θ that has i and j values, respectively. These parameters were calculated at a pixel pitch "d" equal to 1 and with a displacement angle "θ" of 0 • [40]. Table 7 shows the results of the study parameters fractal dimension (DFT), energy (or second angular moment), contrast and entropy.
The co-occurrence matrix is a frequency matrix with which a pixel with a gray level (i) appears in a specific space relationship with another gray level pixel (j). The concurrence matrices are second order measures because they consider pairs of neighboring pixels, separated by a distance d and at a certain angle. Therefore, the occurrence matrices can reveal certain properties in the spatial distribution of the grays in the texture of the image [41].
A fractal entropy/dimension ratio was also calculated. This correlation between entropy and the fractal dimension is inverse: the higher the value of the fractal dimension, the lower the value of the entropy, that is to say, the more homogeneous the image is. This relationship was estimated as the ratio of the entropy values divided into the fractal dimension values calculated from the same image [42]. Therefore, higher values of the entropy/fractal dimension relationship will be related to images with a high degree of complexity and roughness, while low values may be associated with simple and smooth images. Thus, an adequate correlation is shown among the fiber load content parameters of the different LBMs.  The co-occurrence matrix is a frequency matrix with which a pixel with a gray level (i) appears in a specific space relationship with another gray level pixel (j). The concurrence matrices are second   The co-occurrence matrix is a frequency matrix with which a pixel with a gray level (i) appears in a specific space relationship with another gray level pixel (j). The concurrence matrices are second   The co-occurrence matrix is a frequency matrix with which a pixel with a gray level (i) appears in a specific space relationship with another gray level pixel (j). The concurrence matrices are second   The co-occurrence matrix is a frequency matrix with which a pixel with a gray level (i) appears in a specific space relationship with another gray level pixel (j). The concurrence matrices are second   The co-occurrence matrix is a frequency matrix with which a pixel with a gray level (i) appears in a specific space relationship with another gray level pixel (j). The concurrence matrices are second  The co-occurrence matrix is a frequency matrix with which a pixel with a gray level (i) appears in a specific space relationship with another gray level pixel (j). The concurrence matrices are second ( a, b, c ) values (average ± standard deviation, n = 5) in a column with the different letters show significant differences (p < 0.05).

Assessment of Cytotoxicity According to ISO: 10993-5: 2009
Quantitative and Qualitative Evaluation Cytotoxicity assays performed on the FC and FL membranes at different concentrations showed that almost all evaluated LBMs have an acceptable viability. Only two membranes were below the viability threshold, FL70 (61.13%) and FC30 (62.12%), according to ISO: 10993-5: 2009. The FC30 mixture showed the lowest viability percentage of the LBMs evaluated, reaching 62.12%, while the FC70 sample showed the highest percentage of viability (80.84%). However, due to sample size and media volume as well as direct contact and lack of evidence of adherence, this would be a preliminary in vitro evaluation.
In stereotypically observed micrographs (Figure 2) of the different cytotoxicity evaluations, the fibroblast culture media are observed in a typical arrangement, in the form of a spindle with a distance growth similar to that of the control or blank in the cases of FC samples. The zone of inhibition and minimization of growth was less obvious in the case of FC30 and FC50.
For the FL50 and FL70 membranes, a large number of many devitalized cells are observed in the vicinity of the material, as well as small areas of inhibition. In this case, the cell is adopting a contracted form, which would indicate a low adhesion with the scaffolding material. Clear differences are observed among the morphologies adopted by the cells in these samples, leading to the conclusion that cell adhesion depends on the physicochemical characteristics of the surface of the material [43]. Lignocellulosic fibers have hygroscopic properties [44]. This is consistent with many results in which different cell lines showed variable adhesion based on surface wettability [45]. Cells have been considered to generally adhere better to moderately hydrophilic surfaces compared to hydrophobic or hydrophilic ends [46].
The qualitative cytotoxic behavior was classified as mild reactivity since no more than 20% of the cells are round, freely bound and without intracytoplasmic granules, and these do not show changes in morphology (Table 3); a slight inhibition of the growth of occasional lysed cells is observed. LBMs showed considerable swelling due to the absorbed culture medium because of the insert. In the case of the FC30 membrane, there was a deformation and shedding of it. Some results have showed that LBMs do not produce cytotoxic effects in indirect contact with the culture of fibroblast cells in vitro, since no major malformation, degeneration, propagation, or lysis of fibroblast cells was observed according to stereoscopic micrographs [47].
Any cytotoxic effect may be cause for concern. However, it is primarily an indication of the potential for in vivo toxicity, and it cannot be determined necessarily that the device is unsuitable for a given clinical application, based solely on cytotoxicity data [22]. Consequently, the results of in vitro cytotoxicity tests should be viewed in a complementary context of biocompatibility tests performed on these membranes to obtain a more accurate assessment of the biological risk associated with Eastern clinical use [21].

