In vitro assessment of the antimicrobial activity of silver and zinc oxide nanoparticles against fish pathogens

Background Antibiotic resistance is a global issue that threatens public health. The excessive use of antibiotics contributes to this problem as the genes of antibiotic resistance can be transferred between the bacteria in humans, animals and aquatic organisms. Metallic nanoparticles could serve as future substitutes for some conventional antibiotics because of their antimicrobial activity. The aim of this study was to evaluate the antimicrobial effects of silver and zinc oxide nanoparticles against major fish pathogens and assess their safety in vitro. Silver nanoparticles were synthesized by chemical reduction and characterized with UV–Vis spectroscopy, transmission electron microscopy and zeta sizer. The concentrations of silver and zinc oxide nanoparticles were measured using inductively coupled plasma-mass spectrometry. Subsequently, silver and zinc oxide nanoparticles were tested for their antimicrobial activity against Aeromonas hydrophila, Aeromonas salmonicida subsp. salmonicida, Edwardsiella ictaluri, Edwardsiella tarda, Francisella noatunensis subsp. orientalis, Yersinia ruckeri and Aphanomyces invadans and the minimum inhibitory concentrations were determined. MTT assay was performed on eel kidney cell line (EK-1) to determine the cell viability after incubation with nanoparticles. The interaction between silver nanoparticles and A. salmonicida was investigated by transmission electron microscopy. Results The tested nanoparticles exhibited marked antimicrobial activity. Silver nanoparticles inhibited the growth of both A. salmonicida and A. invadans at a concentration of 17 µg/mL. Zinc oxide nanoparticles inhibited the growth of A. salmonicida, Y. ruckeri and A. invadans at concentrations of 15.75, 31.5 and 3.15 µg/mL respectively. Silver nanoparticles showed higher cell viability when compared to zinc oxide nanoparticles in the MTT assay. Transmission electron microscopy showed the attachment of silver nanoparticles to the bacterial membrane and disruption of its integrity. Conclusions This is the first study on inhibitory effects of silver and zinc oxide nanoparticles towards A. salmonicida and A. invadans. Moreover, zinc oxide nanoparticles inhibited the growth of Y. ruckeri. In low concentrations, silver nanoparticles were less cytotoxic than zinc oxide nanoparticles and represent an alternative antimicrobial compound against A. hydrophila, A. salmonicida and A. invadans.


Background
Increases in global fish consumption have resulted in greater development and intensification of aquaculture worldwide [1,2] which have led to a massive use of antibiotics for promoting growth and prophylaxis, especially in intensive aquaculture [2]. The EU has prohibited the use of antibiotics as growth promoters in animals since 2006 [3]. However, it is difficult to assess the quantity and identify the classes of antimicrobial agents in aquaculture [4]. Tuševljak et al. [5] conducted a survey of fish

