利用粘液红酵母绿色合成氯化银纳米颗粒

I. Ghiuta, D. Cristea, R. Wenkert, D. Munteanu
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Introduction The development of materials and structures at nanoscale dimensions has gained a huge interest in the nanomaterials and nano-technology research fields. One of the most important properties of metallic nanoparticles is their antimicrobial activity. Eco-friendly methods concerning nanomaterials synthesis present a substantial importance for biological applications, mainly due to nontoxic substances and environmentally friendly procedures employed [1]. Green synthesis of silver chloride nanoparticles has been reported to be mediated by different kinds of organisms, from bacteria to plant extracts. Cell-free culture supernatant of Streptomyces strain, Klebsiella planticola, biomass of Bacillus subtilis, leaf extract of Cissus quadrangularis, aqueous extract of Sargassum plagiophyllum, extract from needles of Pinus densiflora, Prunus persica L. outer peel extract are just a few examples of organisms able to synthesize AgCl NPs [2]-[8]. Weili Hu et al. have presented the synthesis of silver chloride nanoparticles under ambient conditions in nanoporous bacterial cellulose membranes as nanoreactors. It has been demonstrated that the synthesized silver chloride nanoparticles exhibited high hydrophilic ability and a strong antimicrobial activity against Staphylococcus aureus and Escherichia coli bacteria [9]. The antibacterial effect of biosynthesized AgCl NPs investigated against Escherichia coli was found to be dose-dependent [6]. The biosynthesized silver chloride nanoparticles exhibited besides the antimicrobial activity, cytotoxicity activity against HeLa and SiHa cancer cell lines [2]. Powder Metallurgy and Advanced Materials – RoPM&AM 2017 Materials Research Forum LLC Materials Research Proceedings 8 (2018) 28-34 doi: http://dx.doi.org/10.21741/9781945291999-4 29 M. Sophocleous and J. K. Atkinson have described in their review the significant development of Ag/AgCl screen printed sensors [10]. Moreover, Ag/AgCl NPs are examined for further applications of nanoparticles as a plasmonic photocatalyst [6]. The reports which have shown the importance of the AgCl NPs application, from sensors, catalysts, to antimicrobial activity, have led to the research results presented herein. Even though several methods to obtain nanoparticles are currently developed, the green methods have captured the interest of researchers due to their lack of toxicity. In the present work, the green synthesis of silver chloride nanoparticles is described. This is, to the best of our knowledge, the first report for green synthesis of AgCl NPs mediated by Rhodotorula Mucilaginosa. Materials and Methods 1. Fungi and culture conditions The fungi Rhodotorula Mucilaginosa used in this study were provided from Soroka University Medical Center from Beersheva, Israel. The fungi were cultivated in the solid media, Sabouraud agar supplied by Scharlau Chemicals, and incubated at 35 °C for 48 h. 2. Biosynthesis of AgCl nanoparticles using Rhodotorula Mucilaginosa In order to synthesize the silver chloride nanoparticles, 1μl of bacterial strains were freshly inoculated in test tubes containing 15 ml of growth medium, namely Brain Heart Infusion from Sigma Aldrich. The liquid media contained beef heart (infusion from 250 g), 5 g/L; calf brains (infusion from 200 g), 12.5 g/L; disodium hydrogen phosphate, 2.5 g/L; D(+)-glucose, 2 g/L; peptone, 10 g/L; sodium chloride, 5 g/L. The liquid culture was kept in a thermostat at 35 °C for 24 h, followed by centrifugation at 4000 rpm for 30 min. The supernatant and biomass were tested in parallel. In the first situation 5 ml of supernatant was used, while for the second one the biomass was kept with the addition of 5 ml of distilled water. The next step was similar by adding the 5-ml culture over 40 ml Ag