Antioxidant and Antiaging Properties of Agar Obtained from Brown Seaweed Laminaria digitata (Hudson) in D-Galactose-Induced Swiss Albino Mice

The present paper explores the antioxidant and antiaging properties of agar extracted from Laminaria digitata (L. digitata) on a D-galactose (D-Gal)-induced mouse model. Experimental mice were divided into four groups: group I comprised of control nontreated mice, group II comprised of D-Gal-induced mice, group III mice were treated with extracted agar after D-Gal induction, and group IV mice were given ascorbic acid as a positive control. Antioxidant enzymes and aging marker proteins declined significantly in group II, whereas they were normal in group III and group IV mice. Expressions of interleukin-1β (IL-1β) in D-Gal-induced mice were significantly enhanced in the liver and brain of the experimental mice, which were otherwise normal in agar-treated mice. Also, IL-6 levels were significantly increased in the liver and reversed in the brain of D-gal mice, while it was regularly in the agar-treated mice. The histopathological analysis of D-Gal-induced mice showed spongiosis and tangles in brain cells, increased fat and decreased collagen contents in the skin, and few dilated sinuses in the hepatic cells. The changes were under control in group III and group IV mice, suggesting the protective effects of agar extracted from L. digitata and ascorbic acid.


Introduction
Aging is a multifactorial natural process of the skin. e changes in the structure and functions of the entire body system are connected to the physical decline associated with aging. Biological aging is rooted in genetics, endocrine, and immune metabolic function factors.
en, environmental influences such as gravity, ultraviolet light exposure, climate, and pollution exacerbate the natural aging process. Several research reports show a correlation between the process of aging and antioxidant functions such as amplified mitochondrial reactive oxygen species (ROS) generation and increased accumulation of oxidant products [1][2][3]. ROS produced by lipid peroxidation has been implicated in the progressive oxidative deterioration of polyunsaturated fatty acids (PUFAs) of the cell membranes [4]. e ROS originates unstable lipid peroxide species incorporating carbonyl group with the end products, namely, reactive aldehydes such as malondialdehyde (MDA) and 4hydroxynonenal (HNE), ultimately causing tissue damage [5,6]. Galactose (Gal) is a monosaccharide that has a similar structure to glucose, differing only in the position of one hydroxyl group. Chronic systemic exposure of rodents to D-Gal causes the acceleration of aging and has been used as an aging agent in experimental models. D-Gal, which is completely metabolized at normal concentrations, is a natural compound in the body. At higher concentrations, however, it converts to aldose and hydrogen peroxide (H 2 O 2 ), a reaction catalyzed by galactose oxidase; conversely, superoxide dismutase (SOD) facilitates the transformation of superoxide anions to H 2 O 2 . e overall increase in ROS leads to disruptions in the activities of macromolecules inside the cell [6]. Cosmetic products are used for human skincare by adolescents. e usage intends to maintain the skin in good condition to shield it from the environment's harsh effects and minimize the aging processes [7,8]. Unfortunately, some of the adverse effects of commercial cosmetics are skin irritation and allergic reactions, swelling, blisters, and surface oozing. On the extreme side, they can cause reproductive toxicity, endocrine disruptions, and cancer to consumers [9,10]. As a result, consumers are on the lookout for more natural sources of skincare products [11]. Seaweeds are rich sources of polysaccharides used as gelling and thickening agents (e.g., alginates, agar, and carrageenan) including some that have become valuable additives in food manufacturing due to their rheological properties. ey are also known to have multiple biological activities, including antioxidant, anticoagulant, antiviral, and immunoinflammatory activities that could find their relevance in nutraceuticals, functional foods, and pharmaceutical applications [12][13][14][15]. Previously, the authors have reported on the antioxidant, anticoagulant, and mosquitocidal properties of water-soluble polysaccharides from green, red, and brown seaweeds [16]. However, to the authors' knowledge, there is no report on the antiaging property of agar. Laminaria digitata belongs to the phylum Ochrophyta, family Laminariaceae, genus Laminaria, and species digitata. Hence, the present study was designed and conducted to evaluate the texture, antioxidant, and in vivo antiaging properties of agar extracted from the brown seaweed L. digitata.

