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Production of silver nanoparticles using yeasts and evaluation of their antifungal activity against phytopathogenic fungi
Accepted Manuscript Title: Production of silver nanoparticles using yeasts and evaluation of their antifungal activity against phytopathogenic fungi Author: Jorge G. Fern´andez Mart´ın A. Fern´andez-Baldo Elias Berni Gerardo Cam´ı Nelson Dur´an Julio Raba Mar´ıa I. Sanz PII: DOI: Reference:
S1359-5113(16)30144-1 http://dx.doi.org/doi:10.1016/j.procbio.2016.05.021 PRBI 10695
To appear in:
Process Biochemistry
Received date: Revised date: Accepted date:
27-10-2015 24-4-2016 20-5-2016
Please cite this article as: Fern´andez Jorge G, Fern´andez-Baldo Mart´ın A, Berni Elias, Cam´ı Gerardo, Dur´an Nelson, Raba Julio, Sanz Mar´ıa I.Production of silver nanoparticles using yeasts and evaluation of their antifungal activity against phytopathogenic fungi.Process Biochemistry http://dx.doi.org/10.1016/j.procbio.2016.05.021 This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
1
Production of silver nanoparticles using yeasts and evaluation of their antifungal
2
activity against phytopathogenic fungi
3 4 5 6 7 8 9 10
1,3
Jorge G. Fernández, 1,3 Martín A. Fernández-Baldo, 2 Elias Berni, 3 Gerardo Camí, 2,4 Nelson Durán, 1,3 Julio Raba, 1,3 María I. Sanz*
1
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INQUISAL, CONICET. Universidad Nacional de San Luis, Chacabuco 917.
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D5700BWS. San Luis, Argentina. 2
13 14 15
Institute of Chemistry, Biological Chemistry Laboratory, Universidade Estadual de Campinas, CEP 13083-970, Caixa Postal 6154, Campinas, SP, Brazil.
3
Facultad de Química, Bioquímica y Farmacia, Universidad Nacional de San Luis, San
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Luis, Argentina. 4
Center of Natural and Human Sciences, Department of Biochemistry and Biophysics, Universidade Federal do ABC, CEP 09210-170, Santo André, SP, Brazil.
19 20 21 22 23 24
*Author to whom correspondence should be addressed: (e-mail) [email protected]
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(phone) +54-2652-425385; (Fax) +54-2652-430224.
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INQUISAL, Departamento de Química. Universidad Nacional de San Luis, CONICET.
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Chacabuco 917. D5700BWS. San Luis, Argentina.
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Facultad de Química Bioquímica y Farmacia, Universidad Nacional de San Luis, San
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Luis, Argentina. 1
31 32 33 34 35 36 37 38 39 40 41 42 43 44
Highlights Production of Ag NPs was carried out using the yeasts C. laurentii and R. glutinis. Ag NPs from both yeasts showed differences in their physicochemical properties. Ag NPs from both yeasts showed antifungal activity against pathogens of postharvest. Ag NPs from R. glutinis showed the major antifungal activity. Ag NPs from R. glutinis were similarly effective than Iprodione.
45
3
46
Abstract
47
The present study investigated the biological synthesis, characterization and
48
antifungal activity of silver nanoparticles (Ag NPs). The production of Ag NPs was
49
performed using the culture supernatants of two yeasts: Cryptococcus laurentii and
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Rhodotorula glutinis. These yeasts were chosen for their nitrate reductase activity. The
51
role of nitrate reductase in the production of nanoparticles was assessed using inhibitors.
52
The characterization of Ag NPs was made by UV-visible spectrophotometry, photon
53
correlation spectroscopy, transmission electron microscopy and X-ray diffraction.
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Moreover, the FTIR spectrum identified the possible stabilizing agents present in
55
supernatants. The Ag NPs obtained from both yeasts were disperse and stable and
56
exhibited differences in sizes, zeta potential, concentration and stabilizing compounds.
57
The antifungal activity of the Ag NPs was evaluated against the relevant
58
phytopathogenic fungi, the common producers of postharvest diseases in pome fruits.
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Susceptibility tests on agar demonstrated that the antifungal activity of the nanoparticles
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from R. glutinis was higher than that from the ones from C. laurentii, and both were
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significantly more effective for inhibiting the fungi than the nanoparticles made from
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chemical synthesis. At 3 ppm, the nanoparticles from R. glutinis had similar efficacy to
63
iprodione, a fungicide commonly utilized for combating postharvest diseases.
64 65 66 67 68
Keywords Cryptococcus laurentii; Rhodotorula glutinis; Silver nanoparticles;
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Antifungal activity; Postharvest phytopathogen fungi 4
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1. Introduction
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The synthesis of nanomaterials with a specific composition and size and distinct
72
properties has expanded the scope of their applications in several industries, including
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agriculture, textile, food, biomedical, optical, and electronic fields. In recent years,
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silver nanoparticles (Ag NPs) have gained significance due to their potential
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applicability in many fields [1-5].
76
The development of environmentally friendly, benign and green technologies for
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the production of nanoparticles with a range of chemical and physical properties is one
78
of the challenges in the newly emerging field of nanobiotechnology [6-8]. The
79
microbiological synthesis of Ag NPs presents several important advantages over
80
chemical synthesis, such as higher production and lower costs, and overall, it is an eco-
81
friendly method [9]. In fact, a number of different species of bacteria and fungi are able
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to reduce silver ions, producing Ag NPs with antimicrobial properties [4, 10-14].
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To date, there has been a continued search for novel microorganisms that
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synthesize Ag NPs. In this regard, owing to the promising application of Ag NPs for
85
plant disease management, researchers have begun to use biological agents for Ag NP
86
synthesis. The involvement of agriculturally important microbes for Ag NP synthesis
87
could lead to more environmentally friendly and biocompatible nanoparticles for the
88
efficient application in agroecosystems [15]. In this context, most recently, a well-
89
known plant growth-promoting Serratia sp. has been used to synthesize Ag NPs with
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antifungal activity against Bipolaris sorokiniana, the spot blotch pathogen of wheat
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[15].
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Cryptococcus laurentii and Rhodotorula glutinis are two yeasts that have been
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reported as biological control agents [16, 17]. These yeasts were chosen in this case to 5
94
produce Ag NPs. The aim of this work was to produce Ag NPs using these epiphytic
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yeasts isolated from apple peel, to compare their characteristics and to investigate their
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potential application to the control of fungi that cause postharvest diseases in pome
97
fruits.
98 99 100
2. Materials and Methods 2.1. Microorganisms
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Cryptococcus laurentii (BNM 0525) and Rhodotorula glutinis (BNM 0524)
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previously isolated from apple peel and identified in our laboratory [16] were selected
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for the synthesis of Ag NPs. Both strains are deposited in the National Bank of
104
Microorganisms (WDCM938) of the “Facultad de Agronomía, Universidad de Buenos
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Aires (FAUBA)”, Argentina. The yeasts were grown on potato dextrose agar (PDA) at
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25°C for 48 to 72 h and were maintained on PDA slants. These yeasts were chosen for
107
the nitrate reductase activities that they displayed. The antifungal activity was assessed
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against the phytopathogenic fungi: Botrytis cinerea (BNM 0528), Penicillium expansum
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(CEREMIC 151-2002), Aspergillus niger (NRRL 1419), Alternaria sp. (NRRL 6410),
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and Rhizopus sp. (NRRL 695). The isolates were maintained on PDA at 4°C for further
111
studies.
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2.2. Culture
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C. laurentii and R. glutinis were cultured in Muller-Hinton broth (MHB), the
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composition of which was (g L-1): beef infusion, 2; acid casein peptone, 17.5; corn
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starch, 1.5; pH 7.4. The medium was inoculated with a suspension of 2.0×106 yeast
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cells mL-1. Next, the culture flasks were incubated at 28ºC and 100 rpm in an orbital
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shaker. After 24 h of incubation, the cultures were centrifuged at 11,000 g for 10 min 6
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in a Sorvall SS-3 (DuPont Instruments), and the supernatants were reserved for the
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synthesis of Ag NPs. Before their use, the supernatants were analyzed immediately,
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evaluating the cells by microscopic analysis, and a portion was subsequently seeded on
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potato dextrose agar (PDA) to search for viable cells.
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2.3. Nitrate reductase assay
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The enzyme-nitrate reductase was assayed in the supernatant from culture yeast
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according to the procedure followed by Harley [18] and Saifuddin et al. [19]. A 5 mL
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aliquot of culture supernatant of the yeast was mixed with 5 mL of assay medium (30
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mM KNO3 and 5% propanol in 0.1 M phosphate buffer of pH 7.5) and incubated in the
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dark for 1 h. After incubation, the nitrites formed in the assay mixture were estimated
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by adding 2.5 mL of sulphanilamide and N-(1-naphthyl) ethylene diamine
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dihydrochloride solutions to it. The color developed was measured in an UV–Vis
132
spectrophotometer at 540 nm. The enzyme activity was finally expressed in terms of
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nmol of nitrite h-1 mL-1.
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2.4. Synthesis of silver nanoparticles
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For the synthesis of the Ag NPs, one milliliter of an aqueous silver nitrate
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solution (1 mM) was added to Erlenmeyer flasks containing 100 mL of yeast culture
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supernatant free of cells. The resulting mixture was shaken at 100 rpm in an orbital
139
shaker for 48 h at 28 ± 4ºC in dark. Appropriate controls (uninoculated MH medium
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plus silver nitrate and yeast culture supernatant without silver nitrate) were run
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simultaneously. The experiment was carried out in triplicate. 7
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2.5. Nitrate reductase inhibition
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The inhibition study was performed to confirm the mechanism of the Ag NP
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biosynthesis. The inhibitors used were phenyl methane sulfonyl fluoride (PMSF),
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ethylene diamine tetra acetic acid (EDTA) and sodium azide. Experiments were carried
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out similarly to those described in 2.4.
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milliliter of AgNO3 (1 mM) were added to Erlenmeyer flasks with 100 ml of the
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supernatant. Three separate trials were performed for each inhibitor. The concentration
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of Ag NPs produced was measured for each case. The nitrate reductase activity was
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measured prior the addition of the silver nitrate solution.
One milliliter of inhibitor (10 mM) and one
151 152
2.6. Physicochemical characterization of silver nanoparticles
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To characterize the Ag NPs, standard protocols were used. Spectroscopic
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analyses of surface plasmon resonance (SPR) and fluorescence were measured in an
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UV-visible spectrophotometer model UV-1650 PC, Shimadzu, and Perkin-Elmer (LS-
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55) luminescence spectrophotometer, respectively. The average diameter of the
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nanoparticles was determined by Zetasizer Nanoseries ZEN3600, Malvern Instruments,
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through the technique of photon correlation spectroscopy (PCS). Zeta potential was
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measured in the same equipment. The structure and morphology were studied by means
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of transmission electron microscopy (TEM; Carl Zeiss CEM902) and X-ray diffraction
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(Shimadzu XRD6000).
