Antimicrobial Effect of Carbon Nanodots–ZnO Nanocomposite Synthesized Using Sargassum horneri

: For several years, industrial damages caused by massive blooming and drifting of Sargassum horneri ( S. horneri ) called “golden tides” seaweeds have been continuously reported in Korea. National efforts have been made to produce useful cases of application by using the troublesome S. horneri . As a part of that, a CNDs–ZnO nanocomposite with antibacterial and antifungal properties was synthesized through a simple hydrothermal reaction using S. horneri , and the results were veriﬁed in this paper. The antibacterial and antifungal activities were mainly determined by the disk diffusion test against ﬁve bacterial and fungal strains, respectively. Of note, the inhibitory effect of the CNDs–ZnO on the growth of both Gram-positive ( Bacillus cereus and Staphylococcus aureus ) and Gram-negative ( Escherichia coli , Salmonella typhimurium , and Vibrio alginolyticus ) bacteria was highly effective. Moreover, the nanocomposite showed low toxicity compared to chlorine bleach. In addition, the CNDs–ZnO showed antifungal activities against both yeast ( Saccharomyces cerevisiae and Rhodotorula mucilaginosa ) and mold ( Aspergillus ﬂavus , Aspergillus niger , and Aspergillus terreus ). This work showed the potential usability in antimicrobial application based on poor marine brown alga considered as useless in Korea. Through this paper, it seems that sufﬁcient utility and possibility can be expected upon various unappreciated and uninterested marine species.

Interestingly, CNDs have been revealed to possess photocatalytic characteristics resulting in light-activated antimicrobial activities under visible light through several research studies. The fluorescence emission parameters of CNDs correlated with the photoexcited states and redox processes are major important factors to induce their antimicrobial activities [4,[11][12][13][14]. These carbon-based fluorescent materials of typically less than 10 nm in diameter are usually synthesized by top-down or bottom-up methods. In particular, green

Synthesis of CNDs-ZnO Nanocomposite
The CNDs-ZnO using S. horneri was easily synthesized by a one-pot hydrothermal reaction. First, 2 g of S. horneri was washed thoroughly under running tap water to remove some remained salt and sand and dried at 25 • C. The washed and dried brown algae were frozen using liquid nitrogen and finely crushed in a mortar, and the fine powders were mixed with 10 wt% of zinc acetate solution in 15 mL of ethanol absolute and 15 mL of ultrapure water (volume ratio of EtOH:ultrapure water = 1:1). The mixed solution was sonicated for 30 min using an ultrasonic bath sonicator (S60H; Elma Schmidbauer GmbH, Singen, Germany) and it was transferred into a 50 mL polypropylene (PPL)-lined hydrothermal autoclave reactor (TEFIC Biotech Co., Xi an, China) for hydrothermal reaction at 180 • C for 6 h. The heated reactor was cooled down naturally at room temperature to 25 • C. The obtained aqueous CNDs-ZnO solution was centrifuged using a Frontier TM 5718R centrifuge (Ohaus, Parsippany, NJ, USA) at 5500 rpm for 30 min. The supernatant after centrifugation was gathered and then filtered using a syringe filter with a 0.22 µm pore sized membrane. The final CNDs-ZnO solution (pH 6-6.5) was stored in the refrigerator at 4 • C until use. Using freeze-drying, the concentration of the CNDs-ZnO nanocomposite was determined to be 58-60 mg/mL.