Open Access
Acta Veterinaria Scandinavica *Correspondence: mansour.el-matbouli@vetmeduni.ac.at 1 Clinical Division of Fish Medicine, University of Veterinary Medicine, Veterinärplatz 1, 1210 Vienna, Austria Full list of author information is available at the end of the article farms in 25 countries in North America, South America, Europe, Africa and Asia, and found that tetracycline and quinolones are applied frequently, especially in salmon aquaculture. Nevertheless, detailed investigations about the types and the amounts of antibiotics in fish farms are still needed [4,6]. The problem of antibiotic resistance has become a major concern in human and veterinary medicine [2,3,7]. The antibiotic resistance genes could be transferred between bacteria from different environments. Sharing of such genes occurs between bacteria which infect aquatic animals, terrestrial animals and humans, and thereby poses a hazard to animal and human health [7]. The closing statement of the joint science ministers meeting at the G8 summit in 2013 emphasized that antimicrobial resistance is one of the most important global health challenges in the 21st century. At the same time, bacterial, viral, mycotic and parasitic fish diseases constitute a massive threat to the aquaculture industry [8]. Aeromonas hydrophila is a major bacterial pathogen, which causes dermal ulceration and haemorrhagic septicemia in many fish species [9]. Aeromonas salmonicida was one of the first discovered causative agents of fish diseases, and is a widely-occurring pathogen of salmonids, which causes septicemia with high mortality rates [10,11]. Edwardsiella ictaluri is responsible for enteric septicemia of channel catfish (Ictalurus punctatus), while Edwardsiella tarda is the causative agent of emphysematous putrefactive disease in the same species [12,13]. Francisella noatunensis subsp. orientalis is an intracellular bacterial pathogen, which infects tilapia and produces a chronic granulomatous inflammation [14]. Yersinia ruckeri is the causative agent of enteric red mouth disease (ERM), which causes a wasting condition in fish and result in cumulative mortalities with high economic losses in fish farms [15,16]. In spite of the production of a commercial vaccine against motile and non-motile strains of Y. ruckeri, field cases of vaccination failure have been reported [17]. Oomycete infections caused by Aphanomyces invadans induce skin ulcerations that extend deep into the underlying muscles leading to high morbidity and mortality in fish during outbreaks of epizootic ulcerative syndrome (EUS) [18]. Sørum [7] has reported the emergence of antibiotic resistant strains of A. hydrophila, A. salmonicida, and Y. ruckeri in fish farms. One of the recent strategies to combat microbes and multi-drug resistant bacteria is the application of metallic nanoparticles, which exhibit antimicrobial activities [19][20][21][22].
Silver nanoparticles show antibacterial effects against A. hydrophila, Aeromonas bestiarum, Pseudomonas flourescens, E. tarda, Vibrio harveyi, Proteus spp. and Flavobacterium spp. [23][24][25][26][27][28]30] and inhibit the growth of multiple drug resistant isolates of Staphylococcus aureus, Micrococcus luteus and Klebsiella pneumonia [31,32]. One advantage of silver nanoparticles over conventional antibiotics is that their antimicrobial action arises through interference with multiple cellular processes of the bacteria, so the emergence of resistance is less likely [33]. Exact mechanisms that underlie the antibacterial actions of silver nanoparticles are not completely understood [34,35]. However, modes of action have been suggested by different researchers [22,[33][34][35][36] and include the interaction of the silver nanoparticles with the bacterial cell wall, production of reactive oxygen species (ROS), interaction with DNA, and release of Ag + ions.
Similarly, zinc oxide nanoparticles exhibit potent antimicrobial activities [29,30,37], which are suspected of arising through complex mechanisms of action that include release of Zn 2+ ions, production of ROS and interference with bacterial replication by inhibition of cellular processes like glycolysis, acid tolerance and transmembrane proton translocation [36,38].
In this study, we investigated the antibacterial and antifungal activity of silver and zinc oxide nanoparticles against A. hydrophila, A. salmonicida subsp. salmonicida, E. ictaluri, E. tarda, F. noatunensis subsp. orientalis, Y. ruckeri and A. invadans. We also assessed cytotoxicity and host cell viability using an MTT assay after incubating nanoparticles with eel kidney-1 cells (EK-1).

Materials
Silver (≈100 nm) and zinc oxide (≈66 nm) nanoparticles were purchased from Sigma-Aldrich, Austria. Chemicals and reagents used for silver nanoparticles synthesis [silver nitrate, sodium citrate tribasic hydrate, sodium borohydride, polyvinyl pyrrolidone (PVP) and de-ionized water] were also purchased from Sigma.

Silver nanoparticles synthesis
All beakers and cylinders were thoroughly cleaned and autoclaved before use and deionized water was used for the synthesis. Silver nanoparticles synthesis was carried out by the chemical reduction method as previously described [39]. Briefly, silver nitrate was used as a source of silver, sodium borohydride solution was used as a reducing agent, and PVP acted as a stabilizing agent to prevent particles agglomeration [40]. Sodium citrate tribasic hydrate functions as both reducing and stabilizing agent at the same time, besides, the combination of PVP and sodium citrate increases the stability of the newly formed nanoparticles [41]. Silver nitrate was dissolved completely in de-ionized water then sodium citrate tribasic hydrate and PVP were added. After complete dissolving, sodium borohydride solution was added to the mixture and stirred for 30 min. The color of the solution changed from colorless to brown indicating the formation of silver nanopaticles.
As silver nanoparticles are sensitive to light, they were kept dark in a clean autoclaved bottle at 4 °C.