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The determination of Ag NPs concentration in culture supernatant from yeasts was
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carried out by UV-visible spectrophotometry at 420 nm. A calibration curve was made
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with the Ag NPs (Sigma-Aldrich St. Louis, MO, USA) between 5 and 20 mg.L-1. For
165
the spectrophotometric assay validation, the method of adding an internal standard 8
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(spiking) was used. A known concentration of Ag NPs (Sigma-Aldrich St. Louis, MO,
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USA) was added to suspensions of Ag NPs (Sigma-Aldrich St. Louis, MO, USA) of 5,
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10 and 20 mg.L-1 and samples (biosynthesized Ag NPs from culture supernatant of C.
169
laurentii and R. glutinis). The concentration results were plotted against spiking levels
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and interpolated using weighted linear regression (Table 1). The determination of the
171
residual ionic silver concentration was carried out by potentiometry in a potentiostat
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PGSTAT 302N, AUTOLAB.
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2.7. Fourier transform infrared (FTIR) analysis
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The Fourier transformed infrared (FTIR) spectrum of Ag NPs was obtained
176
from Nicolet Protégé 460 spectrometer provided with a CsI beam splitter in the 4000-25
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cm-1 range, 64 scans/sample with a spectral resolution of 4 cm-1 using the KBr pellet
178
technique. The sample was prepared by adding supernatant with Ag NPs onto a KBr
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pellet in a drop-wise manner and drying at 100°C in an oven for 15 min.
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2.8. Assessment of antifungal activity
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For the assessment of antifungal activity, 200 µL of fungal spores suspension
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(2.0×106 spores mL-1) were aseptically spread onto plates of PDA. Next, wells of 3 mm
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were made aseptically and were filled with 60 µL of extracts containing biosynthesized
185
Ag NPs or chemically synthesized Ag NPs (Sigma-Aldrich St. Louis, MO, USA). The
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concentrations of the Ag NPs were adjusted to 3 mg L-1. Yeast culture supernatants and
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sterile distilled water were used as controls. The plates were incubated at 28 ± 4ºC for 7
9
188
days. After incubation, the zones of inhibition (mm) were measured. The assays were
189
performed in triplicate.
190
The chemical, iprodione “Rovral 50 WP” (Rhone-Poulenc Agrochimie) was
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dissolved in an acetone–water mixture. A concentrated stock solution was prepared and
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progressively diluted in sterile water to provide an appropriate concentration for the
193
assay. The concentration used was 500 mg L−1, the normal concentration recommended
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for standard postharvest treatments [17]. Controls with dilutions of acetone–water
195
mixture were made.
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The minimal concentration of the Ag NPs, that causes 100% of spores
197
germination inhibition (MIC), was determined using a microdilution method in Potato
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Dextrose Broth (PDB).
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spores. mL-1), different volumes of extracts containing nanoparticles (50, 100, 150 and
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200 l) and PBD until final volume of 300 l. The mixture was incubated for 24 h at
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28 ºC. The final concentrations of the Ag NPs were
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silver nanoparticles from R. glutinis and C. laurentti respectively. Approximately 50 µl
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of the samples were placed on microscope slides and 100 spores per slide were
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evaluated. Controls were performed without nanoparticles. Experiments were repeated
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three times.
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2.9. Assessment of toxicity
In a vial were put 100 l of the spores suspension (2 X 106
0-2 mg.L-1 and 0-4 mg.L-1 for
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Standardized bioassays using seeds of the lettuce (Lactuca sativa) were
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performed to assess the toxicity of biosynthesized and Commercial AgNPs and also of
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the yeast culture supernatants without AgNPs. To these assays, 10 seeds were placed in
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a Petri dish with filter paper in the bottom as the support; afterwards, 2.5 ml of each
211
treatment were applied. Distilled water was used as a negative control and a Cu+2
212
solution as the positive control. After 5 days of incubation at 25 ± 1°C, the number of 10
213
germinated seeds was counted, and expressed as the percentage of germination (G%).
214
Also root elongation (RE) was analyzed and the results were expressed in mm.
215
Experiments were done in triplicate and were repeated three times. The results were
216
analyzed using analysis of variance. Statistical analyses were done with OriginPro 7.0
217
(MicroCal Software, Inc. 2002).
218 219
3. Results and Discussion
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The primary objective of this work was to study the production of Ag NPs using
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epiphytic yeasts isolated from fruits, compare their characteristics and investigate their
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potential application for the control of phytopathogenic fungi that cause rotting in pome
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fruits.
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The selection of the yeasts was based in their nitrate reductase activity because
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this enzyme seem be involved in the Ag NP synthesis [18-20]. Then, the nitrate
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reductase activity was assayed in the culture supernatant of various epiphytic yeasts
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previously isolated in our laboratory from different fruits (data not shown). The higher
228
values of nitrate reductase activities were found in the supernatant from C. laurentii and
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R. glutinis, which were 266.56±13.11 nmol h-1 mL-1 and 216.85±11 nmol h-1 mL-1,
230
respectively.
Therefore, these yeasts were selected for the synthesis of the
231
nanoparticles.
Both yeasts are considered GRAS microorganisms and are classified
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among “risk group 1” by the World Health Organization (WHO).
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When the supernatants that were free of cells, derived from the yeast cultures,
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were incubated with silver nitrate, the production of silver nanoparticles was evidenced
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by the appearance of a color change from pale yellow to dark brown in the reaction
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flasks. The reaction mixture remained a dark brown color for various months. On the
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other hand, the control reaction mixtures did not show any change in color. 11
238
The Ag NP formation was verified by surface plasmon resonance (Figure 1). In
239
both cases, a wide spectrum, characteristic of a high distribution of size nanoparticles,
240
was observed. These samples were analyzed for size distribution and zeta potential by
241
photon correlation spectroscopy. The Ag NPs produced by C. laurentii showed two
242
populations of different sizes (Figure 2a), one centered at 400 nm (13%) and another
243
around of 35 nm (74%).
244
confirmed by the transmission electron microscopy images (Figure 2b). The
245
quantification of the size distribution of the Ag NPs from R. glutinis was as follow:
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65% at 15 nm, 17% at 160 nm and 18% at 220 nm (Figure 3a). The TEM images are
247
shown in Figure 3b.
The presence of these two populations of particles was
248
A spectroscopic analysis by fluorescence emission was also performed. Figure 4
249
shows the fluorescence emission spectra of the Ag NPs from R. glutinis and C.
250
laurentii. An emission band centered at 345-355 nm (λexc 295 nm) was observed. The
251
nature of the emission indicated presence of proteins in the supernatant containing the
252
nanoparticles. Similar results were obtained by Durán et al. (2005) [20].
253
Further studies using X-ray diffraction were carried out to confirm the
254
crystalline nature of the particles produced by the yeasts.
255
supernatants (Figure 5) shows the four intense peaks ((111), (200), (220) and (311)) at
256
2θ° values, confirming that the silver particles that were formed have a nanocrystalline
257
nature.
The XRD pattern of both
258
The concentrations of Ag NPs determined by UV-visible spectrophotometry in
259
culture supernatants from C. laurentii and R. glutinis were 6 ± 0.2 and 3 ± 0.3 mg/L-1,
260
respectively. The method was validated by adding an internal standard to discard the
261
matrix effect in measuring the nanoparticle concentration in the supernatants. As can be 12
262
seen in Table 1, the recovery percentage was satisfactory; therefore the UV-visible
263
spectrophotometry was considered a valid method for the estimation of the nanoparticle
264
concentration. The Ag NP concentration obtained from R. glutinis was half of the Ag
265
NP concentration of the other yeast. These results were coincident with the first
266
estimation of concentration performed by UV-visible spectrophotometry (Figure 1).
267
The concentrations of residual ionic silver measured in the supernatants were in the
268
range of 0,001 mg.L-1.
269
FTIR spectroscopy was carried out to investigate the chemical nature of the
270
compounds present in supernatants, which could be involved in the stabilization of
271
nanoparticles. The FTIR spectrum of synthesized Ag NPs from C. laurentii (Figure 6a)
272
showed a pattern of peaks similar to R. glutinis (Figure 6 b), although with a number of
273
differences.
274
biosynthesized Ag NPs, the presence of proteins and polymeric carbohydrates can be
275
inferred, the latter to a greater extent because the peaks of the absorption of C=O and
276
CN (characteristics of proteins) appear with less intensity (band amide 2 and band
277
amide 3) with respect to the other vibrational modes. Another interesting point is the
278
important intensity of the peaks C-OH and C-O-C, together to the peaks aliphatic C-C
279
and C-H, which justifies the presence of polymeric carbohydrates. The bands observed
280
in the range between 902 and 462 cm-1 in the spectrum of C. laurentii and between 909
281
and 523 cm-1 in that of R. glutinis correspond to vibrational modes of the structural net
282
of biological polymers present in the supernatants. The most interesting peaks appear at
283
902 and 837 cm-1 for Ag NPs from C. laurentii and 909 y 840 cm-1 for Ag NPs from R.
284
glutinis, indicating glycosidic linkages and type, respectively, in coincidence with
285
the presence of polymeric carbohydrates, perhaps of arabinogalactan type for C.
According to the pattern of peaks, for the two supernatants containing
13
286
laurentii and arabinan and galactoglucomannan types for R. glutinis. The peak at 3382
287
cm-1, corresponding to the –OH and NH groups of Ag NPs from C. laurentii, is very
288
wide and difficult to resolve. However, the deconvolution of this peak shows two peaks
289
of low intensity at 3252 and 3237 cm-1, which would indicate the presence of NH
290
groups of amide (band amide 1), corresponding to peptides, while the peak 3394 cm-1,
291
corresponding to Ag NPs from R. glutinis, does not show other peaks after performing
292
the deconvolution. Furthermore, the decrease in the intensity of the carbonyl bands (C
293
= O) and CN bands show that the proportion of proteins was lower in the supernatant
294
from R. glutinis [21, 22, 23]. The FTIR spectrum of chemical Ag NPs (Figure 6c) only
295
showed a pattern corresponding to peaks of acetic acid-acetate buffer.