Preparation of "CNDs Alone" and Pure ZnO Nanoparticles
CNDs based on S. horneri, which were denoted by "CNDs alone", were fabricated as a control to prove the antibacterial activity of CNDs-ZnO. The fabrication procedure was highly similar to that of CNDs-ZnO. First, 2 g of ground S. horneri powders was mixed with 15 mL of ethanol absolute and 15 mL of ultrapure water (volume ratio of EtOH:ultrapure water = 1:1), and the mixed solution was ultrasonicated for 30 min in an ultrasonic bath. The solution was subjected to a hydrothermal reaction at 180 • C for 6 h and subsequently cooled down to 25 • C. The final solution was obtained through centrifugation at 5500 rpm for 30 min and filtration using a 0.22 µm pore filter. Two kinds of pure ZnO solutions were prepared based on zinc acetate dehydrate and commercial ZnO NPs. The first pure ZnO NPs were fabricated under a virtually identical synthetic condition to that of CNDs-ZnO based on several references [47][48][49][50][51][52]. In brief, 2 g of zinc acetate dehydrate with 10 g of sodium hydroxide were dissolved into 10 mL of ultrapure water and 10 mL of ethanol absolute. Then, the mixed solution was heated at 180 • C for 6 h. After cooling to room temperature, the as-obtained white powders were washed with ultrapure water and ethanol absolute three times through centrifugation. Finally, the powders were reconstituted in 20 mL of mixed ultrapure water and ethanol absolute solution (volume ratio = 1:1). Another type of pure ZnO NPs (60 mg/mL of concentration) was prepared using commercialized ZnO NPs in ethanol-ultrapure water at pH 9. Both pure ZnO NPs were also used as experimental controls.

Characterization of CNDs-ZnO
Transmission electron microscopy (TEM) images of the CNDs-ZnO were taken by using a H-7650 microscope operated at 100 kV (Hitachi, Ltd., Tokyo, Japan) and EDS analysis was performed simultaneously. For TEM image analysis, the diluted CNDs-ZnO solution added with ultrapure water was dropped on the TEM grid and dried at room temperature. The particle size distribution analysis of the CNDs-ZnO was performed by the Gatan DigitalMicrograph program (v 3.30), and its histogram was represented through the Gaussian distribution function in Origin software (8.6 version, OriginLab Corp., Northampton, MA, USA). Fourier-transform infrared (FT-IR) spectroscopy and X-ray photoelectron spectroscopy (XPS) were analyzed using a Frontier MIR/FIR spectrometer from 400 cm −1 to 4000 cm −1 (PerkinElmer, Inc., Waltham, MA, USA) by the ATR method and a PHI5000 VersaProbe III photoelectron spectrometer (Ulvac-Phi, Inc., Kanagawa, Japan) including an Al Kα radiation source (hv = 1486.6 eV), respectively. For FT-IR and XPS analyses, the CNDs-ZnO solution was lyophilized through the temperature change from −40 • C to 20 • C using the FreeZone benchtop freeze dryer (Labconco, Kansas city, MO, USA). Photoluminescence (PL) spectra were acquired through a FluoroMax-4 spectrometer (HORIBA, Ltd., Kyoto, Japan) within the range from 270 nm to 700 nm in 10 nm-step increments under the excitation range between 250 nm and 550 nm. The UV-Vis absorption spectra were investigated from 220 nm to 800 nm using a BioSpectrometer ® basic (Eppendorf, Hamburg, Germany). Photo-images of the fluorescent CNDs-ZnO solution were recorded using a commercial digital camera (EOS M6, Canon, Tokyo, Japan) while irradiating an LED light with 430-440 nm or UV-AC hand lamp with 365 nm (VL-6.LC; Vilber, Collégien, France).