Seaweed Collection and Processing.
Brown seaweeds (L. digitata) were collected from Kanyakumari (Lat 8.0866oN and Long 77.5544oE), Tamil Nadu, India. e samples were identified according to the renowned monograph of Marine Biology, Annamalai University, Tamil Nadu, India. First, the seaweeds were washed in seawater, followed by distilled water, and finally were washed with 70% alcohol to remove microflora and other contaminants on the seaweed surface. Finally, the processed seaweeds were shadow dried and stored at −20°C for further study.

Extraction of Aqueous Polysaccharide.
e dried seaweed samples were blended and ground into a fine powder using a blender. A 5 g of powdered seaweeds was dissolved in 100 ml of Milli-Q water and then autoclaved at 121°C for 1 hour. e water-soluble polysaccharides were filtered through a Whatman no. 1 filter paper to remove debris in the extract and further centrifuged at 5000xg for 15 min at room temperature to eliminate any particulate matter. e solution was kept at room temperature until gelation. e gelated agar was frozen at room temperature overnight. After bleaching, the samples were dried at 60°C overnight [17].

Bleaching of Agar.
e gelated agar seaweed samples were washed with sodium hypochlorite (NaClO). e washing was repeated up to 5 times. After NaClO treatment, it was diluted with H 2 O 2 . e color change has been noted as dark brown to pale yellow color [18].

Food Texture Analyses.
e texture parameters of the extracted agar from L. digitata were measured using the TA.XTplus Texture Analyzer (Stable Microsystems, UK) in back extrusion mode and constituted with a 36 mm cylinder probe. e parameters were set as follows: data acquisition rate: 200 PPS, test speed: 1.0 mm/s, load cell: 5 mm, and distance: 40 mm. e agar from L. digitata was loaded onto the analyzer platform, and the probe was allowed to be flush with the surface. e extract holders were supported by a heavy-duty rig plate attached to the crosshead of the instrument. Upon data acquisition, it was plotted as a graph. e peaks on the graph represent the force at which the probe reaches a maximum penetration depth of 75% of the original agar height. A relaxation of the sample over the twosecond holding period resulted in subsequent decay in force, followed by the withdrawal of the probe to a tracking force of 5 g, thus allowing the sample to "spring back". e maximum force (g) required to penetrate the product was recorded as the hardness, adhesiveness, cohesiveness, springiness, and gumminess of agar from L. digitata. e experiments were run in triplicate, and an average value was statistically reported [19].
e DPPH radical scavenging assay was performed using a 96-well microtiter plate. A 50 µl of 100 µg/ml methanolic DPPH solution was added to 200 µl of different concentrations of agar sample (12.5-100 µg/ml) and mixed with a vortex mixer. Ascorbic acid was used as a standard [20].

H 2 O 2 Scavenging Activity.
e scavenging activity of the agar was determined. A 0.3 ml agar solution was reacted with 600 µl H 2 O 2 40 mM solution. en, it was allowed to stand for 10 min at room temperature. e absorbance of the reaction mixture was measured at 230 nm by a UV spectrophotometer [21].

Total Antioxidant Capacity.
e total antioxidant activities of the agar from the seaweeds were determined. A 0.3 ml agar sample was reacted with 3 ml total antioxidant capacity reagent solution (0.6 M H 2 SO 4 , 28 mM sodium phosphate, and 4 mM ammonium molybdate). e reaction mixture was incubated in a water bath at 95°C for 90 min. e absorbance of the reaction mixture was measured at 695 nm by a UV-visible spectrophotometer [21].

Phosphomolybdate Activity.
e antioxidant activity of agar was evaluated by the green phosphomolybdenum complex formation protocol. A reaction mixture solution was prepared by adding 0.588 ml of sulfuric acid (H 2 SO 4 ), 0.049 g ammonium molybdate, and 0.036 g sodium phosphate. e volume of the final solution was made up to 10 ml with distilled H 2 O. Afterwards, 10 mg of agar was dissolved in 1 ml of dimethyl sulfoxide (DMSO). A 100 μl from the prepared agar sample was taken, and 1 ml of the reagent mixture solution was added to it and then incubated in a boiling water bath at 95°C for 90 min. After 90 min, the absorbance of the solution was read at 695 nm. Ascorbic acid (10 mg/ml DMSO) was used as a standard [22].