NO3 precursor solution, at 1 mM, 2 mM and 3 mM concentration, respectively. The culture, supernatant and biomass + distilled water and precursors were kept as control. The samples were kept in a thermostat set at 35 °C, for 48 h. 3. Characterization of AgNPs Ultraviolet-visible spectral analysis was carried-out by using Jasco V-630 spectro-photometer. The UV-visible spectra were measured in the range 200-600 nm with a wavelength step size of 1.5 nm. For morphological characteristics and chemical composition, a JSM 7400f scanning electron microscope (SEM) with a platform for Energy Dispersive Spectroscopy (EDS) was used. The silver chloride nanoparticles colloid was dropped on a copper grid and coated with a platinum thin film. After this the samples were mounted on a double sided adhesive carbon-tape. The acceleration voltage was fixed to 10kV. The crystalline nature of silver chloride nanoparticles was analyzed by XRD using a Philips PW 1050/70 X-ray powder diffractometer with graphite monochromator using CuKα1 (λ =1,54Å), at a voltage of 40 kV, a current of 28 mA, in the scan range 10÷80 °, in Bragg-Brentano geometry. Results and Discussion After incubation in the thermostat for 48 h at 35 °C, the final color of the colloid, containing biomass of Rhodotorula Mucilaginosa, changed from light yellow to light brown. The change in color is an indication for the formation of nanoparticles. In Fig.1 the obvious difference in color can be observed, depending on the precursor concentration. The samples with supernatant and the control have remained unchanged. Furthermore, considering the optical indication (changing the color), the UV-visible absorption spectra of the colloidal solutions with nanoparticles was measured (shown in Fig. 2). Powder Metallurgy and Advanced Materials – RoPM&AM 2017 Materials Research Forum LLC Materials Research Proceedings 8 (2018) 28-34 doi: http://dx.doi.org/10.21741/9781945291999-4 30 Fig. 1. Image of colloidal nanoparticles synthesized in the presence of Rhodotorula Mucilaginosa. 200 300 400 500 600 0.2 0.4 0.6 0.8 1.0 1.2 Ab so rb an ce (a .u .)","PeriodicalId":20390,"journal":{"name":"Powder Metallurgy and Advanced Materials","volume":null,"pages":null},"PeriodicalIF":0.0000,"publicationDate":"2018-11-05","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"1","resultStr":"{\"title\":\"Green synthesis of silver chloride nanoparticles using Rhodotorula Mucilaginosa\",\"authors\":\"I. Ghiuta, D. Cristea, R. Wenkert, D. Munteanu\",\"doi\":\"10.21741/9781945291999-4\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"The biosynthesis of silver chloride nanoparticles (AgCl NPs) is presented in this paper. Silver chloride nanoparticles were synthesized using fungi culture from Rhodotorula Mucilaginosa and aqueous AgNO3 solution, as precursor. The plasmon resonance of the nanoparticles containing solution has shown through UV-visible spectrophotometry an absorbance peak at about 437 nm. Scanning Electron Microscopy, Energy Dispersive Spectroscopy, and X-ray Diffraction analyses confirmed the presence of spherical silver chloride nanoparticles with a face centered cubic crystal structure and an average particle size of 25 nm. Silver chloride nanoparticles have been shown to be able to inhibit the growth of different microorganisms, including bacteria and fungi, which would make them suitable for antimicrobial applications. Introduction The development of materials and structures at nanoscale dimensions has gained a huge interest in the nanomaterials and nano-technology research fields. One of the most important properties of metallic nanoparticles is their antimicrobial activity. Eco-friendly methods concerning nanomaterials synthesis present a substantial importance for biological applications, mainly due to nontoxic substances and environmentally friendly procedures employed [1]. Green synthesis of silver