Antioxidant and Teratogenic Activities of Formulated Agar Extracted from Brown Seaweed Turbinaria conoides against Zebrafish Larvae

This study examines the antioxidant and teratogenic effects of two different type's methods of formulating agar from Turbinaria conoides (T. conoides) using a zebrafish model. The agar was extracted using the aqueous extraction method and developed in two different formulations using separate procedures. Formulated agar1 (FA1) used a higher concentration of the ingredients while formulated agar 2 (FA2) had a lesser concentration. The two unique formulated agars (FAs) were studied using biochemical composition, Fourier infrared (FT-IR) spectroscopy, gas chromatography-mass spectroscopy (GC-MS), and scanning electron microscopy (SEM). The antioxidant activities of both FAs in vitro were shown to be significantly different (P < 0.05) at various concentrations (60–180 μl/ml) in the study. The toxicity of the FAs was dose-dependent, with FA1 having the least teratogenic activity when compared to FA2. In comparison to FA2, FA1 was found to have higher antioxidant activity. At various concentrations (0.5, 0.25, and 0.125 μg/ml), the teratogenic activity of two FAs was examined in zebrafish embryos (ZFE) at 24, 48, 72, and 96 hours post fertilization (hpf). Both FAs exhibit dose-dependent toxicity and increased antioxidant activity, and this can be utilized as an alternative for standard antioxidants, according to this study.


Introduction
Seaweeds/marine algae are a major part of the structurally diverse marine flora with several properties like antibacterial, anti-inflammatory, antiaging and anticarcinogenic. Seaweeds are rich in antioxidants and have potentially higher cosmetic effects due to the presence of several active ingredients. Cosmetic products derived from seaweed are increasingly preferred over synthetic compounds, with no harmful chemical compounds [1,2]. Polysaccharides extracted from seaweeds play a pivotal role as humectants and moisturizers in cosmetic formulations, and can also be used as thickeners, gelling agents, film formers and emulsifiers [3]. Turbinaria conoides (T. conoides), brown algae which belong to the Sargassaceace family and the Fucales order, are a rich source of polysaccharides. e ethyl acetate extract of Turbinaria conoides was reported to have several properties like antibacterial, anticancer and higher antioxidant activity. Antioxidants are vital to reduce oxidative stress by removing the excess free radicals which have been associated with the emergence of degenerative processes in molecular biology, which encourage oxidative activities that are harmful to the body. e capacity of antioxidant chemicals in plants (carotenoids, polyphenols, polysaccharides, unsaturated fatty acids, vitamins, enzymes, and cofactors) to trap free radicals has inspired interest in employing them in preventative and curative phytotherapy [4]. T. conoides are a rich source of several phytochemical components such as sulphated polysaccharides, glucuronic acid, and alginic acid, and also contain compounds such as digestible proteins, mineral salts (K, Ca, and Fe), and polyunsaturated fatty acids [5]. Our laboratory had previously investigated the anti-skin cancer and antioxidant effects of FA from the brown seaweed Laminaria digitata [6], but this finding has not been reported using the standard FA method. Drug screening with zebrafish has several advantages, like increased efficiency, lower operating costs, shorter testing periods, easily controllable experimental conditions, and most significantly, increased genetic similarities between zebrafish and humans (approximately 70%) which makes the zebrafish a successful animal model [7]. Hence, the current study compared the antioxidant capabilities and toxicity of FA in zebrafish embryos (ZFEs).

Seaweed Collection.
e brown seaweeds (T. conoides) were collected from the Gulf of Mannar (9.1278°N, 79.4662°E), Tamil Nadu, India, during the period of December 2020-January 2021. e brown seaweeds were known and confirmed by the Central Marine Fisheries Research Institute (CMFRI). Brown seaweeds were collected and then washed in fresh water to remove any undesired elements, such as other seaweed species. ese samples were meticulously cleaned with seawater before being rinsed in double-distilled water. e seaweeds were dried in the shade and finely powdered with a blender before being stored at −20°C for subsequent investigation.