Characterization of silver nanoparticles
The absorption spectra were determined using a UV-Vis spectrophotometer (NanoDrop 2000 ® , Thermo Fischer Scientific, Massachusetts, USA) against the spectrum of deionized water as a blank. All measurements were performed at room temperature on 3 separate days.
Morphology of the synthesized nanoparticles was investigated using transmission electron microscopy (EM 900, Zeiss, Oberkochen, Germany) operating at an accelerating voltage of 80 kV. One drop of silver nanoparticle solution was deposited on the carbon-coated copper grid then left to evaporate at room temperature forming a monolayer. The mean size of the particles was calculated using (Image SP Viewer ® ) software to measure 100 randomly sampled nanoparticles.
Nanoparticles size distribution and zeta potential were measured based on the dynamic light scattering (DLS) using a Malvern zeta sizer Nano ZS ® device. Three separate measurements on different days were performed at room temperature.

Determination of nanoparticles concentration
Elemental concentrations of the nanoparticle solutions were measured using inductively coupled plasma-mass spectrometry (ICP-MS). Milli-Q water and nitric acid were used in all samples, with elemental standards for ICP-MS measurements from CPI international (Amsterdam, The Netherlands). Samples were digested in nitric acid using a microwave discover SP-D system (CEM Microwave Technology, Germany) with parameters: temperature 200 °C; ramp time 4 min; hold time 6 min; maximum power 300 W. Digested samples were diluted with Milli-Q water to give nitric acid concentrations lower than 3% and zinc and silver concentrations lower than 20 ng/g. ICP-MS measurements were performed according to Theiner et al. [42] using an ICP-quadrupole MS instrument Agilent 7500ce (Agilent Technologies, Waldbronn, Germany) equipped with a CETAC ASX-520 autosampler (Nebraska, USA) and a MicroMist nebulizer, at a sample uptake rate of approx. 0.25 mL/min. The instrument was tuned daily, and rhenium served as an internal standard for zinc and silver. The ICP-MS was equipped with nickel cones and operated at an RF power of 1550 W. Argon was used as plasma gas with a flow of 15 L/min and as a carrier gas with a flow of ~1.1 L/min. The dwell time was set to 0.3 s and replicates of 10 measurements were taken. Agilent MassHunter ® (Workstation Software, Version B.01.01, 2012) was used for data processing.

Bacterial growth inhibition test
A single bacterial colony from each strain was inoculated in brain heart infusion (BHI) broth (Sigma-Aldrich) except for F. noatunensis which was inoculated in modified Müller-Hinton II cation-adjusted broth (Sigma-Aldrich) enriched with 2% IsoVitalex (Becton-Dickinson). After inoculation, all isolates were incubated in a shaking incubator (144 rpm) at 22 °C for 24 h, except for A. salmonicida which was incubated at 15 °C for 48 h. A spectrophotometer (Eppendorf BioPhotometer ® , Eppendorf, Hamburg, Germany) was used to determine the optical density (OD 600 ). Bacterial cultures were diluted with BHI broth to adjust their concentration at 10 6 CFU/mL, which was confirmed by plate counting. Equal volumes of each nanoparticle solution and each bacterial strain were mixed to reach a final concentration of 5 × 10 5 CFU/mL. A negative control was prepared by mixing equal volumes of bacteria and deionized water. All samples were then incubated overnight in a shaking incubator at the same conditions as above. After that, 100 µL of each sample was streaked on Müller Hinton agar plate (Sigma Aldrich) or cystine heart agar supplemented with 2% horse blood and incubated in a static incubator to observe the bacterial growth, according to Bresee et al. [43]. The test was performed in triplicate.