Environmental Scanning Electron Microscopy
The use of ESEM in this study allowed the visualization of LMB FL, which have a very rough and porous structure; they are more irregular and full of fibers, showing wide cavities delimited by fibers. A crossing of the structure with crosses and valleys is observed. The pores were larger with more irregularity in shape. On the other hand, LBM FC show a smoother structure with a more uniform texture, a more regular surface without fibers, and no apparent cavities in the amplification used. In other studies, similar observations were made [48] with Agave and polyethylene fiber composites produced by compression molding.
ESEM micrographs of the longitudinal sections of the LBMs show the conformation between natural binders and lignocellulosic materials (fiber matrix), forming porous structures. These interactions between fibrous material and mucilages is certainly due to the formation of an interwoven network between both biopolymers with similar structural and chemical characteristics [49].
Both conformations show porosity. The LBM FL exhibited a more porous network within the composite matrix. The property of porosity ( Figure 3) in a biomaterial extends the scope of applications. In porous biopolymers, you can find closed (isolated) pores and open (connected) pores. Pore interconnectivity is important for the accessibility of gas, liquid, and particle suspensions [50], and even for the incorporation of cell populations [51]. The pore structure in LBM LF has greater penetrability of substances and possible interactions between compounds, giving it impact characteristics in tissue engineering applications, since the behavior of cell/tissue growth depends on a porous structure [50].
The membranes of short fibers and long fibers are porous materials with micro and nano pores made of natural polymers that are of special interest for medical, cosmetic, pharmaceutical, and other applications where biocompatibility and biodegradability are required [52].

Fourier Transform Infrared Spectroscopy (FTIR)
The absorption peaks between 700 and 650 cm −1 are due to the presence of acetyl groups that grant biological activity. Due to the abundance of hydroxyl groups, when there is cross-linking, a conformational variation of the polymer begins and the polymer may act in such a way that hydroxyl groups are exposed [53], thus showing cross-linking of the membranes. These spectra indicate that obtained LBMs contain a variety of functional groups such as carbonyls, amino acids, hydroxyls, aldehydes, anthraquinones, and effective cross-linking agents [54], which suggests their possible use as an alternative for human topical use.
The absorption band between 1185 and 1045 cm −1 is related to the stretching vibrations of the glycosidic bonds (CO, ether bond) and the pyranoid rings (CC) attributed to the polysaccharides that are part of the pectins of the mucilage [55,56].
Stretch groups = CO were observed from 650 to 1580 cm −1 , indicating the presence of carbonyl compounds, amino acids, and polysaccharides, which coincides with what was reported in [57]. The spectral characteristic bands of the C = C ring are observed at 1608 cm −1 [58].
The stretching of the phenolic OH group in the absorption bands around 3600 and 3200 cm −1 explains the presence of aloe-specific phenols, including flavonoids, flavonols, phenolic anthraquinones, etc. These have application as corrosion inhibitors [59].
Biochemicals are important in the composition of the medicinal attributes of aloe (in addition to enzymes, minerals, amino acids, and some vitamins) [60]. The peaks of the 2900-2970 cm −1 region belong to the stretches that have the stretching links of the CH bond of carbohydrates and a flexion that belongs to the COH, COC bonds, which are characteristic of various oligosaccharides and polysaccharides. The spectrum showed a change in intensity at the peak around 1593, depending on the concentration and whether it was LBM FC or LBM FL, as part of the C = C bonds of the lignin molecules [61].
The band around 3276 cm −1 is mainly related to the vibration of the intramolecular hydrogen bond stretch of the amino group of amide A, while the observed band around 2936 cm −1 is assigned to the C-H stretch of the amide B [62].
The band around 3298 cm −1 is mainly related to the stretch bands of the hydroxyl groups, -OH, of carboxylic acids, amino acids, alcohols, and water molecules [58].