Antibacterial Test
To examine the antibacterial activity of the as-fabricated CNDs-ZnO, three strains of Gram-negative bacteria (E. coli, S. typhimurium, and V. alginolyticus) and two strains of Gram-positive bacteria (B. cereus and S. aureus) were selected. The bacterial strains were first cultured in 20 mL of Luria-Bertani (LB) liquid media broth at 30 • C overnight. Colony-forming units (CFUs) were determined using a QUANTOM Tx TM microbial cell counter (Logos Biosystems, Anyang, South Korea), and all bacterial strains were adjusted to 1 × 10 7 cfu/mL. Then, 200 µL of each bacterial suspension was spread evenly over LB-agar plates. Paper discs (ϕ = 8 mm) were soaked in 30 µL of CNDs-ZnO or control solutions and then placed on LB-agar plates. The plates were incubated at 30 • C overnight. The antibacterial activity of the CNDs-ZnO solution was observed by examining the disks for an inhibition zone. Disk diffusion tests were performed with or without UV irradiation at 365 nm to investigate the photo-induced antibacterial effect attributed to the CNDs of the nanocomposite. Moreover, the CNDs-ZnO solution was lyophilized by freeze-drying, and the powder was reconstituted in ultrapure water without subsequent EtOH addition to examine its antibacterial activity through the disk diffusion test under the same method mentioned above. The experiments to measure the inhibition zones were conducted in triplicate, and the sizes of the inhibition zones were measured using a digital caliper (CD-8" ASX; Mitutoyo Corp., Kanagawa, Japan). A minimum inhibitory concentration test (MIC) for the bacterial strains was also performed using the CNDs-ZnO solution.
Every strain was incubated to 1 × 10 5 cfu/mL in LB liquid media broth at 30 • C and then transferred to a 96-well plate. A total of 11 different concentrations of CNDs-ZnO solutions were prepared by two-fold serial dilution and combined with as-prepared bacterial strains. The plates were incubated at 30 • C for 20 h, and then turbidity was observed at OD 600 through a Multiskan™ GO Microplate Spectrophotometer (Thermo Scientific, Waltham, MA, USA). In addition, bacterial growth curve analysis according to the adjusted CNDs-ZnO solution was conducted using a Multiskan™ GO Microplate Spectrophotometer for 20 h.

Antifungal Test
The antifungal activities of CNDs-ZnO were determined using a disk diffusion test against two species of yeasts (R. mucilaginosa and S. cerevisiae) and three species of molds (A. flavus, A. niger, and A. terreus). The selected fungal strains were cultivated on potato dextrose agar (PDA; BD, Franklin Lakes, NJ, USA) at 28 • C for 5 days. Their spores were collected using sterile ultrapure water and counted using a hemocytometer (INCYTO, Cheonan, South Korea). Then, 1 × 10 6 of fungal spores were prepared in 5 mL of melted PDA with 0.7% agar and overlaid onto 25 mL of PDA. Before the paper discs were placed on the PDA plates, 50 µL of CNDs-ZnO or pure ZnO as a control were dispensed to 10 mm discs. The disks were subsequently placed on the as-prepared fungal plates and then cultured at 28 • C for 2-3 days. Antifungal activity was evaluated by checking each disk for an inhibition zone. This experiment was performed in triplicate, and the sizes of the inhibition zones were also evaluated using a digital caliper (CD-8" ASX; Mitutoyo Corp., Kanagawa, Japan).

Toxicity Test in Zebrafish Embryos
The in vivo toxicity of the CNDs-ZnO solution was confirmed using wild-type zebrafish embryos. At 4 h after fertilization, embryos without deficiencies were selected visually using a stereomicroscope (S6D, Leica, Germany). The selected normal zebrafish embryos were transferred to a 24-well plate with 5 specimens per well and exposed to serially diluted CNDs-ZnO-1, CNDs-ZnO-2, pure ZnO NPs, and chlorine bleach. The zebrafish embryos were incubated at 28.5 • C for 24 h and then observed using a stereomicroscope.