296
As previously described, both systems exhibited particles of different sizes with
297
a high percentage of small particles. It is believed that biogenic systems at certain
298
conditions produced small Ag NPs, and then after a certain period an agglomeration is
299
initiated due to coalescence and Ostwald ripening processes. However, the
300
agglomeration phenomena can be reduced by the use of templates that can offer
301
electrostatic and steric barriers [24]. In the case of biogenic synthesis, the compounds
302
present in supernatants are probably able to provide these two barriers. The electrostatic
303
barrier is easily measured through the zeta potential, which determines the surface
304
charge of biosynthesized Ag NPs. In this case, the results were ξ=-24.9 ± 0.5 mV and
305
ξ=-13.5 ± 0.8 mV for Ag NPs from C. laurentii and R. glutinis, respectively. Although
306
it is considered that the optimum zeta potential to avoid the formation of agglomerates
307
is close to ± 30 mV, in this case the steric barriers provided by polymeric carbohydrates
308
and proteins must be taken into account because structures compatible with
309
agglomerates were not observed. However, the steric barrier is not easy to measure, and 14
310
in this instance, it would be more efficient for the nanoparticles from R. glutinis because
311
the predominant population was smaller nanoparticles, and their size was approximately
312
half that of the nanoparticles obtained with C. laurentii.
313
To confirm whether nitrate reductase was involved in the synthesis of Ag NPs,
314
the effect of the inhibitors on the enzyme activity and the ability to synthesize
315
nanoparticles was studied. The results are shown in Figures 7 and 8. Several
316
conclusions were obtained from these studies. First, it was clear that the concentration
317
of nanoparticles was dependent on the activity of the enzyme. Second, the effect of
318
inhibitors is not the same for both cases. Third, according to the relationship between
319
enzyme activity and the concentration of the nanoparticles, the supernatant of C.
320
laurentii seemed more effective for the synthesis. Other authors have reported the
321
correlation between enzyme activity and the synthesis of nanoparticles and also the
322
influence the physiological state of the culture in the process, particularly the redox state
323
[25]. The mechanism for the synthesis of Ag NPs, proposed by Duran et al [20], is
324
shown in Scheme 1. There, the involvement of cofactors that are dependent on the redox
325
state of the culture at the harvest time can be observed.
326
For investigating the applicability of biosynthesized Ag NPs to the control of
327
postharvest diseases, their antifungal activity was evaluated against the most important
328
pathogenic fungi that rot apples, pears and grapes.
329
expansum, A. niger, Alternaria sp. and Rhizopus sp. cause diseases that limit the storage
330
period and marketing life of fruits and vegetables. For this reason, these fungi were
331
selected for these assays. Tests (Table 2) showed that the antifungal activity of Ag NPs
332
from R. glutinis was higher than the ones from C. laurentii, and both were significantly
333
more effective in inhibiting the fungi than the nanoparticles of chemical synthesis. 15
Fungi such as B. cinerea, P.
334
Moreover, at 3 ppm, the nanoparticles from R. glutinis were similarly effective to
335
iprodione against all fungi with the exception of Rhizopus. Iprodione is a fungicide
336
commonly utilized for combating postharvest diseases, which was assayed at 500 ppm,
337
which is the concentration recommended for standard postharvest treatments. Controls,
338
with yeast crude extracts alone and an acetone-water mixture did not show antifungal
339
activity. This fact allowed us to discard the presence of antifungal compounds produced
340
by the yeasts and also the effect of the solvent employed for the dissolution of
341
iprodione. The MIC for silver nanoparticles from R. glutinis against all fungi tested was
342
2 mg. L-1 while the MIC for nanoparticles from C. laurentii was 4 mg. L-1. The
343
antifungal activity of Ag NPs produced by both yeasts was effective for one year.
344
From the results of the antifungal activity tests, it can be inferred that the size of
345
the nanoparticles clearly influenced their antifungal activity. According to different
346
authors [26, 27], silver nanoparticles have the ability to anchor the microbial cell wall
347
and then penetrate it, thereby causing structural changes that affect the permeability of
348
the cell membrane and cause cell death. The size and surface area of the nanoparticles
349
are closely related because a decreasing size increases the relative surface area of Ag
350
NPs, leaving a greater number of atoms exposed on the surface, which will be available
351
to redox reactions, photochemical reactions and physicochemical interactions with cells.
352
The antifungal activity of the nanoparticles from C. laurentii and R. glutinis could be
353
explained by the previously described mechanisms, because in both cases, small
354
particles are predominant. Moreover, the polymeric carbohydrates and proteins that
355
accompany to nanoparticles would favor the interactions with the cell membrane.
356
The preliminary assays demonstrated the antifungal activity of fruit packaging
357
paper imbibed with Ag NPs from R. glutinis and C. laurentii and also a better 16
358
absorption onto the paper of the biosynthesized AgNPs (Figure 9). With respect the
359
toxicity, bioassays using seeds of the lettuce (Lactuca sativa) [28] showed that AgNPs
360
from chemical synthesis resulted more toxics than Ag NPs from R. glutinis or C.
361
laurentii (Table 3). Despite these auspicious results, further studies are necessary for
362
investigate the feasibility of incorporating Ag NPs into films and other packaging
363
materials of fruits.
364 365
4. Conclusions
366
In this study, the two assessed yeasts were adequate for the biosynthesis of Ag
367
NPs. As the epiphytic yeasts, such as C. laurentii and R. glutinis, are harmless, and they
368
are considered GRAS microorganisms, the production of nanoparticles using these
369
yeasts possesses significant advantages. Further studies are needed to optimize the
370
production of nanoparticles, which should be based on increasing the concentration of
371
nitrate reductase, optimizing the redox state in the supernatant and study and improving
372
the production of exocellular polymeric carbohydrates involved in the stabilization of
373
the nanoparticles. The antifungal activity of these nanoparticles and the potential
374
application as an effective fungicide against some phytopathogenic fungi that affect
375
pome fruits was demonstrated. Additional studies are needed to investigate the
376
feasibility of incorporating Ag NPs into films and other packaging materials of these
377
fruits.
378 379
Contributors
380
Jorge G. Fernández performed the experiments and prepared the manuscript.
381
Martín Fernández-Baldo performed the experiments, contributed to the silver
382
nanoparticles’ characterization and prepared the manuscript. Elias Berni contributed to 17
383
the silver nanoparticles’ characterization and analyzed the characterization data.
384
Gerardo Camí contributed to the silver nanoparticles’ characterization and tested in
385
vitro antifungal activity. Nelson Duran helped perform the experiments and contributed
386
significantly to manuscript preparation. Julio Raba analyzed results and contributed to
387
manuscript preparation. María I. Sanz conceived and designed the experiments,
388
analyzed results and contributed to manuscript preparation.
389 390
Acknowledgments
391
Support from CNPq, FAPESP, INOMAT (MCT/CNPq) (Brazil), NanoBioss
392
(MCTI/CNPq), the Brazilian Network on Nanotoxicology (MCTI/CNPq) and
393
Universidad Nacional de San Luis, the Agencia Nacional de Promoción Científica y
394
Tecnológica, and Consejo Nacional de Investigaciones Científicas y Técnicas
395
(CONICET) (Argentina) are acknowledged.
396 397
References
398
[1] Shaligram NS, Bule M, Bhambure R, Singhal RS, Singh SK, Szakacs G, Pandey
399
A. Biosynthesis of silver nanoparticles using aqueous extract from the compactin
400
producing fungal strain. Process Biochem 2009; 44:939-943.
401
[2] Durán N, Marcato PD, Ingle A, Gade A, Rai M. Fungi mediated-synthesis of
402
silver nanoparticles: characterization processes and applications. In: Progress and
403
Micology, Rai M and Kovics G editors. Scientific Publishers. Jodhpur, India, Ch 16;
404
2010. p. 425–449.
18
405
[3] Gade A, Ingle A, Whiteley C, Rai M. Mycogenic metal nanoparticles: Progress
406
and applications. Biotechnol Lett 2010;32:593-600.
407
[4] Li WR, Xie XB, Shi QS, Duan SS, Ouyang YS, Chen YB. Antibacterial effect
408
of silver nanoparticles on Staphylococcus aureus. Biometals 2011;24:135–141.
409
[5] Raman J, Reddy GR, Lakshmanan H, Selvaraj V, Gajendran V, Nanjian R,
410
Chinnasamy A, Sabaratnam V. Mycosynthesis and characterization of silver
411
nanoparticles from Pleurotus djamor var. roseus and their in vitro cytotoxicity effect
412
on PC3 cells. Process Biochem 2015;50:140-147.
413
[6] Alani F, Moo-Young M, Anderson W. Biosynthesis of silver nanoparticles by a
414
new strain of Streptomyces sp. compared with Aspergillus fumigatus. World J
415
Microbiol Biotechnol 2012;28:1081–1086.
416
[7] Shivaji S, Madhu S, Singh S. Extracellular synthesis of antibacterial silver
417
nanoparticles using psychrophilic bacteria. Process Biochem 2011;46:1800-1807.
418
[8] Malhotra A, Dolma K, Kaur N, Rathore YS, Ashish Mayilraj S, Choudhury AR.
419
Biosynthesis of gold and silver nanoparticles using a novel marine strain of
420
Stenotrophomonas. Bioresour Technol 2013;142:727–731.
421
[9] Durán N, Marcato PD, Durán M, Yadav A, Gade A, Rai M. Mechanistic aspects
422
in the biogenic synthesis of extracellular metal nanoparticles by peptides, bacteria,
423
fungi, and plants. Appl Microbiol Biotechnol 2011;90:1609-1624.
424
[10] Bawaskar M, Gaikwad S, Ingle A, Rathod D, Gade A, Duran N, Marcato PD,
425
Rai M. A New Report on Mycosynthesis of Silver Nanoparticles by Fusarium
426
culmorum. Curr Nanosci 2010;6:376-380.
427
[11] Kumar RR, Priyadharsani KP, Thamaraiselvi K. Mycogenic synthesis of silver
428
nanoparticles by the Japanese environmental isolate Aspergillus tamarii. J
429
Nanoparticle Res 2012;14:860-864. 19
430
[12] Rodrigues AG, Ping LY, Marcato PD, Alves OL, Silva MCP, Ruiz RC, Melo IS,
431
Tasic L, De Souza AO. Biogenic antimicrobial silver nanoparticles produced by
432
fungi. Appl Microbiol Biotechnol 2013;97:775–782.
433
[13] Zhang X, Yan S, Tyagi RD, Surampalli RY. Synthesis of nanoparticles by
434
microorganisms and their application in enhancing microbiological reaction rates.
435
Chemosphere 2011;82:489-494.
436
[14] Durán N, Marcato PD. Nano-Antimicrobials: Progress and Prospects. In: Rai M
437
and Cioffi N editors. Springer, Germany, Part 3; 2012. p. 337-374.
438
[15] Mishra S, Singh HB. Biosynthesized silver nanoparticles as nanoweapon against
439
phytopathogens: exploring their scope and potential in agriculture. Appl Microbiol
440
Biotechnol 2015; 99:1097–1107.
441
[16] Calvo J, Calvente V, Orellano ME, Benuzzi D, Sanz MI. Control of Penicillium
442
expansum and Botrytis cinerea on apple fruit by mixtures of bacteria and yeast. Food
443
Bioprocess Technol 2010; 3:644–650.
