Transparent Nanocrystallite Silver for Antibacterial Coating

Ismail, W. Ahliah; Ali, Zainal Abidin; Puteh, R.

doi:https://doi.org/10.1155/2013/901452

Journal of Nanomaterials

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Research Article | Open Access

Volume 2013 | Article ID 901452 | https://doi.org/10.1155/2013/901452

Transparent Nanocrystallite Silver for Antibacterial Coating

W. Ahliah Ismail,¹Zainal Abidin Ali,¹and R. Puteh¹

Academic Editor: William W. Yu

Received18 Mar 2013

Revised27 May 2013

Accepted27 May 2013

Published11 Jun 2013

Abstract

Transparent sol-gel film with antibacterial coating property incorporating silver nanoparticles has been successfully developed. Silver nanoparticles were synthesized by precipitation method at room temperature. XRD structural studies show that crystallite sizes in the range of 18 nm to 40 nm were produced. The coating system used methyltrimethoxy silane as binder and N-propanol as diluent to obtain the highest transperancy. 2.5% wt of nanosilver crystallites was added as antibacterial agent. The coating mixture was applied onto glass plates using sponges and tested against Staphylococcus aureus, Escherichia coli, and Pseudomonas aeruginosa. Values of antimicrobial activity of 4.6, 7.2, and 4.2 were, respectively, obtained for Staphylococcus aureus, Escherichia coli and Pseudomonas Aeruginosa. Coating with antimicrobial activity greater than 2 classified as antibacterial.

1. Introduction

Antibacterial is an important branch of functional coating that plays an important role not only for general hygiene but also for saving life as disinfectant in places such as operation theatre in hospitals. Antibacterial studies are mostly evolved around Staphylococcus aureus [1], Escherichia coli [2] and Pseudomonas aeruginosa [3]. Staphylococcus aureus is frequently found in human respiratory tract and skin. It is a common cause of skin infections, respiratory disease, and food poisoning. On the other hand, Escherichia coli is commonly found in lower intestine of warm blooded organism. It usually causes the food poisoning and is occasionally responsible for product recalls due to food contamination. The third bacteria Pseudomonas Aeruginosa is considered as one of the toughest bacterial strain and able to survive in harsh environments. It does not usually cause illness to healthy people but it is described as an opportunistic organism causing serious infection when our normal defences system weakened. It represents a great threat to the most vulnerable hospital patients, for example, intensive care patients, those with depleted immune system such as cancer patients, people with serious burn, and premature babies in neonatal units.

There is enormous interest in the research of highly efficient and low-cost antibacterial surface treatments to avoid the breeding and spreading of the harmful microorganisms [4, 5]. Most of the approaches for achieving antibacterial surfaces are based on silver particles [6–9]. The silver particles provide ions which are highly toxic to bacteria. The advantage of silver as antibacterial agent is the selective toxicity to a wide range of microorganism. Over the years, studies have shown that the miniaturization of silver particles has significantly improved the performance as antibacterial agent [2, 6]. Nanoparticles with higher specific area are more efficient in releasing silver ions. Sol gel is one of the methods used to incorporate silver nanoparticles in the coating. It has several advantages such as high purity, homogeneity, and low processing temperatures. Since sol is usually applied to the surface by dip coating or spin coating, this limits the application of the coatings to only small size materials or substrates as dip or spin coater is unable to accommodate bigger material. Thus the coater itself becomes a limiting factor in the antibacterial applications.

Therefore in this work, we would like to report the antibacterial behaviour of our transparent coating against Staphylococcus aureus, Escherichia coli, and Pseudomonas aeruginosa, in which the sol was applied using only a sponge. No dip or spin coater was used. The coating has been prepared according to our previous work [10], where the details on the coating properties are available.

For antibacterial activity measurement, it is a common procedure to carry out the test according to Japanese Industrial Standard, JIS Z 2801. This method was developed to measure the antibacterial activity in hydrophobic materials, originally resulting from the incorporation of silver ions into rigid polymers. Developed by a consortium of workers comprised of manufacturers of silver-based antimicrobial agents, government-based research organisations, and universities under the organisation of the Society of Industrial technology for Antimicrobial Articles (SIAA), the method has then been validated by ring tests within Japan [11] and now forms the basis of a draft ISO standard which is being validated by the SIAA in collaboration with the International Biodeterioration Research Group (IBRG [12]). In JIS Z 2801, the antibacterial activity is measured by quantifying the survival of bacterial cells which have been held in intimate contact for 24 hours at 35°C with a surface that contains an antibacterial agent. The antibacterial property is measured by comparing the survival of bacteria on a treated material with that achieved on an untreated material.