chloride nanoparticles has been reported to be mediated by different kinds of organisms, from bacteria to plant extracts. Cell-free culture supernatant of Streptomyces strain, Klebsiella planticola, biomass of Bacillus subtilis, leaf extract of Cissus quadrangularis, aqueous extract of Sargassum plagiophyllum, extract from needles of Pinus densiflora, Prunus persica L. outer peel extract are just a few examples of organisms able to synthesize AgCl NPs [2]-[8]. Weili Hu et al. have presented the synthesis of silver chloride nanoparticles under ambient conditions in nanoporous bacterial cellulose membranes as nanoreactors. It has been demonstrated that the synthesized silver chloride nanoparticles exhibited high hydrophilic ability and a strong antimicrobial activity against Staphylococcus aureus and Escherichia coli bacteria [9]. The antibacterial effect of biosynthesized AgCl NPs investigated against Escherichia coli was found to be dose-dependent [6]. The biosynthesized silver chloride nanoparticles exhibited besides the antimicrobial activity, cytotoxicity activity against HeLa and SiHa cancer cell lines [2]. Powder Metallurgy and Advanced Materials – RoPM&AM 2017 Materials Research Forum LLC Materials Research Proceedings 8 (2018) 28-34 doi: http://dx.doi.org/10.21741/9781945291999-4 29 M. Sophocleous and J. K. Atkinson have described in their review the significant development of Ag/AgCl screen printed sensors [10]. Moreover, Ag/AgCl NPs are examined for further applications of nanoparticles as a plasmonic photocatalyst [6]. The reports which have shown the importance of the AgCl NPs application, from sensors, catalysts, to antimicrobial activity, have led to the research results presented herein. Even though several methods to obtain nanoparticles are currently developed, the green methods have captured the interest of researchers due to their lack of toxicity. In the present work, the green synthesis of silver chloride nanoparticles is described. This is, to the best of our knowledge, the first report for green synthesis of AgCl NPs mediated by Rhodotorula Mucilaginosa. Materials and Methods 1. Fungi and culture conditions The fungi Rhodotorula Mucilaginosa used in this study were provided from Soroka University Medical Center from Beersheva, Israel. The fungi were cultivated in the solid media, Sabouraud agar supplied by Scharlau Chemicals, and incubated at 35 °C for 48 h. 2. Biosynthesis of AgCl nanoparticles using Rhodotorula Mucilaginosa In order to synthesize the silver chloride nanoparticles, 1μl of bacterial strains were freshly inoculated in test tubes containing 15 ml of growth medium, namely Brain Heart Infusion from Sigma Aldrich. The liquid media contained beef heart (infusion from 250 g), 5 g/L; calf brains (infusion from 200 g), 12.5 g/L; disodium hydrogen phosphate, 2.5 g/L; D(+)-glucose, 2 g/L; peptone, 10 g/L; sodium chloride, 5 g/L. The liquid culture was kept in a thermostat at 35 °C for 24 h, followed by centrifugation at 4000 rpm for 30 min. The supernatant and biomass were tested in parallel. In the first situation 5 ml of supernatant was used, while for the second one the biomass was kept with the addition of 5 ml of distilled water. The next step was similar by adding the 5-ml culture over 40 ml Ag NO3 precursor solution, at 1 mM, 2 mM and 3 mM concentration, respectively. The culture, supernatant and biomass + distilled water and precursors were kept as control. The samples were kept in a thermostat set at 35 °C, for 48 h. 3. Characterization of AgNPs Ultraviolet-visible spectral analysis was carried-out by using Jasco V-630 spectro-photometer. The UV-visible spectra were measured in the range 200-600 nm with a wavelength step size of 1.5 nm. For morphological characteristics and chemical composition, a JSM 7400f scanning electron microscope (SEM) with a platform for Energy Dispersive Spectroscopy (EDS) was used. The silver chloride nanoparticles colloid was dropped on a copper grid and coated with a platinum thin film. After this the samples were mounted on a double sided adhesive carbon-tape. The acceleration voltage was fixed to 10kV. 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引用次数: 1