Adsorption of Ultraviolet Radiation
From the tested LBMs (Table 6), a UV light absorption potential from 29.43 to 52.01% was observed in FC membranes and a greater potential for UV light absorbance was observed in FL membranes (from 51.56 to 82.45%). This could be due to lower solubility and higher concentration and dispersion of components over the entire surface. This behavior is because secondary metabolites such as flavonoids and esters in plant leaves can absorb UV radiation [63,64]. Presumably, the polyphenols in the Aloe extracts were the main UV absorbing elements. Aloe gel is believed to have a modulating effect on the skin by preventing sunlight from sensitizing the skin, especially in the first 24 h after exposure [65]. This is corroborated in the FT-IR results, by showing bands associated with Aloe.
Since UV radiation penetrates deeply, affecting the dermis, destroying elastic and collagen fibers, and conditioning aging, immune suppression, photoallergic reactions, and phototoxic reactions [66], a full scan of the UV radiation spectrum was performed. However, the behavior of the percentage of UV light absorbance in both the LBM FC and FL do not show significant differences in the evaluation of the near, medium, and far UV spectrum.
Due to its phenolic structure, both lignin and Aloe vera provide the membrane with light-absorbing properties, a natural potential for protection against UV rays, while also presenting stability against thermal oxidation when present in mixtures with other polymers. Previous research has modified the potential of lignocellulosic materials as a component in UV light-blocking membranes [67].
In addition to this, considering the impediment of the passage of UV radiation through the treated fibrous material, this gives the property of sunscreens, which absorb and/or prevent UV radiation from reaching the skin. The link between chronic human skin exposure to the sun and harmful clinical consequences such as photoaging and skin cancers is indisputable. Sun exposure can quickly induce well-characterized and visible clinical consequences, such as sunburn [68].

Analysis of Image Texture
The texture parameters adequately described the texture of the membranes observed with ESEM microscopy (Table 7).
Regarding contrast, LBM FL had the highest values compared to LBM FC. High contrast values measured in the LBM FC are associated with the fibrillar microstructure formed in the membranes. This is attributed to a greater presence of fibers, which causes the contrast values to increase, which indicates a high degree of local variation of pixels within the image [17].
The highest value of the entropy parameter (9.35) corresponded to LBM FC30, which indicates an inhomogeneous surface. The lowest entropy values were obtained with LBM FL30, which means that its surface texture is more homogeneous.
Finally, the fractal dimension values for all LBMs can be associated with the roughness observed in their respective images, where LBM FC30 (more homogeneous surfaces) had the highest fractal dimension value (2.6452), while low values were observed. (2.5261) for LBM FL70 (heterogeneous surfaces). A roughened surface becomes more susceptible to decay and may fragment. Ultraviolet radiation from sunlight initiates a wide variety of chemical changes in surfaces, which causes them to deteriorate, thus losing their usual appearance and also their mechanical properties, as the strength characteristics are degraded [69]. High roughness could reduce UV light transmission through higher light reflection.
The entropy/fractal dimension relationship values for LBM FC30 (3.5496) and FL70 (3.5539) are related to images with a high degree of complexity and roughness, while LBMFC 50 (3.5242) and FC70 (3.5289) have lower values, which are associated with simpler and smoother images. This fact is associated with the structural complexity observed in the topographic images of the LBM surfaces. This was mentioned in previous works, in which the effect of the addition of surfactants and optical parameters on the microstructure of hydroxypropyl methylcellulose films was studied [70]. Using microscopic characterizations, the complexity of the film surfaces was evaluated using the fractal dimension parameter.
Therefore, it can be said that the texture analysis of images is a complementary tool for qualitative studies of the morphologies of the surface of biomaterials, in addition to having the advantages of being an economic and fast tool, which allows the analysis of samples with larger surfaces [30].

Conclusions
FC70 and FL30 membranes were not a significant difference between cell growing control. They had 10,000 cells/cm 2 in the culture of normally growing primary dermal fibroblast. In this study, particle size was relevant in the FC membranes because better distribution and a greater contact area provided a greater interaction with the culture medium, which leads to better cell viability (93.52%) in respect to FL membranes. These results for FC70 and FL30 membranes correlated with the image analysis of texture from the ESEM micrographs and FT-IR spectrophotometry.
The particle size in the FL membranes established a high level of porosity, lower solubility, and a higher solid concentration and dispersion. These aspects were related to greater potential for UV light absorption in FL membranes for all the different wavelengths, 254, 302, and 365 nm, covering the entire spectrum of UV light radiation. However, FL70 membrane had the greatest potential for UV light absorption with 82.45% absorbance at 254 nm of UV light radiation.