444
[17] Sansone G, Rezza I, Calvente V, Benuzzi D, Sanz De Tosetti MI. Control of
445
Botrytis cinerea strains resistant to iprodione in apple with rhodotorulic acid and
446
yeasts. Postharvest Biol Technol 2005;35:245–251.
447
[18] Harley SM. Use of a simple, colorimetric assay to demonstrate conditions for
448
induction of nitrate reductase in plants. Am Biol Teach 1993;55:161–164.
449
[19] Saifuddin N, Wong CW, Nur Yasumira AA. Rapid biosynthesis of silver
450
nanoparticles using culture supernatant of bacteria with microwave irradiation. E-J
451
Chem 2009;6:61-70.
452
[20] Durán N, Marcato PD, Alves OL, De Souza GIH, Esposito E. Mechanistic
453
aspects of biosynthesis of silver nanoparticles by several Fusarium oxysporum
454
strains. J Nanobiotechnology 2005; 3:1-8. 20
455
[21] Barth A. Infrared spectroscopy of proteins. Biochimica & Biofisica Acta 2007;
456
1767:1073-1101.
457
[22] Prestch E., Clerc T., Seibl J., Simon W. Tablas para la dilucidación estructural
458
de compuestos orgánicos por métodos espectroscópicos:
459
EM, UV-Vis. Barcelona. España: Singer Verlag-Ibérica (1998).
460
[23] Kačuráková M, Capek P, Sasinková V, Wellner N, Ebringerová A. FT-IR study
461
of plant cell wall model compounds: pecticpolysaccharides and hemicelluloses.
462
Carbohydrate Polymers 2000; 43:195-203.
463
[24] Cao G. Nanostructures & Nanomaterials: Synthesis, Properties & Applications.
464
Imperial College Press, England, 2004, Chapter 2, p. 32-48.
465
[25] Vaidyanathan R, Gopalram S, Kalishwaralal K, Deepak V, Pandian SRK,
466
Gurunathan S. Enhanced silver nanoparticle synthesis by optimization of nitrate
467
reductase activity. Colloids Surf, B 2010;75:1335–341.
468
[26] Prabhu S, Poulose E. Silver nanoparticles: mechanism of antimicrobial action,
469
synthesis, medical applications, and toxicity effects. International Nano Letters 2012;
470
2:32-35.
471
[27] Ortega F, Fernández-Baldo M, Fernández G, Serrano M, Sanz MI, Diaz-
472
Mochón J, Lorente J, Raba J. Study of antitumor activity in breast cell lines using
473
silver nanoparticles produced by yeast. International Journal of Nanomedicine 2015;
474
0:2021–2031.
475
21
13
CRMN, 1H-RMN, IR,
476
[28] Charles J, Sancey B, Morin-Crini N, Badot P, Degiorgi, Trunfio G, Crini G.
477
Evaluation of the phytotoxicity of polycontaminated industrial effluents using the
478
lettuce plant (Lactuca sativa) as a bioindicator. Ecotoxicol Environ Safety, 2011;74:
479
2057-2064
480
481
482
483
484
485
486
487
488
489
490
491
492
493 22
494
495
496
Figures
497
Scheme 1: Possible mechanism of silver reduction by nitrate reductase. From Duran et
498
al (2005). [20]
499
Figure 1: UV–Vis spectra recorded after the addition of 1 ml of silver nitrate solution
500
(1 mM) to 100 ml of culture supernatants of C. laurentii or R. glutinis. The mixture
501
was shaken at 100 rpm in an orbital shaker for 48 h at 28±4ºC in the dark.
502
Figure 2: Size distribution (a) and TEM images (b) of Ag NPs produced with the
503
supernatant from C. laurentii. The average diameter size of the nanoparticles was
504
determined by Zetasizer Nanoseries ZEN3600, Malvern Instruments, through the
505
technique of photon correlation spectroscopy (PCS) and the structure and morphology
506
were studied by means of transmission electron microscopy (TEM; Carl Zeiss
507
CEM902).
508
Figure 3: Size distribution (a) and TEM images (b) of Ag NPs produced by using
509
supernatant from R. glutinis. The average diameter size of the nanoparticles was
510
determined by Zetasizer Nanoseries ZEN3600 – Malvern Instrument, through the
511
technique of photon correlation spectroscopy (PCS) and the structure and morphology
512
were studied by means of transmission electron microscopy (TEM; Carl Zeiss CEM
513
902).
514
Figure 4: Fluorescence emission spectra recorded from the Ag NPs-yeasts reaction
515
mixture. The excitation wavelength was 295 nm. Spectra were obtained in a Perkin-
516
Elmer (LS-55) luminescence spectrophotometer. 23
517
Figure 5: X-Ray diffraction pattern of Ag NPs from C. laurentii or R. glutinis. Peaks,
518
((111), (200), (220) and (311)) at 2θ° values, confirmed that the silver particles formed
519
have a nanocrystalline nature. (Shimadzu XRD6000).
520
Figure 6: The FTIR spectra of silver nanoparticles from: (a) C. laurentii, (b) R. glutinis
521
and (c) chemical synthesis. Spectra were obtained from Nicolet Protégé 460
522
spectrometer provided with a CsI beam splitter in the 4000–25 cm-1 range, 64
523
scans/sample, with spectral resolution of 4 cm-1, using the KBr pellet technique
524
Figure 7:
525
synthesis in supernatant from C. laurentii. Phenyl methane sulfonyl fluoride (PMSF),
526
ethylene diamine tetra acetic acid (EDTA) and sodium azide were assayed at a
527
concentration of 10 mM.
528
Figure 8: Effect of inhibitors on nitrate reductase activity and nanoparticles synthesis
529
in supernatant from R. glutinis. Phenyl methane sulfonyl fluoride (PMSF), ethylene
530
diamine tetra acetic acid (EDTA) and sodium azide were assayed at a concentration of
531
10 mM.
532
Figure 9: Antifungal activity of fruit packaging paper imbibed with Ag NPs. Assays
533
were performed using discs of packaging paper imbibed with extracts containing 3 ppm
534
of biosynthesized Ag NPs (R.glutinis, C.laurentii), 3 ppm of chemically synthesized
535
Ag NPs (Ch) or 500 ppm of Iprodione. Discs were put onto plates of PDA with 200 µL
536
a B.cinerea BNM 0527 spores suspension (2.0×106 spores mL-1). Yeast culture
537
supernatants without AgNPs (SR, SC) were used as controls.
538
incubated at 28 ± 4ºC for 7 days. Assays were performed by duplicate.
The effect of inhibitors on nitrate reductase activity and nanoparticles
539 540 541 24
The plates were
542
Table 1
543
Determination of Ag NPs concentration in culture supernatant
544
Nanoparticles
Concentration measureda (mg L-1)
From C. laurentii From R. glutinis 5 mgL-1(Sigma) 10 mgL-1(Sigma) 20 mgL-1(Sigma)
6.0 ± 0.2 3.0 ± 0.3 5.6 ± 0.3 11.0± 0.1 18.0± 0.1
a
Ag NPs spiking level/mg L-1 20 Recovery (%)
27.0 ± 0.2 22.7 ± 0.1 25.7 ± 0.1 29.0 ± 0.2 39.0 ± 0.3
103.8 94.0 100.3 93.5 102.0
X ± SD, mean ± standard deviation (n=3)
Determination of Ag NP concentration in culture supernatant was carried out by UVvisible spectrophotometry at 420 nm. Calibration curve was made with Ag NPs (Sigma-Aldrich St. Louis, MO, USA) in concentrations between 5 and 20 mg.L-1. For validating spectrophotometric assay, a known concentration of Ag NPs (20 mg.L1) (Sigma-Aldrich St. Louis, MO, USA) was added to the samples and to suspensions of Ag NPs (Sigma-Aldrich St. Louis, MO, USA) of 5, 10 and 20 mg.L-1.
545 546 547 548 549 550 551 552 553 554 555 556 557 558 25
577
Table 2
578
Antifungal activity of Biosynthesized AgNPs against Postharvest phytopathogenic fungi
Diameter of inhibition zone (mm)a B. cinereaa
P. expansuma
A. nigera
Alternaria sp.a
Rhizopus sp.a
15.1 ± 1.6a
11.1 ± 1.4b
14.8±2.2a
11.3 ±1.6ab
9.7 ± 2.1b
11.4 ± 1.4b
8.3 ± 1.2b
10.5±1.2b
9.6 ± 2.3b
7.9 ± 1.8b
2.2 ±0.5c
1.9 ± 0.7c
3.0 ± 0.3c
1.7 ± 0.5c
1.3 ± 0.5c
Iprodione
17.1± 1.1a
14 ± 2.1a
15.9±1.4a
10.2 ± 1.5b
13.5 ± 1.1a
distilled water
n.m.b
n.m
n.m
n.m
n.m
Acetone water mixture supernatant from yeasts
n.m.b
n.m
n.m
n.m
n.m
n.m b
n.m
n.m
n.m
n.m
AgNPs from R. glutinis AgNPs from C. laurentii AgNPs (Sigma)
579 580 581 582 583 584 585 586 587 588 589 590 591 592 593
a
X ± SD, mean ± standard deviation.(n=3)
594
b
n.m: non measurable
27
595 596 597 598 599 600
Assays were performed by the method of diffusion on agar. 200 µL of fungal spores suspension (2.0×10 6 spores mL-1) were spread onto plates of PDA. Samples and controls (60 µL ) were put in wells of 3 mm. Concentration of nanoparticles was adjusted at 3 ppm and iprodione was assayed at concentration of 500 ppm. Controls consisted in distilled water, supernatant from yeasts and dilutions of acetone–water mixture. The plates were incubated at 28±4ºC for 7 days. The assays were performed by triplicate. Values with different letters in the same column are significantly different.
601 602 603
28
604
Table 3
605 606
Evaluation of toxicity of biosynthesized and Commercial AgNPs using lettuce
607
seeds
608
Treatment
Germination (%)
Root elongation ( mm) a
AgNPs from C. laurentii
80
27.7 + 2.1a
Supernatant (C.laurentii)
90
29.2 + 1.3a
AgNPs from R.glutinis
90
28.5 ± 1.3a
Supernatant (R. glutinis)
90
30.4 ± 0.9 a
Ag NPs (Sigma)
60
22.5 ± 3.2b
Distilled water
90
31.2 ± 4.2a
Cu2+ Solution
40
12.5 ± 2.2c
609 610
a
X ± SD, mean ± standard deviation.(n=3)
611 612 613 614 615 616
To these assays, 10 seeds were placed in a Petri dish with filter paper in the bottom as the support; afterwards, 2.5 ml of each treatment were applied. Distilled water was used as a negative control and a Cu+2 solution as the positive control. After 5 days of incubation at 25 ± 1°C the percentage of germination (G%) and root elongation (RE) were determined . Experiments were done in triplicate. Values with different letters in the same column are significantly different.