Optical Properties of the CNDs-ZnO
A CNDs-ZnO aqueous ethanol solution that appeared brown-colored in daylight was fabricated by a one-pot hydrothermal reaction with S. horneri and zinc acetate dihydrate. The nanocomposite solution appeared yellowish green and light coral blue under irradiation of LED light at 430-440 nm and UV light at 365 nm ( Figure 1a). Interestingly, the PL brightness of the CNDs-ZnO solution was higher than that of the CNDs solution (CNDs alone) fabricated under identical conditions without zinc acetate dehydrate. Their morphological difference was later verified by TEM imaging and is described in Section 3.2. The UV-Vis absorption spectrum of CNDs-ZnO showed a broader absorption band between 240 and 480 nm than that of CNDs alone (Figure 1b). The absorption peak at 265 nm was attributed to the carbonic core center [52] and a faint shoulder peak at approximately 326 nm corresponded to the π-π* transition of C=C bonds in the aromatic sp2 domain and n-π* transition of C=O bonds, respectively. Their excitation wavelength-dependent PL behavior was the same as that of typical CNDs. Upon the change in excitation wavelength, the PL wavelength shifted from blue to red (Figure 1c). The excitation wavelength-dependent behavior of the CNDs-ZnO was attributed to the entrapment of the generated excitons in the defects, which resulted from surface passivation induced by carbonization during hydrothermal treatment [43,44]. The emission maximum of the CNDs-ZnO was observed at approximately 500 nm under 420 nm of excitation wavelength. For CNDs alone, similar PL-shifted characteristics were observed, but its PL intensity behavior upon each excitation wavelength band was evidently different from that of CNDs-ZnO. carbonization during hydrothermal treatment [43,44]. The emission maximum of the CNDs-ZnO was observed at approximately 500 nm under 420 nm of excitation wavelength. For CNDs alone, similar PL-shifted characteristics were observed, but its PL intensity behavior upon each excitation wavelength band was evidently different from that of CNDs-ZnO.     (Figure 3). Although some peaks from residual elements such as Mg, Cl, and K were measured, they seemed to originate from salts that were incompletely washed away from S. horneri; these salts were also detected in the TEM images. The percentage of atomic concentrations in CNDs-ZnO is also displayed in Figure Figure 3). Although some peaks from residual elements such as Mg, Cl, and K were measured, they seemed to originate from salts that were incompletely washed away from S. horneri; these salts were also detected in the TEM images. The percentage of atomic concentrations in CNDs-ZnO is also displayed in Figure 3, with C = 54.78%, N = 2.95%, O = 32.40%, and Zn = 9.87%; by contrast, the atomic concentrations in CNDs alone were C = 68.79%, N = 8.70%, and O = 22.50%.      (Figure 4c,d). The high-resolution O 1s spectra of CNDs-ZnO and CNDs alone showed similar binding energies at 531.52 and 532.77 eV in CNDs-ZnO and at 531.14 and 532.41 eV in CNDs alone, as shown in Figure 4e,f, respectively. The changes in the O 1s spectra apparently resulted from the formation of the structures of oxide and carbonate with zinc in the nanocomposite. In the O 1s spectrum of the CNDs-ZnO, the peak centered at 531.52 eV represented the O 2− state of oxygen vacancies or defects, involving the formation of nonstoichiometric ZnO, and another peak centered at 532.77 eV was assigned to the weak bonds of OH groups on the surface. In addition, the double peaks of Zn 2p corresponding to the Zn 2+ oxidation state were detected at 1021.93 and 1044.96 eV, which are assigned to Zn 2p 3/2 and Zn 2p 1/2 , respectively, with a separation of 23.03 eV (Figure 4g). The binding energies of Zn 2p also showed a positive shift compared to those of typical pure-zinc oxide nanostructures owing to the formation of the nanocomposite structure with carbon dots from S. horneri.

Morphological Characteristics of the CNDs-ZnO
A TEM study of the CNDs alone and the CNDs-ZnO nanocomposite was performed to further analyze the structure and calculate the size distribution of the nanocomposite. The TEM image in Figure 5a,b shows various spherical-like carbon dots (CNDs alone) and the nanocomposite (CNDs-ZnO), where carbon dots are decorated on zinc oxide nanoparticles. Their morphological differences could be clearly identified in Figure 5a,b. Additionally, the elemental composition of the CNDs-ZnO was determined by EDS analysis. Figure S1 shows the elemental distribution with the atomic percentage. From the EDS data, the CND-ZnO consisted of carbon, oxygen, and zinc with residual Na, Mg, and Cl resulting from seawater that had not been thoroughly washed. The sizes of the CNDs-ZnO in Figure 5b were widely distributed from approximately 30 nm to 170 nm, with nanocomposites of 70-90 nm size occupying the largest proportion, as determined by counting 124 particles. Therefore, the marine brown algae S. horneri, which is considered useless, acts as a good reducing agent for synthesizing zinc oxide and as an excellent biomaterial for fabricating carbon dots.