Ferric Reducing Antioxidant Power Assay (FRAP Assay).
e working FRAP reagent was produced by mixing 300 mM acetate buffer (pH 3.6), 10 mM 2,4,6-tripyridyl-striazine (TPTZ) solution, and 20 mM FeCl 3 .6H 2 O in a 10 : 1: 1 ratio before use and was heated to 37°C in a water bath for complete dissolution. e blank reading was measured by adding 200 μl of this working solution to the microtiter plate and read at 593 nm using a UV spectrophotometer. e sample reading was calculated by adding 3 ml of the freshly prepared working solution with 100 μl of agar extracts and 300 μl of distilled water and then left for 4 min at room temperature before reading absorbance at 593 nm using a UV spectrophotometer. Here, ferrous sulfate (FeSO 4 ) was used as standard and for calibration in the concentrations of 0 to 1000 μM [23].

Behavioral Studies.
Antiaging was experimentally induced in female Swiss albino mice following the ethical clearance obtained from Institutional Animal Ethics Committee (IAEC4/Alr.No. 23/dated 12.12.17). Extracted agar (100 mg/kg) was suspended in 0.1 M phosphate-buffered saline (PBS) and administered orally using an 18 mm gauge for 42 days. Control mice received regular food and water ad libitum. Ascorbic acid (100 mg/kg)-treated mice served as the positive control. e animals were divided into four groups (Table 1). Food and water intake of all mice groups were measured up to 42 days. e behavioral parameters such as locomotor function, light-dark, hot plate, and rotarod test of experimental mice groups were determined on 0, 2 nd , 4 th , and 6 th weeks [24]. At the end of the experimental period, blood was collected using a 1 ml syringe from the tail vein of the mice. e mice were then sacrificed by halothane inhalation. e liver, brain, kidney, and portions of the skin were dissected, fixed in formalin, and embedded in paraffin, and the morphological changes were detected under the microscope. e rest of the dissected organs were stored in PBS and stored at −20°C for further use.
2.6.1. Locomotor Activity. Locomotor activity was evaluated by placing a mouse into the center of a clear Plexiglas (40 × 40 × 30 cm) open-field arena and allowing the mouse to explore for 5 min. Bright overhead lighting was approximately 500 lux inside the arenas, while noise was present at about 60 dB (INCI Photoactometer, India). e total distance (locomotor activity), movement time (sec), movement speed (cm/sec), and center distance (the distance traveled in the center of the arena) were recorded manually. e center distance was divided by the total distance to obtain a center distance-to-total distance ratio. e center distance-to-total distance ratio can be used as an index of anxiety-related responses. Data were collected at 2, 3, 4 and 5 min intervals over the session [25].

Light-Dark Exploration
Test. Experimental mice were put through the light-dark exploration test, which consists of a polypropylene chamber (44 × 21 × 21 cm) unequally divided into two chambers by a black partition containing a small opening. e large chamber was open and brightly illuminated (800 lx), while the small chamber was closed and dark. White noise was present in the room at approximately 55 dB in the test chamber. Mice were placed on the illuminated side and allowed to move freely between the two chambers for 5 min [26].

Hotplate Test.
e hotplate test was used to evaluate sensitivity to a painful stimulus. Mice were placed on a 55.0°C (±0.3) hotplate, and the latency to the first hind-paw response was recorded. e hind-paw response was either a foot shake or a paw lick [27].

Rotarod Test.
Mice were placed on a rotating rod (INCI Rotarod, India) that accelerated from 4 to 40 rpm. For two consecutive days, four trials were performed per day with 45-60 min intervals between trials. e maximum duration of each trial was 5 min. e time at which the mice fell off the rod was recorded [28].

In Vivo Antiaging Marker Studies
e amount of collagen in the dermis was measured using a Sircol Collagen Assay Kit based on the fact that the Sirius red dye binds to the side chains of the amino acids in collagen [29].

Elastin Measurement.
e amount of elastin in the dermis was measured using a Fastin Elastin Assay Kit based on the fact that the Fastin dye binds to the side chains of the amino acids in elastin [29].

Protein Extraction.
e frozen skin samples were minced and homogenized in 10 volumes of extraction buffer Tris-HCl (pH 7.8).
e homogenate was centrifuged at 9,000xg at 4°C for 15 min, and the supernatant was collected as an extracted protein. e protein concentration of the supernatant was measured by Lowry's method using a DC Protein Assay Kit [29].