617 618 619 620 621 622 623 624 625 626 29
S1359-5113(16)30144-1 http://dx.doi.org/doi:10.1016/j.procbio.2016.05.021 PRBI 10695
To appear in:
Process Biochemistry
Received date: Revised date: Accepted date:
27-10-2015 24-4-2016 20-5-2016
Please cite this article as: Fern´andez Jorge G, Fern´andez-Baldo Mart´ın A, Berni Elias, Cam´ı Gerardo, Dur´an Nelson, Raba Julio, Sanz Mar´ıa I.Production of silver nanoparticles using yeasts and evaluation of their antifungal activity against phytopathogenic fungi.Process Biochemistry http://dx.doi.org/10.1016/j.procbio.2016.05.021 This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
1
Production of silver nanoparticles using yeasts and evaluation of their antifungal
2
activity against phytopathogenic fungi
3 4 5 6 7 8 9 10
1,3
Jorge G. Fernández, 1,3 Martín A. Fernández-Baldo, 2 Elias Berni, 3 Gerardo Camí, 2,4 Nelson Durán, 1,3 Julio Raba, 1,3 María I. Sanz*
1
11
INQUISAL, CONICET. Universidad Nacional de San Luis, Chacabuco 917.
12
D5700BWS. San Luis, Argentina. 2
13 14 15
Institute of Chemistry, Biological Chemistry Laboratory, Universidade Estadual de Campinas, CEP 13083-970, Caixa Postal 6154, Campinas, SP, Brazil.
3
Facultad de Química, Bioquímica y Farmacia, Universidad Nacional de San Luis, San
16 17 18
Luis, Argentina. 4
Center of Natural and Human Sciences, Department of Biochemistry and Biophysics, Universidade Federal do ABC, CEP 09210-170, Santo André, SP, Brazil.
19 20 21 22 23 24
*Author to whom correspondence should be addressed: (e-mail) [email protected]
25
(phone) +54-2652-425385; (Fax) +54-2652-430224.
26
INQUISAL, Departamento de Química. Universidad Nacional de San Luis, CONICET.
27
Chacabuco 917. D5700BWS. San Luis, Argentina.
28
Facultad de Química Bioquímica y Farmacia, Universidad Nacional de San Luis, San
29
Luis, Argentina. 1
31 32 33 34 35 36 37 38 39 40 41 42 43 44
Highlights Production of Ag NPs was carried out using the yeasts C. laurentii and R. glutinis. Ag NPs from both yeasts showed differences in their physicochemical properties. Ag NPs from both yeasts showed antifungal activity against pathogens of postharvest. Ag NPs from R. glutinis showed the major antifungal activity. Ag NPs from R. glutinis were similarly effective than Iprodione.
45
3
46
Abstract
47
The present study investigated the biological synthesis, characterization and
48
antifungal activity of silver nanoparticles (Ag NPs). The production of Ag NPs was
49
performed using the culture supernatants of two yeasts: Cryptococcus laurentii and
50
Rhodotorula glutinis. These yeasts were chosen for their nitrate reductase activity. The
51
role of nitrate reductase in the production of nanoparticles was assessed using inhibitors.
52
The characterization of Ag NPs was made by UV-visible spectrophotometry, photon
53
correlation spectroscopy, transmission electron microscopy and X-ray diffraction.
54
Moreover, the FTIR spectrum identified the possible stabilizing agents present in
55
supernatants. The Ag NPs obtained from both yeasts were disperse and stable and
56
exhibited differences in sizes, zeta potential, concentration and stabilizing compounds.
57
The antifungal activity of the Ag NPs was evaluated against the relevant
58
phytopathogenic fungi, the common producers of postharvest diseases in pome fruits.
59
Susceptibility tests on agar demonstrated that the antifungal activity of the nanoparticles
60
from R. glutinis was higher than that from the ones from C. laurentii, and both were
61
significantly more effective for inhibiting the fungi than the nanoparticles made from
62
chemical synthesis. At 3 ppm, the nanoparticles from R. glutinis had similar efficacy to
63
iprodione, a fungicide commonly utilized for combating postharvest diseases.
64 65 66 67 68
Keywords Cryptococcus laurentii; Rhodotorula glutinis; Silver nanoparticles;
69
Antifungal activity; Postharvest phytopathogen fungi 4
70
1. Introduction
71
The synthesis of nanomaterials with a specific composition and size and distinct
72
properties has expanded the scope of their applications in several industries, including
73
agriculture, textile, food, biomedical, optical, and electronic fields. In recent years,
74
silver nanoparticles (Ag NPs) have gained significance due to their potential
75
applicability in many fields [1-5].
76
The development of environmentally friendly, benign and green technologies for
77
the production of nanoparticles with a range of chemical and physical properties is one
78
of the challenges in the newly emerging field of nanobiotechnology [6-8]. The
79
microbiological synthesis of Ag NPs presents several important advantages over
80
chemical synthesis, such as higher production and lower costs, and overall, it is an eco-
81
friendly method [9]. In fact, a number of different species of bacteria and fungi are able
82
to reduce silver ions, producing Ag NPs with antimicrobial properties [4, 10-14].
83
To date, there has been a continued search for novel microorganisms that
84
synthesize Ag NPs. In this regard, owing to the promising application of Ag NPs for
85
plant disease management, researchers have begun to use biological agents for Ag NP
86
synthesis. The involvement of agriculturally important microbes for Ag NP synthesis
87
could lead to more environmentally friendly and biocompatible nanoparticles for the
88
efficient application in agroecosystems [15]. In this context, most recently, a well-
89
known plant growth-promoting Serratia sp. has been used to synthesize Ag NPs with
90
antifungal activity against Bipolaris sorokiniana, the spot blotch pathogen of wheat
91
[15].
92
Cryptococcus laurentii and Rhodotorula glutinis are two yeasts that have been
93
reported as biological control agents [16, 17]. These yeasts were chosen in this case to 5
94
produce Ag NPs. The aim of this work was to produce Ag NPs using these epiphytic
95
yeasts isolated from apple peel, to compare their characteristics and to investigate their
96
potential application to the control of fungi that cause postharvest diseases in pome
97
fruits.
98 99 100
2. Materials and Methods 2.1. Microorganisms
101
Cryptococcus laurentii (BNM 0525) and Rhodotorula glutinis (BNM 0524)
102
previously isolated from apple peel and identified in our laboratory [16] were selected
103
for the synthesis of Ag NPs. Both strains are deposited in the National Bank of
104
Microorganisms (WDCM938) of the “Facultad de Agronomía, Universidad de Buenos
105
Aires (FAUBA)”, Argentina. The yeasts were grown on potato dextrose agar (PDA) at
106
25°C for 48 to 72 h and were maintained on PDA slants. These yeasts were chosen for
107
the nitrate reductase activities that they displayed. The antifungal activity was assessed
108
against the phytopathogenic fungi: Botrytis cinerea (BNM 0528), Penicillium expansum
109
(CEREMIC 151-2002), Aspergillus niger (NRRL 1419), Alternaria sp. (NRRL 6410),
110
and Rhizopus sp. (NRRL 695). The isolates were maintained on PDA at 4°C for further
111
studies.
112
2.2. Culture
113
C. laurentii and R. glutinis were cultured in Muller-Hinton broth (MHB), the
114
composition of which was (g L-1): beef infusion, 2; acid casein peptone, 17.5; corn
115
starch, 1.5; pH 7.4. The medium was inoculated with a suspension of 2.0×106 yeast
116
cells mL-1. Next, the culture flasks were incubated at 28ºC and 100 rpm in an orbital
117
shaker. After 24 h of incubation, the cultures were centrifuged at 11,000 g for 10 min 6
118
in a Sorvall SS-3 (DuPont Instruments), and the supernatants were reserved for the
119
synthesis of Ag NPs. Before their use, the supernatants were analyzed immediately,
120
evaluating the cells by microscopic analysis, and a portion was subsequently seeded on
121
potato dextrose agar (PDA) to search for viable cells.
122 123 124
2.3. Nitrate reductase assay
125
The enzyme-nitrate reductase was assayed in the supernatant from culture yeast
126
according to the procedure followed by Harley [18] and Saifuddin et al. [19]. A 5 mL
127
aliquot of culture supernatant of the yeast was mixed with 5 mL of assay medium (30
128
mM KNO3 and 5% propanol in 0.1 M phosphate buffer of pH 7.5) and incubated in the
129
dark for 1 h. After incubation, the nitrites formed in the assay mixture were estimated
130
by adding 2.5 mL of sulphanilamide and N-(1-naphthyl) ethylene diamine
131
dihydrochloride solutions to it. The color developed was measured in an UV–Vis
132
spectrophotometer at 540 nm. The enzyme activity was finally expressed in terms of
133
nmol of nitrite h-1 mL-1.
134 135
2.4. Synthesis of silver nanoparticles
136
For the synthesis of the Ag NPs, one milliliter of an aqueous silver nitrate
137
solution (1 mM) was added to Erlenmeyer flasks containing 100 mL of yeast culture
138
supernatant free of cells. The resulting mixture was shaken at 100 rpm in an orbital
139
shaker for 48 h at 28 ± 4ºC in dark. Appropriate controls (uninoculated MH medium
140
plus silver nitrate and yeast culture supernatant without silver nitrate) were run
141
simultaneously. The experiment was carried out in triplicate. 7
142
2.5. Nitrate reductase inhibition
143
The inhibition study was performed to confirm the mechanism of the Ag NP
144
biosynthesis. The inhibitors used were phenyl methane sulfonyl fluoride (PMSF),
145
ethylene diamine tetra acetic acid (EDTA) and sodium azide. Experiments were carried
146
out similarly to those described in 2.4.
147
milliliter of AgNO3 (1 mM) were added to Erlenmeyer flasks with 100 ml of the
148
supernatant. Three separate trials were performed for each inhibitor. The concentration
149
of Ag NPs produced was measured for each case. The nitrate reductase activity was
150
measured prior the addition of the silver nitrate solution.
One milliliter of inhibitor (10 mM) and one
151 152
2.6. Physicochemical characterization of silver nanoparticles
153
To characterize the Ag NPs, standard protocols were used. Spectroscopic
154
analyses of surface plasmon resonance (SPR) and fluorescence were measured in an
155
UV-visible spectrophotometer model UV-1650 PC, Shimadzu, and Perkin-Elmer (LS-
156
55) luminescence spectrophotometer, respectively. The average diameter of the
157
nanoparticles was determined by Zetasizer Nanoseries ZEN3600, Malvern Instruments,
158
through the technique of photon correlation spectroscopy (PCS). Zeta potential was
159
measured in the same equipment. The structure and morphology were studied by means
160
of transmission electron microscopy (TEM; Carl Zeiss CEM902) and X-ray diffraction
161
(Shimadzu XRD6000).