Disk Diffusion Test for Antibacterial Activity
The antibacterial activities of CNDs-ZnO were determined by using a disk diffusion test with three Gram-negative and two Gram-positive bacteria. First, the CNDs-ZnO nanocomposites were fabricated with S. horneri from Buan-gun and Sinan-gun via the synthetic method described in Section 2.2. The as-synthesized CNDs-ZnO solutions with S. horneri from Buan-gun and Sinan-gun were denoted by CNDs-ZnO-1 and CNDs-ZnO-2, respectively. The two as-prepared pure ZnO NPs were used as experimental controls. After 30 µL of each CNDs-ZnO and pure ZnO was applied to paper disks on LB-agar plates containing the bacteria, the plates were incubated at 30 • C overnight, and then their inhibition zones were checked ( Figure S2a). Clear inhibition zones were observed from both CNDs-ZnO-1 and CNDs-ZnO-2, whereas the pure ZnO samples showed poor inhibition zones. Because the antibacterial test for V. alginolyticus was additionally conducted solely, the photos are not shown. The results are summarized in Table 1. A TEM study of the CNDs alone and the CNDs-ZnO nanocomposite was performed to further analyze the structure and calculate the size distribution of the nanocomposite. The TEM image in Figure 5a,b shows various spherical-like carbon dots (CNDs alone) and resulting from seawater that had not been thoroughly washed. The sizes of the CNDs-ZnO in Figure 5b were widely distributed from approximately 30 nm to 170 nm, with nanocomposites of 70-90 nm size occupying the largest proportion, as determined by counting 124 particles. Therefore, the marine brown algae S. horneri, which is considered useless, acts as a good reducing agent for synthesizing zinc oxide and as an excellent biomaterial for fabricating carbon dots.