Skin Aging Assay.
e levels of elastin, collagen, hyaluronidase, and tyrosinase in skin tissues were examined using the kits procured from Cayman Chemicals, USA [30].

Biochemical Analysis and Histological Analysis.
e blood and tissue levels of reduced glutathione (GSH), hydroxyproline, malondialdehyde (MDA), total protein, and the activities of total SOD, catalase (CAT), and total antioxidant capacity (T-AOC) in the blood and tissues were determined using commercial kits (Sigma, USA). e brain, liver, kidney, and skin of each group of mice were fixed in 10% formalin for 24 h; tissues and dorsal skin samples were dehydrated in various ways before being implanted in paraffin, sectioned thinly, dewaxed, and stained with hematoxylin-eosin [31]. Cross sections were selected from three plates per sample, and the morphological changes were examined under the microscope.

RNA Extraction and Quantitative PCR.
A 100 mg of the brain tissue sample was taken, and 1 ml of TRIzol (Sigma, USA) was added and homogenized. e solution was incubated at room temperature for 30 min and then centrifuged at 12,000 rpm for 10 min. e supernatant was transferred, and after 5 min, about 200 μl of chloroform was added, mixed, and incubated at room temperature for 15 min. en, it was followed by centrifugation at 12,000 rpm for 10 min at 4°C. e upper aqueous layer was transferred, and a 500 μl of isopropanol was added and then incubated at room temperature for 10 min and finally centrifuged at 12,000 rpm for 10 min at 4°C. To the pellet, a 500 μl of 70% ethanol was added, washed (5000 rpm for 5 min at 4°C), and then air-dried. e pellet was then dissolved in 20 μl of diethyl pyrocarbonate (DEPC)-treated water.
e RNA was quantified using a UV spectrophotometer by measuring the ratio of absorbance at wavelengths 260 nm and 280 nm (NanoDrop, ermo Scientific, USA).

Statistical Analysis.
Each test was performed on six mice, and all results were expressed as the mean ± SD. A P value of <0.05 was considered significant. Statistical analysis was performed using the IBM SPSS Statistics for Windows, version 22 (IBM Corp., Armonk, N.Y., USA).