Minimal inhibitory concentration (MIC)
Nanoparticles that inhibited bacterial growth were subjected to the minimal inhibitory concentration (MIC) assay in triplicate, according to Swain et al. [30] with some modifications. Double fold serial dilutions of nanoparticles were added to the cultures containing 10 6 CFU/ mL of bacteria and incubated as before. Then 100 µL of each was streaked on Müller Hinton agar plates. The double fold serial dilutions were prepared for each nanoparticle solution up to five times to determine the MIC value at which no bacterial growth on the plate was observed.
The effect of silver and zinc oxide nanoparticles on bacterial growth kinetics in BHI broth was measured using Eppendorf ® spectrophotometer at 600 nm. The determined MICs of silver and zinc oxide nanoparticles were applied in this assay. Oxytetracycline (25 µg/mL) and bacterial cultures only were used as positive and negative controls, respectively. The absorbance values (OD 600) were recorded at 4, 8, 12, 16, and 24 h. The experiment was performed in triplicate.

Fungal growth inhibition test
Silver and zinc nanoparticles were tested for their inhibitory effects against A. invadans. The fungus was isolated from infected dwarf gourami (Colisa lalia). It was grown on glucose-peptone (GP) agar and incubated at 26 °C for 5 days [18]. An anti-fungal assay was conducted as described by Mori et al. [44] with some modifications. Mycelia from the periphery of the growing fungus (about 1 mm) were inoculated in 2 mL GP broth in 10 mL falcon tubes. Equal volumes (2 mL) of each tested nanoparticle solution were added to the broth. An equal volume (2 mL) of deionized water was added to one tube as a negative control. All tubes were incubated at 26 °C for 5 days. Then, 100 µL of broth from each tube was inoculated in the center of a GP agar plate and incubated again at 26 °C for 5 days to monitor fungal growth or inhibition. Nanoparticles that inhibited the fungal growth were further diluted in twofold serial dilutions to determine the MIC. The experiment was performed in triplicate.

Assessment of cytotoxicity via MTT assay
We assessed three concentrations of silver and zinc oxide nanoparticles for their cytotoxicity, to determine the safety of these concentrations as therapeutants in vitro. Nanoparticle concentrations were chosen based on our MIC data. Eel kidney cells (EK-1) were used in 96-well plates at approximately 1.5 × 10 4 cells per well in L-15 medium + GlutaMAX (Gibco) supplemented with 10% fetal bovine serum (FBS) and antibiotics (Penicillin100 IU/mL and streptomycin 100 μg/mL). After 24 h incubation at 26 °C, three concentrations of silver (8.5, 17, 25.5 µg/mL) and zinc oxide nanoparticles (7.88, 15.75, 23.63 µg/mL) were added to the EK-1 cells; cells with medium alone served as negative controls. The medium was then removed and wells were washed with phosphate buffered saline (PBS) twice to remove any residual nanoparticles. Subsequently, cell viability was assessed by incubating the triplicate wells of silver and zinc oxide nanoparticles, negative control cells and blank (medium only) with MTT (3-[4,5-dimethylthiazol-2-yl]-2,5-diphenyl tetrazolium bromide, Sigma-Aldrich). MTT assay was performed as described by Mosmann [45]. 10 µL of the MTT (5 mg mL −1 dissolved in PBS) per 100 µL media were added to each well and incubated for 3 h at the same temperatures as described above. After that, 100 µL of MTT solubilization solution (Sigma-Aldrich) was added into each well to solubilize formazan crystals, and mixed using a rotatory shaker. The absorbance values of each well were recorded at 570 nm using EnSpire ® multimode plate reader. Triplicate tests were performed for each concentration and the control. After blank correction, the percentage of cell viability was calculated as the optical density values of nanoparticlestreated cells/the mean optical density of non-treated control cells ×100. Data were analyzed using one-way ANOVA test with SPSS ® 16.0 software.