2. Experimental Method

2.1. Nanosilver Crystal Precipitation

Silver nanocrystals were prepared according to the method reported in [13]. 20 mL of ethylene diamine was added into the silver nitrate solution and stirred for 5 minutes. Cetyltrimethylammonium bromide (CTAB) was added to the solution as a dispersing agent and stirred vigorously for another 5 minutes before adding hydrazine hydrate. The solution was stirred and kept at the room temperature for 15 minutes. The particles were separated from the solution by centrifuging the solution at 5000 rpm for 20 minutes. The particles were washed from the reactants chemicals by repeating the centrifuging process with deionised water and lastly with ethanol. The particles gathered were dried in desiccators for 24 hrs. Ball milling process with weight ratio of ball to sample 120 : 1 was carried out for 4 hours at 300 rpm. The milled particles were characterised using XRD to confirm the crystal structure and estimate the crystallite size.

2.2. Preparation of Coating Mixture for Antibacterial Testing

N-propanol and methyltrimethoxy silane (Si–CH₃–(OCH₃)₃) was mixed in a beaker with the ratio of 1 : 1. 2.5% wt of silver nanocrystal was added into the system and was grinded in the ball mill for 1 hr. Nitric acid was diluted to obtain the pH of 0.1 and was used as catalyst (10% wt). The coating process was carried out in room temperature of 26°C and absolute humidity 30%. These two factors were kept constant throughout the experiment. The dried samples were measured for transparency using haze meter with D65 illumination light at room temperature, and surface quality was evaluated using a microscope with 500x maximum magnification.

2.3. Antibacterial Activity Test

The dried sample was tested against Staphylococcus aureus, Escherichia coli, and Pseudomonas Aeruginosa according to JIS Z 2801:200 (Antimicrobial product: test for antimicrobial activity and efficacy) by an accredited testing lab (SIRIM QAS International Sdn Bhd). This ensures and guarantees reliability, accuracy, and validity of the results.

As reported by [11–13], the test microorganism is prepared by growth in a liquid culture medium. The suspension of test microorganism is standardized by dilution in a nutritive broth (this affords microorganisms the potential to grow during the test). Control and test surfaces are inoculated with 0.4 mL of the germ suspension in triplicate. Then the inoculum is covered with a film to prevent the evaporation of the suspension and to ensure close contact with the samples surface. Immediately after inoculation, the bacteria from the reference sample are separated from the sample surfaces and the number of viable germs is determined ( value) by elution followed by dilution and plating. The other samples () are allowed to incubate in a humid environment for 24 hours. After incubation, microbial concentrations are determined by elution followed by dilution and plating. Activity/efficacy is calculated by comparing the germ concentration after 24 hours relative to concentration of the blank sample after 24 hours.

3. Result and Discussion

3.1. Structural Study and Determination of Crystallite Size

The chemical route for the formation of silver nanoparticles can be described as follows [14]: In (1), the first reaction of Ag⁺ with the ethylenediamine is to form the [Ag (CH₂NH₂)₂]⁺ complex and the following reaction in (2) with the hydrazine hydrate to form silver metal. CTAB was added to disperse the particles formed. The silver precipitate produced was structurally analysed by XRD from 5° to 90° 2θ angle (Figure 1). The same peaks appeared in all of the samples and after fitting, and it is confirmed that the crystal consists of silver atoms only. There was no evidence of oxygen or other atoms existed in the crystal structure. The crystals formed are face-centered cubic structure.

Estimation of silver crystallite size was made through Lorentzian curve fit to the strongest peak in the XRD pattern Ag which is from 37° to 42°. XRD testing was repeated for all the samples zoomed in at the angle of 2θ from 37° to 42°. β and θ of every sample were determined from the peak, and through Scherrer Equation the crystallite size of the samples was calculated and shown in Figure 2.

From Figure 2, it clearly shows that at the molarity of 0.3 M to 0.5 M the crystallite size was the smallest. Size of the silver crystals formed is one of the most important factors in determining the antibacterial efficiency of the silver to fight the microbes. This is attributed to the high surface area to volume ratio and the quantum confinement effect caused by extremely reduced size (i.e., electron confinement in a small area) [15]. The nanocrystallite silver that was synthesised from 0.3 M was then used for the antibacterial testing.