摘要

紫外可见光谱测量范围为200 ~ 600 nm,波长步长为1.5 nm。利用JSM 7400f扫描电子显微镜(SEM)和能谱仪(EDS)对样品的形态特征和化学成分进行分析。将氯化银纳米颗粒胶体滴在铜网格上,并涂上一层铂薄膜。在此之后,样品被安装在双面粘碳带上。加速电压固定为10kV。采用飞利浦PW 1050/70 x射线粉末衍射仪,采用CuKα1 (λ =1,54Å)石墨单色仪,在40 kV电压,28 mA电流下,扫描范围10÷80°,在Bragg-Brentano几何结构下,对氯化银纳米颗粒的晶体性质进行了XRD分析。结果与讨论在35℃恒温箱中孵育48 h后,含有黏胶红霉菌生物量的胶体的最终颜色由淡黄色变为浅棕色。颜色的变化是纳米颗粒形成的指示。在图1中,根据前驱体浓度的不同,可以观察到明显的颜色差异。上清液和对照样品保持不变。此外,考虑光学指示(改变颜色),测量了含有纳米颗粒的胶体溶液的紫外可见吸收光谱(如图2所示)。粉末冶金与先进材料- RoPM&AM 2017材料研究论坛LLC材料研究进展8 (2018)28-34 doi: http://dx.doi.org/10.21741/9781945291999-4 30图1。胶体纳米粒子的图像合成的存在粘液红霉菌。200 300 400 500 600 0.2 0.4 0.6 0.8 1.0 1.2 Ab so b和ce (a .u .)
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Green synthesis of silver chloride nanoparticles using Rhodotorula Mucilaginosa
The biosynthesis of silver chloride nanoparticles (AgCl NPs) is presented in this paper. Silver chloride nanoparticles were synthesized using fungi culture from Rhodotorula Mucilaginosa and aqueous AgNO3 solution, as precursor. The plasmon resonance of the nanoparticles containing solution has shown through UV-visible spectrophotometry an absorbance peak at about 437 nm. Scanning Electron Microscopy, Energy Dispersive Spectroscopy, and X-ray Diffraction analyses confirmed the presence of spherical silver chloride nanoparticles with a face centered cubic crystal structure and an average particle size of 25 nm. Silver chloride nanoparticles have been shown to be able to inhibit the growth of different microorganisms, including bacteria and fungi, which would make them suitable for antimicrobial applications. Introduction The development of materials and structures at nanoscale dimensions has gained a huge interest in the nanomaterials and nano-technology research fields. One of the most important properties of metallic nanoparticles is their antimicrobial activity. Eco-friendly methods concerning nanomaterials synthesis present a substantial importance for biological applications, mainly due to nontoxic substances and environmentally friendly procedures employed [1]. Green synthesis of silver chloride nanoparticles has been reported to be mediated by different kinds of organisms, from bacteria to plant extracts. Cell-free culture supernatant of Streptomyces strain, Klebsiella planticola, biomass of Bacillus subtilis, leaf extract of Cissus quadrangularis, aqueous extract of Sargassum plagiophyllum, extract from needles of Pinus densiflora, Prunus persica L. outer peel extract are just a few examples of organisms able to synthesize AgCl NPs [2]-[8]. Weili Hu et al. have presented the synthesis of silver chloride nanoparticles under ambient conditions in nanoporous bacterial cellulose membranes as nanoreactors. It has been demonstrated that the synthesized silver chloride nanoparticles exhibited high hydrophilic ability and a strong antimicrobial activity against Staphylococcus aureus and Escherichia coli bacteria [9]. The antibacterial effect of biosynthesized AgCl NPs investigated against Escherichia coli was found to be dose-dependent [6]. The biosynthesized silver chloride nanoparticles exhibited besides the antimicrobial activity, cytotoxicity activity against HeLa and SiHa cancer cell lines [2]. Powder Metallurgy and Advanced Materials – RoPM&AM 2017 Materials Research Forum LLC Materials Research Proceedings 8 (2018) 28-34 doi: http://dx.doi.org/10.21741/9781945291999-4 29 M. Sophocleous and J. K. Atkinson have described in their review the significant development of Ag/AgCl screen printed sensors [10]. Moreover, Ag/AgCl NPs are examined for further applications of nanoparticles as a plasmonic photocatalyst [6]. The reports which have shown the importance of the AgCl NPs application, from sensors, catalysts, to antimicrobial activity, have led to the research results presented herein. Even though several methods to obtain nanoparticles are currently developed, the green methods have captured the interest of researchers due to their lack of toxicity. In the present work, the green synthesis of silver chloride nanoparticles is described. This is, to the best of our knowledge, the first report for green synthesis of AgCl NPs mediated by Rhodotorula Mucilaginosa. Materials and Methods 1. Fungi and culture conditions The fungi Rhodotorula Mucilaginosa used in this study were provided from Soroka University Medical Center from Beersheva, Israel. The fungi were cultivated in the solid media, Sabouraud agar supplied by Scharlau Chemicals, and incubated at 35 °C for 48 h. 2. Biosynthesis of AgCl nanoparticles using Rhodotorula Mucilaginosa In order to synthesize the silver chloride nanoparticles, 1μl of bacterial strains were freshly inoculated in test tubes containing 15 ml of growth medium, namely Brain Heart Infusion from Sigma Aldrich. The liquid media contained beef heart (infusion from 250 g), 5 g/L; calf brains (infusion from 200 g), 12.5 g/L; disodium hydrogen phosphate, 2.5 g/L; D(+)-glucose, 2 g/L; peptone, 10 g/L; sodium chloride, 5 g/L. The liquid culture was kept in a thermostat at 35 °C for 24 h, followed by centrifugation at 4000 rpm for 30 min. The supernatant and biomass were tested in parallel. In the first situation 5 ml of supernatant was used, while for the second one the biomass was kept with the addition of 5 ml of distilled water. The next step was similar by adding the 5-ml culture over 40 ml Ag NO3 precursor solution, at 1 mM, 2 mM and 3 mM concentration, respectively. The culture, supernatant and biomass + distilled water and precursors were kept as control. The samples were kept in a thermostat set at 35 °C, for 48 h. 3. Characterization of AgNPs Ultraviolet-visible spectral analysis was carried-out by using Jasco V-630 spectro-photometer. The UV-visible spectra were measured in the range 200-600 nm with a wavelength step size of 1.5 nm. For morphological characteristics and chemical composition, a JSM 7400f scanning electron microscope (SEM) with a platform for Energy Dispersive Spectroscopy (EDS) was used. The silver chloride nanoparticles colloid was dropped on a copper grid and coated with a platinum thin film. After this the samples were mounted on a double sided adhesive carbon-tape. The acceleration voltage was fixed to 10kV. The crystalline nature of silver chloride nanoparticles was analyzed by XRD using a Philips PW 1050/70 X-ray powder diffractometer with graphite monochromator using CuKα1 (λ =1,54Å), at a voltage of 40 kV, a current of 28 mA, in the scan range 10÷80 °, in Bragg-Brentano geometry. Results and Discussion After incubation in the thermostat for 48 h at 35 °C, the final color of the colloid, containing biomass of Rhodotorula Mucilaginosa, changed from light yellow to light brown. The change in color is an indication for the formation of nanoparticles. In Fig.1 the obvious difference in color can be observed, depending on the precursor concentration. The samples with supernatant and the control have remained unchanged. Furthermore, considering the optical indication (changing the color), the UV-visible absorption spectra of the colloidal solutions with nanoparticles was measured (shown in Fig. 2). Powder Metallurgy and Advanced Materials – RoPM&AM 2017 Materials Research Forum LLC Materials Research Proceedings 8 (2018) 28-34 doi: http://dx.doi.org/10.21741/9781945291999-4 30 Fig. 1. Image of colloidal nanoparticles synthesized in the presence of Rhodotorula Mucilaginosa. 200 300 400 500 600 0.2 0.4 0.6 0.8 1.0 1.2 Ab so rb an ce (a .u .)
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