Ultrastructural interaction between silver nanoparticles and A. salmonicida
Aeromonas. salmonicida was incubated in BHI broth at 15 °C for 2 days, as described by Bresee et al. [43] with some modifications (Pellet was fixed with 5% glutaraldehyde in 0.1 M PBS for 4 h instead of overnight fixation with 2.5% glutaraldehyde in 0.1 M sodium cacodylate buffer). The culture was adjusted to 2.1 × 10 8 CFU/mL, then, 1 mL added to 1 mL of silver nanoparticles (34 µg/ mL), and incubated for 1 h at room temperature. The mixture was centrifuged at 11,600×g for 15 min, then the pellet was re-suspended in 1 mL PBS. Centrifugation was repeated with the same conditions. The pellet was fixed with 500 µL of glutaraldehyde (5% in 0.1 M PBS) at 4 °C for 4 h. Glutaraldehyde was removed and the pellet washed twice with 0.1 M PBS and incubated overnight at 4 °C. The pellet was post-fixed in 1% osmium tetroxide for 2 h at 4 °C and washed twice with PBS. Samples were dehydrated using graded alcohol series (70, 96 and 100%) before a 1:1 mixture of glycidyl ether and propylene oxide was added for 45 min then incubated overnight with a 3:1 mixture of glycidyl ether and propylene oxide. Samples were embedded in gelatin capsules then ultrathin sections were prepared using an ultramicrotome. For transmission electron microscopy (TEM) imaging, we used an EM 900 (Zeiss ® , Oberkochen, Germany) and Image SP Viewer ® software.

Characterization of silver nanoparticles
UV-Vis analysis of the synthesized silver nanoparticles showed a sharp absorption peak (0.806) at 395 nm (Fig. 1a). TEM images of the synthesized silver nanoparticles showed they were spherical (Fig. 1b), with a mean diameter of 21 nm (range of sizes 11-39 nm). DLS showed two peaks: a smaller peak at 8.3 nm and a larger peak at 44.5 nm (Fig. 1c), which indicated the presence of two populations of silver nanoparticles, zeta potential value was −30.7 ± 0.45 mV.

Determination of nanoparticles concentration
ICP-MS measurements revealed a silver concentration of 34 µg/mL in the synthesized silver nanoparticles and 16 µg/mL in the commercial silver nanoparticles. The concentration of zinc in zinc oxide nanoparticles was 63 µg/mL. Sizes and concentrations of nanoparticles are summarized in Table 1.

Bacterial growth inhibition test
The synthesized silver nanoparticles and the commercial zinc oxide nanoparticles exhibited antibacterial activity against A. hydrophila, A. salmonicida and Y. ruckeri. However, they were not able to inhibit the growth of E. ictaluri, E. tarda and F. noatunensis. Commercial silver nanoparticles did not inhibit bacterial growth of the strains in this study ( Table 2).

Minimal inhibitory concentration (MIC)
The growth of both A. hydrophila and A. salmonicida was inhibited completely after incubation with the synthesized silver nanoparticles at 17 µg/mL or zinc oxide nanoparticles at 15.75 µg/mL. This was confirmed by the absence of bacterial growth on Müller Hinton agar Fig. 1 Characterization of silver nanoparticles. a UV-Vis analysis of silver nanoparticles showed peak absorption (0.806) at 395 nm, which matches with the surface plasmon resonance of silver nanoparticles, b TEM micrograph showing the morphology of silver nanoparticles: they are spherical with a mean size of 21 nm. (scale bar = 50 nm), c particle size distribution of the synthesized silver nanoparticles, showing two peaks: a smaller peak at 8.3 nm and a larger peak at 44.5 nm, which indicate presence of two particle size populations plates (Figs. 2, 3), and the complete inhibition of bacterial growth in BHI as observed by a spectrophotometer (Fig. 4a, b). The growth of Y. ruckeri was inhibited after incubation with zinc oxide nanoparticles at 31.5 µg/mL ( Table 2). That was confirmed by OD 600 measurements, which indicated complete inhibition of bacterial growth after incubation with zinc oxide nanoparticles at 24 h. In contrast, oxytetracycline (25 µg/mL) failed to reach complete inhibition of Y. ruckeri at the same time point (Fig. 4c).