Results and Discussion
Aging is an intricate progression that disturbs the tasks of all organs and tissues and most often has an irreversible impact on their mechanical behavior. e most significant noticeable effects of aging are perceived in the skin and have been broadly investigated for medical and cosmetic resolutions. From a biological appearance, aging is a predictable natural process [24].
About 5 kg of the selected brown seaweed, L. digitata was collected from the Kanyakumari coast, Tamil Nadu, India, and processed. After being shadow dried, the dry weight and the yield of agar from L. digitata were found to be 266.66 g and 20%, respectively. is yield of agar from L. digitata was high when compared to prior results [32]. It has been documented that the difference in agar yield varies from species to species; also, it is dependent on the harvested season. e study results were in accordance with the report of Armisen et al. [33] who pointed out that the yield of agar varied between species and geographical areas of collections. e proximate biochemical composition and food texture analysis of L. digitata are shown in Table 2. e moisture content of the L. digitata was reported to be 22.18%, and among the selected macroelements, sodium (Na) was found to be maximum (1.74%) while phosphorous (P) was found to be minimum (0.03%). Further, the carbon and phosphorous ratio (C : P) was found to be 0.72% of the sample of harvested brown seaweed L. digitata. Moreover, among the selected microelements, the content of copper was observed at maximum (73.41 ppm), and cobalt was recorded at minimum (2 ppm). e elemental content of agar from L. digitata was higher when compared to the report of Fleuerence et al. [34]. e difference in the mineral content could be attributed to the species difference and the method selection for quantification. e overall biochemical analyses findings were in agreement with Fleuerence et al. [34] who had mentioned that the biochemical concentration of seaweed varies according to the factors stated above.
e texture properties such as hardness (234.43 ± 0.60 g), adhesiveness (50.61 ± 0.40 N/mm), cohesiveness (0.825 ± 0.11), springiness (3.250 ± 0.12), and gumminess (2.969 ± 0.10) of agar from L. digitata were maximum when compared to the texture profile analysis of the starch gel prepared from corn [35]. e difference in the texture analysis was due to the monosaccharide composition differences between the species [36], and the results support the present finding that aqueous extract can be easily degraded due to the presence of monomeric chains [37].
Antioxidant activity was determined from the brown seaweed L. digitata. e methods differ in terms of their assay and experimental conditions. e in vitro antioxidant activity of agar from the brown seaweed L. digitata showed higher activity at higher concentrations [35]. e DPPH scavenging activity in agar from brown seaweed was assayed and is presented in Table 3. e 200 µl concentration of agar showed significantly elevated levels of scavenging activity (83.70 ± 3.83%) (P < 0.05) when compared to the concentration of 50 µl (32.68 ± 1.21%).
e standard 100 µl of ascorbic acid was at (62.42 ± 1.11%) DPPH scavenging activity. Hence, the significant variations in the DPPH scavenging abilities of the bioactive compounds isolated from seaweed might be due to variations in the type of extraction and/or differences in the zone of collection of the seaweeds [35]. Aging-induced mice (100 mg/kg D-Gal; s.c. injection) Group 3 Aging-induced (100 mg/kg; s.c.) mice + 100 mg/kg of agar (orally) Group 4 Positive control mice (100 mg/kg D-Gal; s.c.) + ascorbic acid 100 mg/kg (orally)      Table 3. e agar exhibited increased H 2 O 2 scavenging activity (89.85 ± 3.86%) at a concentration of 200 µl, closely followed by the concentrations of 100 µl (64.99 ± 1.93%) and 50 µl (47.47 ± 0.97%), and the difference was observed to be significant (P < 0.05). Ascorbic acid at 100 µl displayed H 2 O 2 radical scavenging activity of 80.82 ± 3.53%, resulting in complete buffering of the free radicals that might be generated. e results of the present investigation seemed higher when compared to the H 2 O 2 radical scavenging activity of the aqueous extract of Indian seaweed [38]. e observed differences in the percentage of H 2 O 2 scavenging activity might be attributed to the variations in the geographical areas of collection from the sea or season of harvesting. It might also be due to the differences in extraction procedures, like using different solvents and filtration procedures. e total antioxidant activity of agar extracted from brown seaweed is shown in Table 3. e agar significantly showed increased total antioxidant activity (67.03 ± 3.30%) (P < 0.05) at a concentration of 200 µl, followed by concentrations of 100 µl (33.49 ± 2.14%) and 50 µl (16.77 ± 1.08%), respectively. e phosphomolybdate activity of agar extracted from brown seaweed is given in Table 3, which is caused by the reduction of Mo 6+ ions to form a green phosphate/molybdenum V complex. e agar from L. digitata was significantly increased (P < 0.05) by the scavenging phosphomolybdate assay (66.48 ± 3.03%) at a concentration of 200 µl and followed by concentrations of 100 µl (33.21 ± 2.05%) and 50 µl (16.63 ± 2.92%), correspondingly. e standard ascorbic acid exhibited (75.18 ± 3.54%) scavenging phosphomolybdate activity, resulting in complete buffering of the free radicals that might be generated. e potency reduction activity of agar extracted from the selected brown algae was calculated, and the result was expressed as a percentage. e potency reduction activity of FRAP is estimated by measuring the Fe 3 + -Fe 2 + transformation in the presence of agar extracted from L. digitata. e selected brown seaweed exhibited increased FRAP reducing power activity (72.03 ± 3.21%) at 200 µl followed by (82.31 ± 3.78%) at 100 µl (P < 0.05). e antioxidant activity is brought about by the ability to scavenge free radicals, and thus, in the current study, the agar of brown seaweed showed good antioxidant activity by scavenging ROS.