162
The determination of Ag NPs concentration in culture supernatant from yeasts was
163
carried out by UV-visible spectrophotometry at 420 nm. A calibration curve was made
164
with the Ag NPs (Sigma-Aldrich St. Louis, MO, USA) between 5 and 20 mg.L-1. For
165
the spectrophotometric assay validation, the method of adding an internal standard 8
166
(spiking) was used. A known concentration of Ag NPs (Sigma-Aldrich St. Louis, MO,
167
USA) was added to suspensions of Ag NPs (Sigma-Aldrich St. Louis, MO, USA) of 5,
168
10 and 20 mg.L-1 and samples (biosynthesized Ag NPs from culture supernatant of C.
169
laurentii and R. glutinis). The concentration results were plotted against spiking levels
170
and interpolated using weighted linear regression (Table 1). The determination of the
171
residual ionic silver concentration was carried out by potentiometry in a potentiostat
172
PGSTAT 302N, AUTOLAB.
173 174
2.7. Fourier transform infrared (FTIR) analysis
175
The Fourier transformed infrared (FTIR) spectrum of Ag NPs was obtained
176
from Nicolet Protégé 460 spectrometer provided with a CsI beam splitter in the 4000-25
177
cm-1 range, 64 scans/sample with a spectral resolution of 4 cm-1 using the KBr pellet
178
technique. The sample was prepared by adding supernatant with Ag NPs onto a KBr
179
pellet in a drop-wise manner and drying at 100°C in an oven for 15 min.
180 181
2.8. Assessment of antifungal activity
182
For the assessment of antifungal activity, 200 µL of fungal spores suspension
183
(2.0×106 spores mL-1) were aseptically spread onto plates of PDA. Next, wells of 3 mm
184
were made aseptically and were filled with 60 µL of extracts containing biosynthesized
185
Ag NPs or chemically synthesized Ag NPs (Sigma-Aldrich St. Louis, MO, USA). The
186
concentrations of the Ag NPs were adjusted to 3 mg L-1. Yeast culture supernatants and
187
sterile distilled water were used as controls. The plates were incubated at 28 ± 4ºC for 7
9
188
days. After incubation, the zones of inhibition (mm) were measured. The assays were
189
performed in triplicate.
190
The chemical, iprodione “Rovral 50 WP” (Rhone-Poulenc Agrochimie) was
191
dissolved in an acetone–water mixture. A concentrated stock solution was prepared and
192
progressively diluted in sterile water to provide an appropriate concentration for the
193
assay. The concentration used was 500 mg L−1, the normal concentration recommended
194
for standard postharvest treatments [17]. Controls with dilutions of acetone–water
195
mixture were made.
196
The minimal concentration of the Ag NPs, that causes 100% of spores
197
germination inhibition (MIC), was determined using a microdilution method in Potato
198
Dextrose Broth (PDB).
199
spores. mL-1), different volumes of extracts containing nanoparticles (50, 100, 150 and
200
200 l) and PBD until final volume of 300 l. The mixture was incubated for 24 h at
201
28 ºC. The final concentrations of the Ag NPs were
202
silver nanoparticles from R. glutinis and C. laurentti respectively. Approximately 50 µl
203
of the samples were placed on microscope slides and 100 spores per slide were
204
evaluated. Controls were performed without nanoparticles. Experiments were repeated
205
three times.
206
2.9. Assessment of toxicity
In a vial were put 100 l of the spores suspension (2 X 106
0-2 mg.L-1 and 0-4 mg.L-1 for
207
Standardized bioassays using seeds of the lettuce (Lactuca sativa) were
208
performed to assess the toxicity of biosynthesized and Commercial AgNPs and also of
209
the yeast culture supernatants without AgNPs. To these assays, 10 seeds were placed in
210
a Petri dish with filter paper in the bottom as the support; afterwards, 2.5 ml of each
211
treatment were applied. Distilled water was used as a negative control and a Cu+2
212
solution as the positive control. After 5 days of incubation at 25 ± 1°C, the number of 10
213
germinated seeds was counted, and expressed as the percentage of germination (G%).
214
Also root elongation (RE) was analyzed and the results were expressed in mm.
215
Experiments were done in triplicate and were repeated three times. The results were
216
analyzed using analysis of variance. Statistical analyses were done with OriginPro 7.0
217
(MicroCal Software, Inc. 2002).
218 219
3. Results and Discussion
220
The primary objective of this work was to study the production of Ag NPs using
221
epiphytic yeasts isolated from fruits, compare their characteristics and investigate their
222
potential application for the control of phytopathogenic fungi that cause rotting in pome
223
fruits.
224
The selection of the yeasts was based in their nitrate reductase activity because
225
this enzyme seem be involved in the Ag NP synthesis [18-20]. Then, the nitrate
226
reductase activity was assayed in the culture supernatant of various epiphytic yeasts
227
previously isolated in our laboratory from different fruits (data not shown). The higher
228
values of nitrate reductase activities were found in the supernatant from C. laurentii and
229
R. glutinis, which were 266.56±13.11 nmol h-1 mL-1 and 216.85±11 nmol h-1 mL-1,
230
respectively.
Therefore, these yeasts were selected for the synthesis of the
231
nanoparticles.
Both yeasts are considered GRAS microorganisms and are classified
232
among “risk group 1” by the World Health Organization (WHO).
233
When the supernatants that were free of cells, derived from the yeast cultures,
234
were incubated with silver nitrate, the production of silver nanoparticles was evidenced
235
by the appearance of a color change from pale yellow to dark brown in the reaction
236
flasks. The reaction mixture remained a dark brown color for various months. On the
237
other hand, the control reaction mixtures did not show any change in color. 11
238
The Ag NP formation was verified by surface plasmon resonance (Figure 1). In
239
both cases, a wide spectrum, characteristic of a high distribution of size nanoparticles,
240
was observed. These samples were analyzed for size distribution and zeta potential by
241
photon correlation spectroscopy. The Ag NPs produced by C. laurentii showed two
242
populations of different sizes (Figure 2a), one centered at 400 nm (13%) and another
243
around of 35 nm (74%).
244
confirmed by the transmission electron microscopy images (Figure 2b). The
245
quantification of the size distribution of the Ag NPs from R. glutinis was as follow:
246
65% at 15 nm, 17% at 160 nm and 18% at 220 nm (Figure 3a). The TEM images are
247
shown in Figure 3b.
The presence of these two populations of particles was
248
A spectroscopic analysis by fluorescence emission was also performed. Figure 4
249
shows the fluorescence emission spectra of the Ag NPs from R. glutinis and C.
250
laurentii. An emission band centered at 345-355 nm (λexc 295 nm) was observed. The
251
nature of the emission indicated presence of proteins in the supernatant containing the
252
nanoparticles. Similar results were obtained by Durán et al. (2005) [20].
253
Further studies using X-ray diffraction were carried out to confirm the
254
crystalline nature of the particles produced by the yeasts.
255
supernatants (Figure 5) shows the four intense peaks ((111), (200), (220) and (311)) at
256
2θ° values, confirming that the silver particles that were formed have a nanocrystalline
257
nature.
The XRD pattern of both
258
The concentrations of Ag NPs determined by UV-visible spectrophotometry in
259
culture supernatants from C. laurentii and R. glutinis were 6 ± 0.2 and 3 ± 0.3 mg/L-1,
260
respectively. The method was validated by adding an internal standard to discard the
261
matrix effect in measuring the nanoparticle concentration in the supernatants. As can be 12
262
seen in Table 1, the recovery percentage was satisfactory; therefore the UV-visible
263
spectrophotometry was considered a valid method for the estimation of the nanoparticle
264
concentration. The Ag NP concentration obtained from R. glutinis was half of the Ag
265
NP concentration of the other yeast. These results were coincident with the first
266
estimation of concentration performed by UV-visible spectrophotometry (Figure 1).
267
The concentrations of residual ionic silver measured in the supernatants were in the
268
range of 0,001 mg.L-1.
269
FTIR spectroscopy was carried out to investigate the chemical nature of the
270
compounds present in supernatants, which could be involved in the stabilization of
271
nanoparticles. The FTIR spectrum of synthesized Ag NPs from C. laurentii (Figure 6a)
272
showed a pattern of peaks similar to R. glutinis (Figure 6 b), although with a number of
273
differences.
274
biosynthesized Ag NPs, the presence of proteins and polymeric carbohydrates can be
275
inferred, the latter to a greater extent because the peaks of the absorption of C=O and
276
CN (characteristics of proteins) appear with less intensity (band amide 2 and band
277
amide 3) with respect to the other vibrational modes. Another interesting point is the
278
important intensity of the peaks C-OH and C-O-C, together to the peaks aliphatic C-C
279
and C-H, which justifies the presence of polymeric carbohydrates. The bands observed
280
in the range between 902 and 462 cm-1 in the spectrum of C. laurentii and between 909
281
and 523 cm-1 in that of R. glutinis correspond to vibrational modes of the structural net
282
of biological polymers present in the supernatants. The most interesting peaks appear at
283
902 and 837 cm-1 for Ag NPs from C. laurentii and 909 y 840 cm-1 for Ag NPs from R.
284
glutinis, indicating glycosidic linkages and type, respectively, in coincidence with
285
the presence of polymeric carbohydrates, perhaps of arabinogalactan type for C.
According to the pattern of peaks, for the two supernatants containing
13
286
laurentii and arabinan and galactoglucomannan types for R. glutinis. The peak at 3382
287
cm-1, corresponding to the –OH and NH groups of Ag NPs from C. laurentii, is very
288
wide and difficult to resolve. However, the deconvolution of this peak shows two peaks
289
of low intensity at 3252 and 3237 cm-1, which would indicate the presence of NH
290
groups of amide (band amide 1), corresponding to peptides, while the peak 3394 cm-1,
291
corresponding to Ag NPs from R. glutinis, does not show other peaks after performing
292
the deconvolution. Furthermore, the decrease in the intensity of the carbonyl bands (C
293
= O) and CN bands show that the proportion of proteins was lower in the supernatant
294
from R. glutinis [21, 22, 23]. The FTIR spectrum of chemical Ag NPs (Figure 6c) only
295
showed a pattern corresponding to peaks of acetic acid-acetate buffer.
296
As previously described, both systems exhibited particles of different sizes with
297
a high percentage of small particles. It is believed that biogenic systems at certain
298
conditions produced small Ag NPs, and then after a certain period an agglomeration is
299
initiated due to coalescence and Ostwald ripening processes. However, the
300
agglomeration phenomena can be reduced by the use of templates that can offer
301
electrostatic and steric barriers [24]. In the case of biogenic synthesis, the compounds
302
present in supernatants are probably able to provide these two barriers. The electrostatic
303
barrier is easily measured through the zeta potential, which determines the surface
304
charge of biosynthesized Ag NPs. In this case, the results were ξ=-24.9 ± 0.5 mV and
305
ξ=-13.5 ± 0.8 mV for Ag NPs from C. laurentii and R. glutinis, respectively. Although
306
it is considered that the optimum zeta potential to avoid the formation of agglomerates
307
is close to ± 30 mV, in this case the steric barriers provided by polymeric carbohydrates
308
and proteins must be taken into account because structures compatible with
309
agglomerates were not observed. However, the steric barrier is not easy to measure, and 14
310
in this instance, it would be more efficient for the nanoparticles from R. glutinis because
311
the predominant population was smaller nanoparticles, and their size was approximately
312
half that of the nanoparticles obtained with C. laurentii.