Extraction of Agar.
To extract water-soluble polysaccharides, 20 g fine powdered seaweed samples were combined with 200 ml Milli-Q water and autoclaved at 121°C for 1 h. To remove seaweed debris, the extract was then filtered through Whatman No. 1 filter paper and centrifuged at 4500 rpm for 20 min. To produce a gel, the extract was maintained at room temperature [8].

Preparation of FAs.
Agar processing methods have been developed in several countries, as illustrated in Figure 1, the extracted agar was transformed into a formulation using two distinct processes [9,10].

Characterization of FAs.
e colour, odour, consistency, sterility, and homogeneity were all employed to identify the characteristics of both FAs [11][12][13]. pH, vibrational testing, centrifugation tests, and physicochemical properties were all looked into [14,15]. e information presented here pertains to three different determinations.

Biochemical Composition of FAs by Flame Emission
Atomic (FEA) Spectroscopy. 0.2 g of two FAs were mixed with HClO₄ and left undisturbed for 5 min. 5 ml of conc. HNO 3 was mixed and incubated for 5 min followed by adding 5 ml of conc. HCl. e mixture was allowed to evaporate. An FEA spectrophotometer was used to analyze the filtrate. e minerals analyzed were calcium and phosphorus. e results were expressed as ppm and percentage [16].

Fourier Transform Infrared Spectroscopy (FT-IR) of
FAs. FT-IR qualitative analysis of two FAs was performed by using a Bruker Alpha instrument (USA) with the spectrum recorded between 4000 to 400 cm −1 [17].

Gas Chromatography-Mass Spectrometry (GC-MS) of FAs.
e GC-MS spectroscopic analysis was carried out (Agilent, Santa Clara, CA, USA). e detection of an electron ionization system with an activity force of 70 eV and a mass range of 30 to 650 m/z was utilized [18].  200 μl of methanolic DPPH solution was added and mixed thoroughly using a vortex mixer. e absorbance was measured at 517 nm in UV spectroscopy and the state was measured by using the following formula [20]:

Scanning Electron
where A control � absorbance of the control sample; A sample � absorbance of FA.

H 2 O 2 Radical
Scavenging Activity. 0.5 ml of FA solutions was added with 600 μl H 2 O 2 solution (40 Mm) to determine the H 2 O 2 radical scavenging activity. e absorbance was then calculated at 230 nm in UV spectroscopy [16].

Total Antioxidant Activity (TAA).
e TAA of FAs was determined by using a total antioxidant capacity (TAC) solvent (0.6 M sulfuric acid, 28 mM sodium phosphate, and 4 mM ammonium molybdate). 0.2 ml FAs were mixed with 3 ml of the TAC reagent solution and then incubated in a water bath for 90 min. e readings of the reaction were then measured at 695 nm by using a UV-visible spectrophotometer [4]. (2) where A control � absorbance of the control sample and A sample � absorbance of FA.

2,2-Azino-is-3-ethylbenzothiazoline-6-sulfonic Acid (ABTS) Activity.
e ABTS solution absorbance was checked using 1 ml ABTS solvent with 60 ml methanol to attain the readings of 0.73 at 734 nm. e ABTS activity of FAs was compared with standard vitamin E at 734 nm in a UV-visible spectrophotometer [20].
where A control � absorbance of the control sample and A sample � absorbance of FA.

Zebrafish
Husbandry. At a temperature of 28°C, adult wild zebrafish were kept in dark and light for 10 to 14 hrs at a time. Natural spawning was used to gather viable eggs, which were then washed in distilled water the next morning. e E3 medium (34.8 g NaCl, 1.6 g KCl, 5.8 g CaCl 2 ·2H 2 O, 9.78 g MgCl 2 ·6H 2 O) was used to harvest and store embryos. For the teratogenic FAs investigation, coagulated and damaged eggs were removed and viable eggs were chosen [21].