Fungal growth inhibition test
Silver and zinc oxide nanoparticles inhibited A. invadans growth in both GP broth and agar. After double fold serial dilutions, the MIC values were 17 and 3.15 µg/ mL for synthesized silver and zinc oxide nanoparticles, respectively ( Table 2).

Assessment of cytotoxicity via MTT assay
Viability of EK-1 cells varied widely between silver and zinc oxide nanoparticles. The cells viability after addition 8.5 µg/mL of synthesized silver nanoparticles showed no significant difference (P ≤ 0.05) when compared with non-treated control cells. After incubation of the cells with 17 and 25.5 µg/mL of silver nanoparticles the cell viability measured 69.1 and 63% respectively (Table 3). For zinc oxide nanoparticles, all concentrations resulted in 100% cell death.

Ultrastructural interaction between silver nanoparticles and A. salmonicida
Silver nanoparticles were observed attached to the outer membrane of A. salmonicida (Fig. 5a). At two-times higher magnification, we observed that silver nanoparticles induced widening of periplasmic space (arrowhead), and caused diffuse intra-cytoplasmic edema (arrow) (Fig. 5b). Smaller nanoparticles (8 nm) were observed inside the bacterial cytoplasm (arrow) (Fig. 5c). Finally, silver nanoparticles disrupted the bacterial cell membrane, leading to complete cell lysis and leakage of intracellular content (Fig. 5d).