Disk Diffusion Test for Antibacterial Activity
The antibacterial activities of CNDs-ZnO were determined by using a disk diffusion test with three Gram-negative and two Gram-positive bacteria. First, the CNDs-ZnO nanocomposites were fabricated with S. horneri from Buan-gun and Sinan-gun via the synthetic method described in Section 2.2. The as-synthesized CNDs-ZnO solutions with S. horneri from Buan-gun and Sinan-gun were denoted by CNDs-ZnO-1 and CNDs-ZnO-2, respectively. The two as-prepared pure ZnO NPs were used as experimental controls. After 30 μL of each CNDs-ZnO and pure ZnO was applied to paper disks on LB-agar plates containing the bacteria, the plates were incubated at 30 °C overnight, and then their inhibition zones were checked ( Figure S2a). Clear inhibition zones were observed from both CNDs-ZnO-1 and CNDs-ZnO-2, whereas the pure ZnO samples showed poor inhibition zones. Because the antibacterial test for V. alginolyticus was additionally conducted solely, the photos are not shown. The results are summarized in Table 1. Next, the antibacterial activities of the CNDs-ZnO-1 and CNDs-ZnO-2 were compared with those of CNDs alone synthesized based on different S. horneri samples collected from Buan and Sinan, respectively ( Figure S2b). For the CNDs alone, no antibacterial activity and inhibition zones were observed; by contrast, CNDs-ZnO-1 and CNDs-  Next, the antibacterial activities of the CNDs-ZnO-1 and CNDs-ZnO-2 were compared with those of CNDs alone synthesized based on different S. horneri samples collected from Buan and Sinan, respectively ( Figure S2b). For the CNDs alone, no antibacterial activity and inhibition zones were observed; by contrast, CNDs-ZnO-1 and CNDs-ZnO-2 showed excellent antibacterial activities with obvious inhibition zones. After being powdered by lyophilization and re-dissolving in ultrapure water without ethanol, the CNDs-ZnO-1 and CNDs-ZnO-2 still showed clear inhibition zones for all bacterial plates, as shown in Figure S3a. In the figure, their antibacterial ability was maintained after reconstitution in ultrapure water. The solubility of zinc oxide nanoparticles is an important factor that influences the antibacterial property because it affects the distribution of Zn 2+ ions in the media [53,54]. Because the CNDs-ZnO nanocomposites were well-dispersed even in ultrapure water, their antibacterial ability was retained. Furthermore, this antibacterial activity was still maintained even after storage at room temperature after sunlight was blocked for more than 6 months.
Finally, to compare the antibacterial ability of both CNDs-ZnO-1 and CNDs-ZnO-2 with that of a commercially available disinfectant, a 10% chlorine bleach solution (10% Clorox) was reacted with the bacteria. The bleach, which consists of sodium hypochlorite, is a known effective killing agent for bacteria and even the COVID-19 virus. In fact, the Korea Disease Control and Prevention Agency (KDCA) has provided guidelines for typical disinfection of surfaces by using sodium hypochlorite-containing Clorox at concentrations of 500 ppm to 1000 ppm as a precautionary measure to prevent COVID-19. Moreover, the use of 5000 ppm bleach solution to clean up the blood or body fluids of COVID-19 patients is encouraged. According to manufacturer information, the concentration of chlorine bleach is 50,000 ppm. Thus, the concentration of the chlorine bleach in this research was set to 5000 ppm through 1/10 dilution. Similar to the previous method, 30 µL of 1/10-diluted chlorine bleach was applied to the LB-agar plates on four selected bacteria, which were subsequently incubated at 30 • C overnight. Afterward, strongly apparent and large inhibition zones were detected in all bleach-treated plates ( Figure S3b). The sizes of inhibition zones by CNDs-ZnO-1, CNDs-ZnO-2, and chlorine bleach are summarized in Table 1. Inhibition zones smaller than 8.5 mm in size were ignored and are expressed as negligible in the table. The two pure ZnO samples both showed marginal antibacterial activity, such as 17 ± 1 and 15 ± 1 mm in V. alginolyticus and 13 and 12 ± 2 mm in S. aureus, while its antibacterial effect against other bacteria was not noticeable. For CNDs alone based on S. horneri, no antibacterial activity against all bacteria was observed. By contrast, the two CNDs-ZnO nanocomposites exhibited a remarkable antibacterial effect against all bacteria. Except against B. cereus, both CNDs-ZnO presented excellent inhibition regions of 20 mm or larger against most bacteria; these inhibition zones were almost at a similar level or slightly inferior to those of 10% chlorine bleach. Interestingly, both CNDs-ZnO samples showed superior antibacterial activities against E. coli at 22 ± 3 and 21 ± 2 mm and against S. aureus at 25 ± 4 and 25 ± 4 mm compared to those of 10% chlorine bleach at 21 ± 2 and 23 ± 3 mm, respectively. Although the exact mechanism of antimicrobial activity of ZnO NPs is not fully revealed and remains controversial, the dominant principles are that ZnO NPs release Zn 2+ ions or generate reactive oxygen species (ROS), which lead to the disruption of bacterial cell structures or an increase in oxidative stress triggered in preventing DNA replication or protein synthesis, respectively [55][56][57]. Based on the results of several studies, the antibacterial properties of CNDs-ZnO were also due to the same mechanisms mentioned above. Next, photo-induced antibacterial characteristics of the CNDs-ZnO were investigated under UV irradiation at 365 nm. The experimental procedures were identical, but the bacterial plates were incubated while exposed to UV light. The results are shown in Table 2 and compared with the existing CNDs-ZnO antibacterial results in Table 1. Under UV irradiation, the photo-enhanced antibacterial effect of the CNDs-ZnO against bacteria was detected except against E. coli and S. typhimurium. CNDs exhibit antibacterial activity owing to increased oxidative stress in bacteria based on producing ROS by light or UV irradiation [4,11]. In this paper, the photo-induced antibacterial properties of CNDs were similarly demonstrated. Interestingly, recent research has shown that CNDs exert an antibacterial effect by activating ROS in the absence of light [58]. Thus, the mechanism of the antibacterial effect of CND needs to be elucidated more in further studies. Table 2. Enhanced antibacterial effect of CNDs-ZnO through UV irradiation.