3.2. Antibacterial Test Result

Figure 3 shows three glass surfaces that have been applied with the antibacterial coating. Slide A was the uncoated glass whereas slide B and C both were coated with 2.5% and 3.5% of Ag. The coating was transparent. The presence of Ag nanoparticles powder is visible on the surface when the slides were tilted to a certain angle (Figure 3(b)). As has been reported [12], the haze value for 2.5% was 3.42.

(a)

(b)

Figure 4 compares the transparency of the slides optically. The transparency level decreases as the amount of Ag increases from 2.5% to 3.5%. As the coating was purposely developed for surface treatment, it should cause only minimal effect to the applied surface in term of colour and level of haziness.

(a)

(b)

(c)

The results for antibacterial test against Staphylococcus aureus, Escherichia coli and Pseudomonas Aeruginosa according to JIS Z 2801 (antimicrobial product test for antimicrobial activity and efficacy) of the coating are shown in Table 1.

Coating with antimicrobial activity greater than 2 is classified as antibacterial. The antibacterial test result clearly shows value of antimicrobial activity of 4.6 for Pseudomonas Aeruginosa, 7.2 for Escherichia coli, and 4.2 for Staphylococcus aureus. All the values exceeded that of value 2 which confirmed the antibacterial coating and therefore comply with the standard of JIS Z 2801.

In order to verify that the antibacterial properties come only from the Ag nanoparticles and not from the sol-gel formulation, we carried out antibacterial tests to slides coated with only the sol gel (no Ag nanoparticles were used). The noncoated slides were used as controls. The results in Table 2 show that the number of bacterial is increased after 24 hours for all types of bacteria for the sol-gel-coated slides. This verifies and proves that the sol gel does not kill and thus has no antibacterial properties.

Antibacterial nanocrystallite silver may work in two ways; firstly, it breaks through the permeability of outer membrane, resulting in the leakage of cellular materials. It is well known that bacteria possess an outer membrane to serve as a selective permeability barrier which protects bacteria from harmful agents, such as detergents, drugs, toxins, and degradative enzymes, and penetrating nutrients to sustain bacterial growth. Kim et al. [16] reported studies based on S. aureus and E. coli that the free radicals could induce bacterial cell membrane damage by enhancing the permeability of the membrane. The bacteria will then undergo a protein leakage as a result of the increasing membrane permeability.

Secondly, as a result of the increasing permeability nanocrystallite silver can enter the inner membrane and inactivate respiratory chain dehydrogenases, thus inhibiting respiration and growth of cells. Holt and Bard proved this by showing that Ag⁺ can inhibit the respiration of E. coli by determining change of oxygen dissolved in culture resolution [17]. A report [18] on Pseudomonas aeruginosa also suggested that silver nanoparticles not only inhibited the growth but also the ability of the organism to synthesize the exopolysaccharide. The exopolysaccharide functions not only to protect the bacteria from the host defense mechanism but also mediate the adhesion of the organism to the surface. At the same time, the silver could as well affect some proteins and phosphate lipids and induce collapse of membrane, resulting in cell decomposition and death eventually. This is supported by Kim et al. [19] who found that Ag⁺ interacted with thiol (–SH) group of cysteine by replacing the hydrogen atom to form –S–Ag, thus hindering the enzymatic function of affected protein to inhibit growth of E. coli.

The most attractive aspects of this work are the simplicity of the coating method and its effectiveness in killing the bacteria. As has been reported, the coating was applied using only a melamine sponge which means that everybody could use it. No special expertise is required. Moreover, it would provide a simple and cheaper way for medical rooms and facilities (e.g., wall, floor, and table) to be bacterial-free environment anytime required.

4. Conclusion

We managed to develop an antimicrobial coating layer that is very easy to apply and dry in the room temperature. The coating is very transparent, clear, and will not change the original property of the substrate. It is very suitable for the window glasses, wall, and floor coating. The best formulation was obtained from formulation 1 : 1 ratio of methyltrimethoxy silane to N-propanol. The coating shows the antibacterial activity to gram-positive (Pseudomonas Aeruginosa and Escherichia coli) and gram-negative (Staphylococcus aureus) bacteria strain.

Acknowledgment

The authors are thankful to University of Malaya and Fundamental Research Grant Scheme (FRGS)-FP 054-2010B for providing the necessary facilities and funding for this research.

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Copyright

Copyright © 2013 W. Ahliah Ismail et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

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