Discussion
Infectious diseases caused by parasites, bacteria, fungi and viruses constitute major threats to cultured fish [8]. Concurrently, there is a need to minimize use of antibiotics in farming, to combat antibiotic resistance [3,4]. Thus, there is a growing need for alternative antimicrobial therapeutics, and metal and metal oxide nanoparticles are being widely investigated for their potential medical applications, including their use in fish medicine [22].
In this study, we investigated the antibacterial and antifungal effects of commercially obtained zinc oxide and silver nanoparticles, and synthesized silver nanoparticles in-house. For this synthesis, we used PVP as a capping agent, to stabilize the nanoparticles and prevent them from aggregating [46], with the direct benefit that PVP-capped nanoparticles are an ideal form for administration in water for fish. UV-Vis analysis of the synthesized silver nanoparticles showed absorbance peak at 395 nm which lies in the spectrum range of silver nanoparticles and confirms the successful synthesis [47,48]. The analysis of the size distribution of silver nanoparticles using zeta sizer revealed the presence of two peaks, one peak at 8.3 nm and a larger peak at 44.5 nm, which indicates the presence of two populations of silver nanoparticles where the majority of particles were located under the larger peak with mean size of 44.5 nm. TEM images confirmed that silver nanoparticles were spherical in shape, with an average particle size of 21 nm. While TEM provides the morphology and the mean size of the nanoparticles, zeta sizer indicates the real size distribution.
In our study, silver nanoparticles showed antibacterial activity against A. hydrophila which agreed with the results from previous studies [23,25,30]. Also, zinc oxide nanoparticles exhibited antibacterial activity against A. hydrophila which corresponded with Swain et al. [30]. However, in our study the MIC was measured at 15.75 µg/mL which is lower than their results which ranged from 250 to 2500 µg/mL. This difference is mostly due to the variation in the size of the nanoparticles used when comparing these two studies. The particle size along with the concentration plays a crucial role in the antibacterial properties of the nanoparticles. Smallersized nanoparticles have a higher surface area which increases their antibacterial activity [38].
To the best of our knowledge, this is the first study to demonstrate the inhibitory effects of silver and zinc oxide nanoparticles against A. salmonicida and A. invadans, in addition to the inhibitory effect of zinc oxide nanoparticles against Y. ruckeri [49].
Synthesized silver nanoparticles at a concentration of 17 µg/mL were capable of complete inhibition of the growth of both A. salmonicida and A. invadans. In comparison, oxytetracycline (25 µg/mL) required longer time to inhibit the growth of A. salmonicida as shown in Fig. 4b.
Using MTT assay, there was no significant difference between the lowest concentration of silver nanoparticles (8.5 µg/mL) and the control group. Silver nanoparticles were less cytotoxic to EK-1 cells when compared with zinc oxide nanoparticles. However, higher concentrations of silver nanoparticles were reported as cytotoxic and genotoxic to the fish cell lines and zebrafish [50].
Commercial silver nanoparticles failed to inhibit the bacterial growth of the tested pathogens in this study, possibly due to their lower concentration and bigger particle size in comparison with the synthesized silver nanoparticles.
Residual silver nanoparticles in the aqueous environment bind to organic and inorganic sulfur in sea or fresh water. Sulfidation of silver nanoparticles leads to significant decrease of their toxicity due to the lower solubility of the resulting silver sulfide and thus cause low detrimental impact on the environment [51].
Zinc oxide nanoparticles inhibited the growth of A. hydrophila and A. salmonicida at a concentration of 15.75 µg/mL, which is near to the MICs of silver nanoparticles.
Zinc oxide nanoparticles (31.5 µg/mL) inhibited the growth of Y. ruckeri, while oxytetracycline could not completely inhibit the growth of Y. ruckeri after 24 h (Fig. 4c).
Moreover, zinc oxide nanoparticles showed a strong antifungal activity against A. invadans at concentration of only 3.15 µg/mL, which was much lower than the MIC of silver nanoparticles against the same fungus. Unfortunately, the zinc oxide nanoparticles were highly toxic against the EK-1 cell line at all concentrations (7.88, 15.75, 23.63 µg/mL). These results are in accordance with Fernández et al. [52] who report high sensitivity of RTG-2, RTH-149 and RTL-W1 fish cell lines to zinc oxide nanoparticles. The observed cytotoxicity may be attributed to release of free Zn +2 ions [53,54].
When zinc oxide nanoparticles are released into the aquatic environment, their behavior is controlled by water environment such as oxygen level, pH, ionic strength and amount of organic matter. Due to the high ionic strength in sea water, the zinc oxide nanoparticles tend to aggregate and become less mobile [55], while in fresh water they tend to dissolve rapidly which increases the risk of acute toxicity for aquatic organisms [56].
We investigated the interaction between silver nanoparticles and A. salmonicida on the ultrastructural level. TEM showed larger nanoparticles (>20 nm) bound to the bacterial cell membrane (Fig. 4), thereby presumably interfering with its integrity and function. Smaller particles (8 nm) were observed inside the bacterial cytoplasm (Fig. 4c). These observations were in concordance with previous reports [35,57]. Presence of nanoparticles in the cytoplasm suggests that the small-sized nanoparticles could pass through the S-layer pores, which range from 2 to 8 nm in diameter as described in A. salmonicida Fig. 4 Absorbance values (OD 600) measurements for the bacterial cultures only and after incubation with silver nanoparticles, zinc oxide nanoparticles or oxytetracycline, a OD 600 values for A. hydrophila, b OD 600 values for A. salmonicida, c OD 600 values for Y. ruckeri. AgNPs silver nanoparticles (17 µg/mL), ZnONPs zinc oxide nanoparticles for A. hydrophila and A. salmonicida (15.75 µg/mL) and for Y. ruckeri (31.5 µg/mL), OT oxytetracycline (25 µg/mL) [58]. In the cytoplasm, the particles would be able to react directly with the intracellular components and mechanisms.

Conclusions
Due to their high antimicrobial activity and low environmental and cytotoxic effects, silver nanoparticles can be used as an effective antimicrobial agent against A. hydrophila, A. salmonicida and A. invadans. This represents a proof-of-concept for the consideration of silver Table 3 Effect of different silver nanoparticles concentrations (0, 8

.5, 17, 25.5 µg/mL) on EK-1 cells viability
The values are expressed as mean ± SD. Different letters (a, b) in the same column means that they are significantly different (P ≤ 0.05) nanoparticles in novel therapeutics development and disease management in aquaculture. Additional in vivo studies are needed to investigate the efficacy and safety of the silver nanoparticles in the living fish.