Evidence-Based Complementary and Alternative Medicine
Animal experiments revealed significant variations in food and water intake (Figures 1(a) and 2(b)) and body weight change (Table 4), in the D-Gal (group II)-injected mice when compared with the control group (group I) (P < 0.05). e water intake was significantly lower in D-Galinjected mice when compared to group I mice in the second week (P < 0.05). However, it significantly increased in the subsequent weeks (P < 0.05). Prior to the animals being sacrificed, no mice died during the entire experiment. However, at the beginning of the second week, mice demonstrated noticeable effects of D-Gal aging, such as apathy, delayed response, and slow motion, which continued for up to six weeks. Furthermore, group II mice had a significantly higher body weight than group I mice (P < 0.05). Current outcomes were endorsed by Swallow et al. [37] who claimed that food consumption and lack of physical activity played a major role in body composition. For the locomotor and rotarod (Figure 2) and light and dark and hot plate activities (Figure 3), group II mice experienced a significant decline when compared to group I mice in early (0 weeks) and late (6 weeks) (P < 0.05). e results of the present study suggested that all the abovementioned activities clearly proved that aging was induced in the D-Gal (group II) mice. On the other hand, the characteristics in the control sample (group III) and in the ascorbic acid orally administered mice (group IV) were found to be normal.
Figures 3(a) and 3(b) present the light and dark exposure and hot plate activity of experimental mice. According to the data, the time spent in light and dark in group II mice was significant (P < 0.05) compared to group I mice during the 6th week. e response of hot plate activity of group II mice was lower than that of group I mice during the second week onwards, and it was further decreased at the end of the experiment period (6 th week) (P < 0.05). e results strongly suggested that all the abovementioned activities clearly proved that aging was induced in the D-Gal (group II) mice, while these behaviors were stabilized in the control sample (group III) and in the ascorbic acid coadministered mice (group IV) [38]. It was also suggested that behavioral activities were slow in the aging mice. It slows down the rate of aging by influencing the basic cellular metabolism of motor activity at the organism level [24].
Mice injected with D-Gal showed noticeable symptoms of aging. e organ indices in the brain, liver, and kidney of the model group were lower than those of the control group as depicted in Figures 4(a) and 4(c) (P < 0.05). With age comes functional weakening and tissue/organ degeneration. Mostly, changes in the organs such as the brain, liver, and kidney weight were evident. So, the change in organ index is  Evidence-Based Complementary and Alternative Medicine a significant sign of organism senescence. D-Gal could induce physical aging and diminish organ indices of the brain, liver, and kidney in group II, according to the present experimental data. In group II, agar from brown seaweed could efficiently recover all organ indices. It demonstrated that seaweed agar could play a role in preserving the weight of all these organs from declining in the D-Gal experimental mouse model. With increased lifespan comes functional decline and atrophy of all organs and tissues. Differences in brain and kidney mass were noticeable [39]. Consequently, an organ index change was an essential sign of creature senescence, proving that the extracted agar and ascorbic acid     could play a vital role in protecting the weight of those organs from decreasing [40]. e in vivo antioxidant defense systems such as MDA, SOD, CAT, and GSH in mice administered with D-Gal (group II) exhibited a significant decrease in the tissues of the liver, brain, and kidney when compared to the control group I mice (P < 0.05). Group III mice showed a significant increase in the activities of all of these parameters (P < 0.05, Figures 5(a)-5(d)). Cell life in an oxygenated background has necessitated the progression of effective cellular tactics to identify and detoxify metabolites of ROS. e effects mentioned above could significantly disturb a host of physiological practices and metabolic pathways contributing to the aging of the animal and skin. For example, excess ROS   can cause lipid peroxidation in vivo. One of the final oxidation products is MDA, which induces cytotoxicity. erefore, the content of MDA might indicate the body's level of lipid peroxidation [19] and reveal the extent of cell injury carried out by ROS. e rise in the activities of the primary enzymatic antioxidant defenses-MDA, SOD, CAT, and GSH-in the sample coadministered group (group III) and vitamin C (group IV) mice was significant (P < 0.05). Presumably small amounts of agar may enhance the antioxidant activity of SOD. e GSH activity of the brain, liver, kidney, and serum (Figures 6(a)-6(d)) of D-Galinduced (group II) mice was significantly lower than that of the control, the sample, and vitamin C administered groups of mice (P < 0.05). e present findings were supported by the report of Ye et al. [24] who suggested that ethyl acetate extract from the plant (I. polycarpa defatted fruit) increased the antioxidant levels in experimental mice. e GSH level is a significant factor for quantifying the level of antioxidative activity in vivo and has tremendous antioxidant and detoxifying activities. It can protect almost every cell in the body. GSH not only eradicates free radicals in vivo but also boosts the organism's immunity level [41].
All the parameters in behavioral studies and the organ indices of D-Gal-induced aging mice were reduced. e antioxidant enzymes, elastin, collagen, and hyaluronic acid levels were low in D-Gal-induced mice, which endorsed the role of D-Gal on metabolic age changes in the skin. At the same time, all these levels were high in agar-treated mice. Further, the skin's moisture content affects the skin's physiological function. ese expressions (IL-1β and IL-6) were altered in D-Gal-induced mice which were brought to a normal level by mice administered with agar. e loss of elastin and moisture caused by the D-Gal-induced mice group II was significantly lower than that of control mice (group I) (P < 0.05), indicating that elastin and moisture would progressively alter with the age of the skin. Agaradministered group III mice had significantly increased elastin content when compared to group II mice (P < 0.05, Figures 7(a) and 7(b)). e present results were concurrent with the report of Ye et al. [24] who indicated that D-Gal reduced these cytokine factors, which were normalized by the ethyl acetate extract of I. polycarpa defatted fruit. Many scientific experts pointed out that cosmetic usage makes women lose elastin quicker than men [42]. Collagen fiber and hyaluronic acid are critical components of the skin. Collagen and hyaluronic acid content in group II mice decreased significantly relative to group I mice (P < 0.05). e variation in the amount of collagen can therefore accelerate skin aging (Figures 8(a) and  8(b)). Fittingly, brown algae agar improved the condition of mouse skin due to its high moisture and element content. Brown algae agar can effectively enhance the antioxidant activity, maintain collagen, elastin, and hydration, and reduce the MDA content of aging mouse skin. e morphological modifications of mouse skin have demonstrated the antiaging activity of agar. Collagen fibers decrease significantly with age and therefore make the skin inflexible and saggy. us, modifying the collagen content can accelerate the aging process of the skin [42]. e effect on IL-1β and IL-6 in the experimental groups is shown in Figure 9. e D-Gal-treated group exhibited increased IL-1β and IL-6 gene expression in the brain (P < 0.001 and P < 0.01, respectively); meanwhile, they only increased IL-1β gene expression in the liver (P < 0.01). In mice treated with D-Gal + agar 100 mg/kg, the IL-1β and IL-6 gene expression in the brain were inhibited, when compared with the D-gal-treated group alone. Further, IL-1β gene expression in the liver decreased conspicuously in the D-Gal + agar-treated group of mice. e present study reinforced the finding that D-Gal induced noticeable aging and oxidative stress in the brain and liver of experimental animals [24]. e paraffin sections of the brain, the liver, the kidney, and the skin of experimental mice are presented in Figures 10-13. It was noticed that the brain cell number of group II was less than that of groups I, III, and IV. Typically, cells in the brain degenerate with age, much like the reductions seen in group II mice. However, this number was regenerated in the agar-treated (group III) and vitamin C (group IV)-treated mice. In D-Gal-injected mice, hepatocytes were considerably damaged, displaying few appearances of ballooning degeneration and becoming shallow in comparison with group I mice. Further, all these changes were normalized in the sample-administered and ascorbic acid-treated mice. Similar histopathological findings were also reported by Ye et al. [24] who indicated that morphological alterations were seen in organs such as the brain, liver, and skin of the aging mice that administered D-Gal.