Bacteria mm of Inhibition Zone (Mean ± SD)
Photo-Enhanced Antibacterial Activity UV on UV off (From Table 1)

MIC test and Growth Curve Inhibition Analysis
Results of the completed MIC test are shown in Table 3. The starting concentration was 5.8 mg/mL, which is numbered as 1 in the table. As described in Section 2.5, a total of 11 samples were prepared through 1/2 serial dilution. The as-prepared concentrations were 5.8 mg/mL, 2.9 mg/mL, 1.45 mg/mL, 725.0 µg/mL, 362.5 µg/mL, 181.25 µg/mL, 90.63 µg/mL, 45.31 µg/mL, 22.65 µg/mL, 11.33 µg/mL, and 5.66 µg/mL, which were numbered as 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, and 11, respectively. To minimize the error between each well, bacteria that were not treated with CNDs-ZnO and the CNDs-ZnO-treated bacteria were simultaneously placed up and down. After incubation for 20 h, their turbidities were measured at OD 600 . As shown in Table 3, the minimum inhibitory concentrations for each bacteria were 362.5 µg/mL, 725.0 µg/mL, 362.5 µg/mL, 90.63 µg/mL, and 181.25 µg/mL for E. coli, B. cereus, S. typhimurium, S. aureus, and V. alginolyticus, respectively. In fact, the cell growth of V. alginolyticous was not observed visually until 362.5 µg/mL of CNDs-ZnO was added. Based on the MIC test results, the growth curve inhibition for CNDs-ZnO at 1/160-diluted concentration (362.5 µg/mL) against all bacteria in LB media was additionally achieved at OD 600 during culture for 20 h. Commercial pure ZnO solution was prepared as an experimental control. Untreated bacteria were also cultivated together. All samples were prepared in 96-well plates. As shown in Figure 6a-e, except in B. cereus, CNDs-ZnO-treated bacteria noticeably showed growth inhibition compared to pure ZnOtreated or untreated bacteria. For B. cereus, the initial growth was delayed up to 10 h, but the bacteria grew to a certain extent afterward. However, the growth was significantly hindered by the CNDs-ZnO as B. cereus appeared to enter the stationary phase after approximately 18 h. In the results of the MIC test against B. cereus, some cell growth (turbidity value = 0.337 at OD 600 ) was observed in the well added with 362.5 µg/mL of CNDs-ZnO after 20 h. This cell growth inhibition analysis demonstrated the consistency of the MIC test result.

Disk Diffusion Test for Antifungal Activity
The antifungal property of the CNDs-ZnO nanocomposites was also examined using the disk diffusion test ( Figure S4). Similar to the mechanism of antibacterial activity of ZnO, the fungicidal mechanisms induced by ROS or mediation by zinc ions from ZnO are also considered to disrupt the cellular structure and anti-oxidative system of fungi [59][60][61]. In Figure S3, the inhibitory effect of CNDs-ZnO on fungal growth was more pronounced in R. mucilaginosa and A. niger with >20 mm of inhibition zone relative to that on other fungal species. Except for R. mucilaginosa and A. niger, they showed weak antifungal activity with <20 mm in halo size by CNDs-ZnO-1 and 2, and the measured inhibition zone is presented in Table 4. Especially, CNDs-ZnO-1 and CNDs-ZnO-2 showed the most effective antifungal activity against R. mucilaginosa, as indicated by inhibition zones of 24 ± 1 and 28 ± 2 mm in halo sizes, respectively. Although pure ZnO only showed weak antifungal activities against R. mucilaginosa and A. niger and no activity against other species, the inhibition sizes can be considered negligible (<10.5 mm in size). Overall, the inhibition zones of CNDs-ZnO-2 against all fungal species were 10% larger than those of CND-ZnO-1. This phenomenon may have been caused by an unidentified factor in nanocomposite synthesis due to physicochemical influences against S. horneri during drifting or after deposition on the beach. However, further investigation will be needed for a distinct cause of the assumption.