Teratogenic Activities of FAs.
At varied diluted concentrations (0.5, 0.25, and 0.125 μg/ml), the teratogenic activity of the two distinct FAs was tested. A stereomicroscope was used to investigate the ZEF at various phases of growth [22].

Statistical Analysis.
Each test was carried out in a triplicate manner, with the findings reported as the mean SD. Significance was defined as a P value of <0.05. IBM SPSS Statistics for Windows, version 22, was used for statistical analysis (IBM Corp., Armonk, N.Y., USA).

Results and Discussion
e wet weights of FAs obtained by FA1 84.2% and FA2 80.6% are mentioned in (Table 1). e chemicals and quantity have an impact on the yield and rate of an FA. Marine pharmacologist creates methods in the manufacturing business that maximize the yield and production rate of FA.
ey also want to cut waste and energy expenses at every step of the experiment [23]. e agar formulation methods and yield used for developing antioxidant properties for both the FAs from brown seaweed have been successful (T. conoides).
Marine algae are rich sources of macroelements such as K, Ca, Na, and Mg. e results of FA were similar to Sargassum wightii, which also showed higher Na ions concentration. In L. digitata, higher Na, Ca, and Fe were also associated with increased antioxidant capacity, and a lower level had adverse consequences. Brown algae, like Saccharina latissima, were reported to be used as an alternative to Na content. Similarities in higher concentrations of Na, Ca, and Fe were found. As shown in earlier studies, the increased levels of K, Zn, Cu, and Co were associated with higher antioxidant levels [16]. e variation in agar yield has been reported to differ from species to species, depending on the harvest season.
Two distinct agar formulations were created to ensure agar quality, effectiveness, safety, and stability. Table 2 shows both the formulation procedures, FA1 is better for T. conoides agar formulation. Stability may be influenced by environmental factors such as pH, light, temperature, air, and movement. No change in colour or odour, as well as robust consistency, smooth homogeneity, no microbiological contamination, and sterility, were determined as stability parameters in two different types of FAs. ese findings suggest that the two FA gels would be suitable for topical use. ere was no evidence pertaining to the phase separation in the two types of FAs during the three-month investigation.
e FT-IR spectrum of FAs extracted from seaweed confirmed the presence of functional groups and bands absorbed in the 4000-500 cm −1 ranges are clearly displayed as shown in Figure 2. FAs are confirmed by FT-IR spectra, which showed peaks around 3283.4 cm −1 (OH group), 2922.2 cm −1 (alkenes), 1829.7 cm −1 (C-N stretch), 1496.2 cm −1 (alcohols and carboxylic acids), 1038 cm −1 (aliphatic amines), and 892 cm −1 (aromatics). A considerable absorption band is discovered in 1260 cm −1 . e existence of S�O bonds in sulphate ester groups explains this. e FT-IR analysis of FAs confirmed the presence of galactopyranose unit and sulphate content indicating the presence of polysaccharides contents which are compared with the standard. All of the FT-IR spectra indicated a broad band ranging from 2900 to 3300 cm −1 , which is attributed to the O-H stretching vibration from the hydroxyl group of polysaccharides, which corresponded to the hydrophilic property of seaweed [4].
When compared to FA2 (346 kDa), FA1 had a lower molecular weight (205 kDa). e fragmentation spectra of the ions generated from each of the three protonated HexNAcs (m/z 150) were compared first. Despite, the fact that both the HexNAcs have the same composition, GalNAc and GalNAc differ from GlcNAc (Figure 3(a) and B) at a single stereocenter [24]. Agaropectin from red algae has a lower molecular weight and sulphate concentration than other agaropectins, with m/z � 149 for pentoses, 163 for desoxy-hexoses, and 179 for hexoses. [25].