Conclusions
e in vitro antioxidant activity of agar from the brown algae L. digitata showed higher potency at higher concentrations. All parameters in the behavioral studies and organ indices for aging were reduced in the D-Gal-induced mice. Antioxidant enzymes, elastin, collagen, and hyaluronic acid levels were weak in D-Gal-induced mice, suggesting that D-Gal modified the metabolic age of the skin. All the parameters were elevated in mice exposed to agar. e expression of IL-1β and IL-6 was altered in D-Gal-induced mice, which was in turn brought back to normal by mice administered with agar. Finally, the anti-skin aging properties of agar were also confirmed by histopathology. All the outcomes suggested that agar from L. digitata holds promise as an antiaging natural phytomedicine and skincare product in the future.

Data Availability
All data generated or analyzed during this study are included in this published article.

Consent
Not applicable.

Conflicts of Interest
All authors declare that there are no conflicts of interest.

Authors' Contributions
RBS and RS conducted general experiments and assay and in vivo experiments. AT and NV supported data analysis and wide-ranging aspects of the manuscript preparation and development process. MME and MWQ provided research insight, examined the content, and supported wide-ranging aspects of the manuscript development process. RS critically reviewed the final manuscript draft and provided feedback on data and analyses. RS carried out the conceptual work, framework, manuscript preparation, and critical editing/ evaluation. All authors read and approved the final manuscript.