313
To confirm whether nitrate reductase was involved in the synthesis of Ag NPs,
314
the effect of the inhibitors on the enzyme activity and the ability to synthesize
315
nanoparticles was studied. The results are shown in Figures 7 and 8. Several
316
conclusions were obtained from these studies. First, it was clear that the concentration
317
of nanoparticles was dependent on the activity of the enzyme. Second, the effect of
318
inhibitors is not the same for both cases. Third, according to the relationship between
319
enzyme activity and the concentration of the nanoparticles, the supernatant of C.
320
laurentii seemed more effective for the synthesis. Other authors have reported the
321
correlation between enzyme activity and the synthesis of nanoparticles and also the
322
influence the physiological state of the culture in the process, particularly the redox state
323
[25]. The mechanism for the synthesis of Ag NPs, proposed by Duran et al [20], is
324
shown in Scheme 1. There, the involvement of cofactors that are dependent on the redox
325
state of the culture at the harvest time can be observed.
326
For investigating the applicability of biosynthesized Ag NPs to the control of
327
postharvest diseases, their antifungal activity was evaluated against the most important
328
pathogenic fungi that rot apples, pears and grapes.
329
expansum, A. niger, Alternaria sp. and Rhizopus sp. cause diseases that limit the storage
330
period and marketing life of fruits and vegetables. For this reason, these fungi were
331
selected for these assays. Tests (Table 2) showed that the antifungal activity of Ag NPs
332
from R. glutinis was higher than the ones from C. laurentii, and both were significantly
333
more effective in inhibiting the fungi than the nanoparticles of chemical synthesis. 15
Fungi such as B. cinerea, P.
334
Moreover, at 3 ppm, the nanoparticles from R. glutinis were similarly effective to
335
iprodione against all fungi with the exception of Rhizopus. Iprodione is a fungicide
336
commonly utilized for combating postharvest diseases, which was assayed at 500 ppm,
337
which is the concentration recommended for standard postharvest treatments. Controls,
338
with yeast crude extracts alone and an acetone-water mixture did not show antifungal
339
activity. This fact allowed us to discard the presence of antifungal compounds produced
340
by the yeasts and also the effect of the solvent employed for the dissolution of
341
iprodione. The MIC for silver nanoparticles from R. glutinis against all fungi tested was
342
2 mg. L-1 while the MIC for nanoparticles from C. laurentii was 4 mg. L-1. The
343
antifungal activity of Ag NPs produced by both yeasts was effective for one year.
344
From the results of the antifungal activity tests, it can be inferred that the size of
345
the nanoparticles clearly influenced their antifungal activity. According to different
346
authors [26, 27], silver nanoparticles have the ability to anchor the microbial cell wall
347
and then penetrate it, thereby causing structural changes that affect the permeability of
348
the cell membrane and cause cell death. The size and surface area of the nanoparticles
349
are closely related because a decreasing size increases the relative surface area of Ag
350
NPs, leaving a greater number of atoms exposed on the surface, which will be available
351
to redox reactions, photochemical reactions and physicochemical interactions with cells.
352
The antifungal activity of the nanoparticles from C. laurentii and R. glutinis could be
353
explained by the previously described mechanisms, because in both cases, small
354
particles are predominant. Moreover, the polymeric carbohydrates and proteins that
355
accompany to nanoparticles would favor the interactions with the cell membrane.
356
The preliminary assays demonstrated the antifungal activity of fruit packaging
357
paper imbibed with Ag NPs from R. glutinis and C. laurentii and also a better 16
358
absorption onto the paper of the biosynthesized AgNPs (Figure 9). With respect the
359
toxicity, bioassays using seeds of the lettuce (Lactuca sativa) [28] showed that AgNPs
360
from chemical synthesis resulted more toxics than Ag NPs from R. glutinis or C.
361
laurentii (Table 3). Despite these auspicious results, further studies are necessary for
362
investigate the feasibility of incorporating Ag NPs into films and other packaging
363
materials of fruits.
364 365
4. Conclusions
366
In this study, the two assessed yeasts were adequate for the biosynthesis of Ag
367
NPs. As the epiphytic yeasts, such as C. laurentii and R. glutinis, are harmless, and they
368
are considered GRAS microorganisms, the production of nanoparticles using these
369
yeasts possesses significant advantages. Further studies are needed to optimize the
370
production of nanoparticles, which should be based on increasing the concentration of
371
nitrate reductase, optimizing the redox state in the supernatant and study and improving
372
the production of exocellular polymeric carbohydrates involved in the stabilization of
373
the nanoparticles. The antifungal activity of these nanoparticles and the potential
374
application as an effective fungicide against some phytopathogenic fungi that affect
375
pome fruits was demonstrated. Additional studies are needed to investigate the
376
feasibility of incorporating Ag NPs into films and other packaging materials of these
377
fruits.
378 379
Contributors
380
Jorge G. Fernández performed the experiments and prepared the manuscript.
381
Martín Fernández-Baldo performed the experiments, contributed to the silver
382
nanoparticles’ characterization and prepared the manuscript. Elias Berni contributed to 17
383
the silver nanoparticles’ characterization and analyzed the characterization data.
384
Gerardo Camí contributed to the silver nanoparticles’ characterization and tested in
385
vitro antifungal activity. Nelson Duran helped perform the experiments and contributed
386
significantly to manuscript preparation. Julio Raba analyzed results and contributed to
387
manuscript preparation. María I. Sanz conceived and designed the experiments,
388
analyzed results and contributed to manuscript preparation.
389 390
Acknowledgments
391
Support from CNPq, FAPESP, INOMAT (MCT/CNPq) (Brazil), NanoBioss
392
(MCTI/CNPq), the Brazilian Network on Nanotoxicology (MCTI/CNPq) and
393
Universidad Nacional de San Luis, the Agencia Nacional de Promoción Científica y
394
Tecnológica, and Consejo Nacional de Investigaciones Científicas y Técnicas
395
(CONICET) (Argentina) are acknowledged.
396 397
References
398
[1] Shaligram NS, Bule M, Bhambure R, Singhal RS, Singh SK, Szakacs G, Pandey
399
A. Biosynthesis of silver nanoparticles using aqueous extract from the compactin
400
producing fungal strain. Process Biochem 2009; 44:939-943.
401
[2] Durán N, Marcato PD, Ingle A, Gade A, Rai M. Fungi mediated-synthesis of
402
silver nanoparticles: characterization processes and applications. In: Progress and
403
Micology, Rai M and Kovics G editors. Scientific Publishers. Jodhpur, India, Ch 16;
404
2010. p. 425–449.
18
405
[3] Gade A, Ingle A, Whiteley C, Rai M. Mycogenic metal nanoparticles: Progress
406
and applications. Biotechnol Lett 2010;32:593-600.
407
[4] Li WR, Xie XB, Shi QS, Duan SS, Ouyang YS, Chen YB. Antibacterial effect
408
of silver nanoparticles on Staphylococcus aureus. Biometals 2011;24:135–141.
409
[5] Raman J, Reddy GR, Lakshmanan H, Selvaraj V, Gajendran V, Nanjian R,
410
Chinnasamy A, Sabaratnam V. Mycosynthesis and characterization of silver
411
nanoparticles from Pleurotus djamor var. roseus and their in vitro cytotoxicity effect
412
on PC3 cells. Process Biochem 2015;50:140-147.
413
[6] Alani F, Moo-Young M, Anderson W. Biosynthesis of silver nanoparticles by a
414
new strain of Streptomyces sp. compared with Aspergillus fumigatus. World J
415
Microbiol Biotechnol 2012;28:1081–1086.
416
[7] Shivaji S, Madhu S, Singh S. Extracellular synthesis of antibacterial silver
417
nanoparticles using psychrophilic bacteria. Process Biochem 2011;46:1800-1807.
418
[8] Malhotra A, Dolma K, Kaur N, Rathore YS, Ashish Mayilraj S, Choudhury AR.
419
Biosynthesis of gold and silver nanoparticles using a novel marine strain of
420
Stenotrophomonas. Bioresour Technol 2013;142:727–731.
421
[9] Durán N, Marcato PD, Durán M, Yadav A, Gade A, Rai M. Mechanistic aspects
422
in the biogenic synthesis of extracellular metal nanoparticles by peptides, bacteria,
423
fungi, and plants. Appl Microbiol Biotechnol 2011;90:1609-1624.
424
[10] Bawaskar M, Gaikwad S, Ingle A, Rathod D, Gade A, Duran N, Marcato PD,
425
Rai M. A New Report on Mycosynthesis of Silver Nanoparticles by Fusarium
426
culmorum. Curr Nanosci 2010;6:376-380.
427
[11] Kumar RR, Priyadharsani KP, Thamaraiselvi K. Mycogenic synthesis of silver
428
nanoparticles by the Japanese environmental isolate Aspergillus tamarii. J
429
Nanoparticle Res 2012;14:860-864. 19
430
[12] Rodrigues AG, Ping LY, Marcato PD, Alves OL, Silva MCP, Ruiz RC, Melo IS,
431
Tasic L, De Souza AO. Biogenic antimicrobial silver nanoparticles produced by
432
fungi. Appl Microbiol Biotechnol 2013;97:775–782.
433
[13] Zhang X, Yan S, Tyagi RD, Surampalli RY. Synthesis of nanoparticles by
434
microorganisms and their application in enhancing microbiological reaction rates.
435
Chemosphere 2011;82:489-494.
436
[14] Durán N, Marcato PD. Nano-Antimicrobials: Progress and Prospects. In: Rai M
437
and Cioffi N editors. Springer, Germany, Part 3; 2012. p. 337-374.
438
[15] Mishra S, Singh HB. Biosynthesized silver nanoparticles as nanoweapon against
439
phytopathogens: exploring their scope and potential in agriculture. Appl Microbiol
440
Biotechnol 2015; 99:1097–1107.
441
[16] Calvo J, Calvente V, Orellano ME, Benuzzi D, Sanz MI. Control of Penicillium
442
expansum and Botrytis cinerea on apple fruit by mixtures of bacteria and yeast. Food
443
Bioprocess Technol 2010; 3:644–650.