Disk Diffusion Test for Antifungal Activity
The antifungal property of the CNDs-ZnO nanocomposites was also examined using the disk diffusion test ( Figure S4). Similar to the mechanism of antibacterial activity of ZnO, the fungicidal mechanisms induced by ROS or mediation by zinc ions from ZnO are

Toxicity Evaluation of the CNDs-ZnO
Five embryos of zebrafish were selected per batch, and each batch was exposed to chlorine bleach, ZnO NPs (commercial), and serially diluted CNDs-ZnO. The toxicity of CNDs-ZnO was assessed in terms of developmental rates of embryos, which are presented in Table 5. At 24 h post-fertilization, the embryos reared in EM without any exposure to the as-prepared solutions developed to over 60% of larvae. The eggs exposed to chlorine bleach, pure ZnO, and undiluted CNDs-ZnO-1 and CNDs-ZnO-2 failed to develop; furthermore, eggs reacted with chlorine bleach disappeared within 30 min. By contrast, embryos reacted with 1/10-diluted CNDs-ZnO-1 and CNDs-ZnO-2 survived and developed to 24 h successfully. Although the developmental rate of the embryos reacted with 1/10-diluted CNDs-ZnO-1 was 80%, the embryos upon 1/10-diluted CND-ZnO-2 showed a 60% survival rate. However, the 60% survival rate against CND-ZnO-2 was probably not solely attributed to the reaction with CNDs-ZnO-2, because the developmental rate of the embryos with no exposure to the nanocomposite solutions was up to 60%. In the case of a dilution factor of 1/100 or more, all embryos showed a 100% survival rate. In summary, the embryos reacted with CNDs-ZnO at a dilution ratio of 1/10 or more resulted in an 80% survival rate.

Conclusions
This study demonstrated and highlighted the applicability of S. horneri, which is currently treated as a nuisance, for the synthesis of an antimicrobial nanocomposite. The synthesis was designed to entail minimum available equipment, small cost, and simple procedure, and to be ecologically friendly. All fabricated CNDs-ZnO nanocomposites based on S. horneri collected from two different regions in Korea successfully exhibited antibacterial and antifungal activities. Because the nanocomposite with antimicrobial properties can be synthesized and well-dispersed in aqueous solution, the limitation of poor water solubility of the current widely used zinc oxide can be overcome; thus, this nanocomposite is expected to have a wide range of potential industrial applications. Moreover, under UV irradiation, the antibacterial effect was slightly improved, and the photo-induced ROS generation was possibly caused by the carbon nanodots produced from S. horneri on the nanocomposite. This work was a proof-of-concept study to use a hitherto unutilized or veiled marine species and demonstrated a valuable possibility of a wide application prospect using many underestimated marine organisms. However, some limitations of this study still existed. It is unclear by what kind of physicochemical influence the S. horneri used in this experiment had been exposed that could affect the synthesis of the CNDs-ZnO nanocomposites while floating in the sea. Further investigation will be required by comparison with the collection of S. horneri from various regions as well as distinct compositional analysis. In addition, environmental safety and human hazards of the CNDs-ZnO must be examined for the practical industrial applications through further study.

Patents
A Korean patent application has been filed for the contents described in this paper (patent number 10-2021-0067042).