SEM is used to evaluate the morphology and gel surface of the FAs. SEM images of the plain's exterior surface show it to be flattened, rough, and exceedingly uneven, with a porous structure (Figure 4(a) & 4(b)). e FA1 characteristics' results are present in (Figure 4(a)). It appears to be a smooth, stratified, and ordered flat continuous sheet. Whereas FA2 displayed an irregular, continuous network sheet (Figure 4(b)). According to the findings of Syad et al. [19], the morphological analysis (SEM) extracted from green and brown seaweed has a smooth, flat, and continuous sheet appearance.
e ability of the FA to produce radicals scavenging activities are investigated, as shown in (Table 3). When compared to the antioxidant activities of FA2, FA1 has a significant (P < 0.05) increase in antioxidant activities such as DPPH, H 2 O 2 , total antioxidant, and ABTS activities. FA1 has higher sulphate content (41.78%) than FA2(37.25%), which contributes to its high antioxidant activity. Furthermore, when compared to low dose (60 µg/ml) and standard vitamin E, all of the above antioxidant parameters are significantly increased at a highdose (180 µg/ml) concentration of FA1 and FA2. As a result, significant differences in the in vitro antioxidant, scavenging abilities of phytochemicals isolated from seaweed could be due to differences in the type of extraction and/or the collection zone of the seaweeds [26]. e 180 μl concentration of FA 1 from T. conoides showed significant (P < 0.05) increase in equal scavenging (82.28 ± 1.09) activity when compared to the concentration of FA2 of 180 μl (80.11 ± 0.13). e variations in H 2 O 2 scavenging percentages in this analysis may be due to differences in extraction techniques or species-specific differences reported in [4]. e ability of the FA to produce total antioxidant activity was investigated, as shown in (Table 3). e 180 μl concentration of FA1 from T. conoides showed significant (P < 0.05) increase equal scavenging (69.65 ± 3.5) activity when compared to the concentration of FA2 of 180 μl (64.67 ± 1.41). e capability of the FA to produce ABTS radicals was      Evidence-Based Complementary and Alternative Medicine investigated, as shown in (Table 3).
e 180 μl concentration of FA1 from T. conoides showed significantly (P < 0.05) increase equal scavenging (80.66 ± 0.64) activity when compared to the concentration of FA2 of 180 μl (72.41 ± 0.35). Considering the absence of phytochemical components, the overall antioxidant activity of Hypericum olympicum was found to be very high. is is most likely owing to the presence of other compounds mentioned in the study [20]. e toxicity effects of different concentrations of two FAs with different doses of 0.5 μg/ml, 0.25 μg/ml, and 0.125 μg/ml were evaluated in various aspects. In a low concentration of 0.125 μg/ml, FA1 was less teratogenic when compared with FA2 [22]. It shows the development of embryos for different concentrations of two FAs (control, 0.5 μg/ml, 0.25 μg/ml, and 0.125 μg/ml) at various time periods for different concentrations of two FAs (24 hpf, 48 hpf, 72 hpf, and 96 hpf ) (Figure 5(a) and 5(b)). e higher toxicity level resulted in deformities such as yolk sac diffusion, delayed hatching, poor development, and death rate. e lowest concentrations, 0.125 μg/ml and 0.25 μg/ml, showed low pigmentation, tail bending, and body curvature, similarly to the control under constant observation in (Figures 5(a) and 5(b)), and when compared to FA2, the teratogenic activity of the sulphated chitosan, FA1, showed less toxicity in zebrafish larvae [27].

Conclusion
e agar isolated from T. conoides was made into a formulation and FA1 made with more ingredient concentration was found to have higher antioxidant, scavenging activity, and less teratogenicity compared to FA2 made with less ingredient concentration. After clinical trials, the skin permeability of the agar separated may be examined, which could be useful in cosmetic production.

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

Ethical Approval
Human subjects, human material, or human data are not used in this study. e Institutional Animal Ethics Committee, Chettinad Academy of Research and Education (Deemed to be University), Kelambakkam-603 103, Tamil Nadu, India, approved this study, which followed the guidelines of the Committee for the Purpose of Control and Supervision of Experiments on Animals (CPCSEA), Government of India.  Evidence-Based Complementary and Alternative Medicine