444
[17] Sansone G, Rezza I, Calvente V, Benuzzi D, Sanz De Tosetti MI. Control of
445
Botrytis cinerea strains resistant to iprodione in apple with rhodotorulic acid and
446
yeasts. Postharvest Biol Technol 2005;35:245–251.
447
[18] Harley SM. Use of a simple, colorimetric assay to demonstrate conditions for
448
induction of nitrate reductase in plants. Am Biol Teach 1993;55:161–164.
449
[19] Saifuddin N, Wong CW, Nur Yasumira AA. Rapid biosynthesis of silver
450
nanoparticles using culture supernatant of bacteria with microwave irradiation. E-J
451
Chem 2009;6:61-70.
452
[20] Durán N, Marcato PD, Alves OL, De Souza GIH, Esposito E. Mechanistic
453
aspects of biosynthesis of silver nanoparticles by several Fusarium oxysporum
454
strains. J Nanobiotechnology 2005; 3:1-8. 20
455
[21] Barth A. Infrared spectroscopy of proteins. Biochimica & Biofisica Acta 2007;
456
1767:1073-1101.
457
[22] Prestch E., Clerc T., Seibl J., Simon W. Tablas para la dilucidación estructural
458
de compuestos orgánicos por métodos espectroscópicos:
459
EM, UV-Vis. Barcelona. España: Singer Verlag-Ibérica (1998).
460
[23] Kačuráková M, Capek P, Sasinková V, Wellner N, Ebringerová A. FT-IR study
461
of plant cell wall model compounds: pecticpolysaccharides and hemicelluloses.
462
Carbohydrate Polymers 2000; 43:195-203.
463
[24] Cao G. Nanostructures & Nanomaterials: Synthesis, Properties & Applications.
464
Imperial College Press, England, 2004, Chapter 2, p. 32-48.
465
[25] Vaidyanathan R, Gopalram S, Kalishwaralal K, Deepak V, Pandian SRK,
466
Gurunathan S. Enhanced silver nanoparticle synthesis by optimization of nitrate
467
reductase activity. Colloids Surf, B 2010;75:1335–341.
468
[26] Prabhu S, Poulose E. Silver nanoparticles: mechanism of antimicrobial action,
469
synthesis, medical applications, and toxicity effects. International Nano Letters 2012;
470
2:32-35.
471
[27] Ortega F, Fernández-Baldo M, Fernández G, Serrano M, Sanz MI, Diaz-
472
Mochón J, Lorente J, Raba J. Study of antitumor activity in breast cell lines using
473
silver nanoparticles produced by yeast. International Journal of Nanomedicine 2015;
474
0:2021–2031.
475
21
13
CRMN, 1H-RMN, IR,
476
[28] Charles J, Sancey B, Morin-Crini N, Badot P, Degiorgi, Trunfio G, Crini G.
477
Evaluation of the phytotoxicity of polycontaminated industrial effluents using the
478
lettuce plant (Lactuca sativa) as a bioindicator. Ecotoxicol Environ Safety, 2011;74:
479
2057-2064
480
481
482
483
484
485
486
487
488
489
490
491
492
493 22
494
495
496
Figures
497
Scheme 1: Possible mechanism of silver reduction by nitrate reductase. From Duran et
498
al (2005). [20]
499
Figure 1: UV–Vis spectra recorded after the addition of 1 ml of silver nitrate solution
500
(1 mM) to 100 ml of culture supernatants of C. laurentii or R. glutinis. The mixture
501
was shaken at 100 rpm in an orbital shaker for 48 h at 28±4ºC in the dark.
502
Figure 2: Size distribution (a) and TEM images (b) of Ag NPs produced with the
503
supernatant from C. laurentii. The average diameter size of the nanoparticles was
504
determined by Zetasizer Nanoseries ZEN3600, Malvern Instruments, through the
505
technique of photon correlation spectroscopy (PCS) and the structure and morphology
506
were studied by means of transmission electron microscopy (TEM; Carl Zeiss
507
CEM902).
508
Figure 3: Size distribution (a) and TEM images (b) of Ag NPs produced by using
509
supernatant from R. glutinis. The average diameter size of the nanoparticles was
510
determined by Zetasizer Nanoseries ZEN3600 – Malvern Instrument, through the
511
technique of photon correlation spectroscopy (PCS) and the structure and morphology
512
were studied by means of transmission electron microscopy (TEM; Carl Zeiss CEM
513
902).
514
Figure 4: Fluorescence emission spectra recorded from the Ag NPs-yeasts reaction
515
mixture. The excitation wavelength was 295 nm. Spectra were obtained in a Perkin-
516
Elmer (LS-55) luminescence spectrophotometer. 23
517
Figure 5: X-Ray diffraction pattern of Ag NPs from C. laurentii or R. glutinis. Peaks,
518
((111), (200), (220) and (311)) at 2θ° values, confirmed that the silver particles formed
519
have a nanocrystalline nature. (Shimadzu XRD6000).
520
Figure 6: The FTIR spectra of silver nanoparticles from: (a) C. laurentii, (b) R. glutinis
521
and (c) chemical synthesis. Spectra were obtained from Nicolet Protégé 460
522
spectrometer provided with a CsI beam splitter in the 4000–25 cm-1 range, 64
523
scans/sample, with spectral resolution of 4 cm-1, using the KBr pellet technique
524
Figure 7:
525
synthesis in supernatant from C. laurentii. Phenyl methane sulfonyl fluoride (PMSF),
526
ethylene diamine tetra acetic acid (EDTA) and sodium azide were assayed at a
527
concentration of 10 mM.
528
Figure 8: Effect of inhibitors on nitrate reductase activity and nanoparticles synthesis
529
in supernatant from R. glutinis. Phenyl methane sulfonyl fluoride (PMSF), ethylene
530
diamine tetra acetic acid (EDTA) and sodium azide were assayed at a concentration of
531
10 mM.
532
Figure 9: Antifungal activity of fruit packaging paper imbibed with Ag NPs. Assays
533
were performed using discs of packaging paper imbibed with extracts containing 3 ppm
534
of biosynthesized Ag NPs (R.glutinis, C.laurentii), 3 ppm of chemically synthesized
535
Ag NPs (Ch) or 500 ppm of Iprodione. Discs were put onto plates of PDA with 200 µL
536
a B.cinerea BNM 0527 spores suspension (2.0×106 spores mL-1). Yeast culture
537
supernatants without AgNPs (SR, SC) were used as controls.
538
incubated at 28 ± 4ºC for 7 days. Assays were performed by duplicate.
The effect of inhibitors on nitrate reductase activity and nanoparticles
539 540 541 24
The plates were
542
Table 1
543
Determination of Ag NPs concentration in culture supernatant
544
Nanoparticles
Concentration measureda (mg L-1)
From C. laurentii From R. glutinis 5 mgL-1(Sigma) 10 mgL-1(Sigma) 20 mgL-1(Sigma)
6.0 ± 0.2 3.0 ± 0.3 5.6 ± 0.3 11.0± 0.1 18.0± 0.1
a
Ag NPs spiking level/mg L-1 20 Recovery (%)
27.0 ± 0.2 22.7 ± 0.1 25.7 ± 0.1 29.0 ± 0.2 39.0 ± 0.3
103.8 94.0 100.3 93.5 102.0
X ± SD, mean ± standard deviation (n=3)
Determination of Ag NP concentration in culture supernatant was carried out by UVvisible spectrophotometry at 420 nm. Calibration curve was made with Ag NPs (Sigma-Aldrich St. Louis, MO, USA) in concentrations between 5 and 20 mg.L-1. For validating spectrophotometric assay, a known concentration of Ag NPs (20 mg.L1) (Sigma-Aldrich St. Louis, MO, USA) was added to the samples and to suspensions of Ag NPs (Sigma-Aldrich St. Louis, MO, USA) of 5, 10 and 20 mg.L-1.
545 546 547 548 549 550 551 552 553 554 555 556 557 558 25
577
Table 2
578
Antifungal activity of Biosynthesized AgNPs against Postharvest phytopathogenic fungi
Diameter of inhibition zone (mm)a B. cinereaa
P. expansuma
A. nigera
Alternaria sp.a
Rhizopus sp.a
15.1 ± 1.6a
11.1 ± 1.4b
14.8±2.2a
11.3 ±1.6ab
9.7 ± 2.1b
11.4 ± 1.4b
8.3 ± 1.2b
10.5±1.2b
9.6 ± 2.3b
7.9 ± 1.8b
2.2 ±0.5c
1.9 ± 0.7c
3.0 ± 0.3c
1.7 ± 0.5c
1.3 ± 0.5c
Iprodione
17.1± 1.1a
14 ± 2.1a
15.9±1.4a
10.2 ± 1.5b
13.5 ± 1.1a
distilled water
n.m.b
n.m
n.m
n.m
n.m
Acetone water mixture supernatant from yeasts
n.m.b
n.m
n.m
n.m
n.m
n.m b
n.m
n.m
n.m
n.m
AgNPs from R. glutinis AgNPs from C. laurentii AgNPs (Sigma)
579 580 581 582 583 584 585 586 587 588 589 590 591 592 593
a
X ± SD, mean ± standard deviation.(n=3)
594
b
n.m: non measurable
27
595 596 597 598 599 600
Assays were performed by the method of diffusion on agar. 200 µL of fungal spores suspension (2.0×10 6 spores mL-1) were spread onto plates of PDA. Samples and controls (60 µL ) were put in wells of 3 mm. Concentration of nanoparticles was adjusted at 3 ppm and iprodione was assayed at concentration of 500 ppm. Controls consisted in distilled water, supernatant from yeasts and dilutions of acetone–water mixture. The plates were incubated at 28±4ºC for 7 days. The assays were performed by triplicate. Values with different letters in the same column are significantly different.
601 602 603
28
604
Table 3
605 606
Evaluation of toxicity of biosynthesized and Commercial AgNPs using lettuce
607
seeds
608
Treatment
Germination (%)
Root elongation ( mm) a
AgNPs from C. laurentii
80
27.7 + 2.1a
Supernatant (C.laurentii)
90
29.2 + 1.3a
AgNPs from R.glutinis
90
28.5 ± 1.3a
Supernatant (R. glutinis)
90
30.4 ± 0.9 a
Ag NPs (Sigma)
60
22.5 ± 3.2b
Distilled water
90
31.2 ± 4.2a
Cu2+ Solution
40
12.5 ± 2.2c
609 610
a
X ± SD, mean ± standard deviation.(n=3)
611 612 613 614 615 616
To these assays, 10 seeds were placed in a Petri dish with filter paper in the bottom as the support; afterwards, 2.5 ml of each treatment were applied. Distilled water was used as a negative control and a Cu+2 solution as the positive control. After 5 days of incubation at 25 ± 1°C the percentage of germination (G%) and root elongation (RE) were determined . Experiments were done in triplicate. Values with different letters in the same column are significantly different.
617 618 619 620 621 622 623 624 625 626 29