- Email: [email protected]
In-Vitro cytotoxicity, antibacterial, and UV protection properties of the biosynthesized Zinc oxide nanoparticles for medical textile applications
Accepted Manuscript In-Vitro cytotoxicity, antibacterial, and UV protection properties of the biosynthesized Zinc oxide nanoparticles for medical textile applications Amr Fouda, Saad EL-Din Hassan, Salem S. Salem, Th I. Shaheen PII:
S0882-4010(17)31498-5
DOI:
10.1016/j.micpath.2018.09.030
Reference:
YMPAT 3180
To appear in:
Microbial Pathogenesis
Received Date: 13 November 2017 Revised Date:
10 June 2018
Accepted Date: 16 September 2018
Please cite this article as: Fouda A, EL-Din Hassan S, Salem SS, Shaheen TI, In-Vitro cytotoxicity, antibacterial, and UV protection properties of the biosynthesized Zinc oxide nanoparticles for medical textile applications, Microbial Pathogenesis (2018), doi: https://doi.org/10.1016/j.micpath.2018.09.030. 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.
ACCEPTED MANUSCRIPT
1
In-Vitro cytotoxicity, antibacterial, and UV protection properties of the
3
biosynthesized Zinc oxide nanoparticles for medical textile applications
4
Amr Fouda1, Saad EL-Din Hassan1, Salem S Salem1 and Th. I. Shaheen2*
RI PT
2
5 6
1
7
Cairo, 11884, Egypt.
8
2
9
Behouth St. (former El-Tahrir str.), Dokki, P.O. 12622, Giza, Egypt.
SC
Department of Botany and Microbiology, Faculty of Science, Al-Azhar University, Nasr City,
M AN U
National Research Centre (Scopus affiliation ID 60014618), Textile Research Division, El-
10
*Corresponding Author: Dr. Tharwat Ibrahim Shaheen (PhD), Email:
11
[email protected].
12
TE D
13
Abstract
15
Nowadays, medical textiles have become the most essential and developing part in
16
human healthcare sector. This work was undertaken with a view to harness the bio-active
17
macromolecules secreted by fungi e.g. proteins and enzymes in bio-synthesis of ZnO
18
nanoparticles for multifunctional textiles such as antibacterial activity and UV protection
19
with considering the cytotoxicity limitation. Herein, the isolated fungus, Aspergillus
20
terreus, was allowed to produce proteins which has affinity to cape ZnO-NPs. Various
21
factors affecting the behavior of the secreted proteins on the formed nanoparticles were
22
investigated. Thorough characterizations of the protein capped ZnO-NPs were performed
23
by the using of UV-Visible spectroscopy, transmission electron microscope (TEM)
AC C
EP
14
1
ACCEPTED MANUSCRIPT
Fourier Transform-Infra Red (FT-IR) spectroscopy, X-ray diffraction (XRD) analysis and
25
Dynamic light scattering analysis (DLS). Prior treatment of cotton fabrics with ZnO-NPs,
26
the cytotoxicity of the protein capped ZnO-NPs was examined. After that, the
27
antibacterial activity of the ZnO-NPs before and after treating of cotton fabrics, besides,
28
the UV-protection (UPF) properties were investigated. Results obviously demonstrated
29
the ability of the bio-secreted protein to cape and reduce ZnO to spherical ZnO-NPs with
30
particle size lied around 10-45nm, as indicated form UV-vis., spectra TEM, Zeta sizer,
31
FTIR and XRD. Regarding to the results of cytotoxicity, the treatment of the cotton
32
fabrics with ZnO-NPs were performed at safe dose (20ppm). At this dose, ZnO-NPs
33
loaded samples exhibited reasonable antibacterial activity against both Gram positive and
34
Gram negative bacteria; besides, good UV-protection with reasonable increase in UVA
35
and UVB blocking values. Indeed, nanotechnology based microbiological active
36
molecules opens up new opportunities for us to explore novel applications in terms of
37
green technology.
38
Keywords: Zinc oxide nanoparticles; Biosynthesis; Antibacterial; cytotoxicity; UV
39
protection; medical textile.
41 42
SC
M AN U
TE D
EP
AC C
40
RI PT
24
1. Introduction
Bio-Nanotechnology is a correlation of both biology and nanotechnology. Most
43
recently, bio-nanotechnology is growing up day by day as a quickly developing filed with
44
its application in science and technology with the end goal of assembling new materials
45
at the nanoscale level [1, 2]. In recent years, different industries as textile, health, food,
46
chemicals, and cosmetic products incorporated with nanoparticles (NPs). The 2
ACCEPTED MANUSCRIPT
environmental friendly approach for the biosynthesis of nanoparticles is an opportunity to
48
be safely applied in medical fields [3]. Combination of textile technology and medical
49
science has resulted into a new field called medical textiles. New areas of applications for
50
medical textiles have been identified with the development of new either fiber yarns
51
technology or the combined functional biomedical materials such as nanoparticles. Green
52
synthesis of NPs includes synthesis through plants, bacteria, actinomycetes, fungi [4], and
53
algae permit large scale production of NPs free impurities [5].
SC
RI PT
47
Zin oxide nanoparticles (ZnO-NPs) have attracts attention of many researchers for
55
it is biological and chemical behavior which can be returned to their morphology. ZnO-
56
NPs have been used in various biological application as drug delivery and destroying of
57
tumor cell [6], antibacterial and antifungal activity [7], medical textile industry and UV
58
filtering prosperities [8].
M AN U
54
There are several methods for ZnO-NPs synthesis as chemical vapor synthesis [9],
60
sol-gel method [10] sonochemical [11] and thermal decomposition [12]. Processing steps
61
and physical factor as pH, temperature and pressure for these methods are difficult
62
controlling beside producing by-product which may be toxic for ecosystem; therefore,
63
green synthesis of ZnO-NPs is most preferred. Fungi are simple handling and possess
64
different variety of proteins and enzymes in their cell, therefore it is considered excellent
65
candidates for ZnO-NPs synthesis.
EP
AC C
66
TE D
59
Optimization of physic-chemical parameters such as substrate concentration, pH
67
and temperature, agitation rate for medium and incubation period play an important roles
68
in green synthesis of nanoparticles [13, 14]. The activity of ZnO-NPs against tumor cell
3
ACCEPTED MANUSCRIPT
69
due to smaller nanoparticle size, generation of reactive oxygen species (ROS) and highly
70
specific surface area [15]. In the current study, we aimed to fabricate the multifunctional medical textile
72
through using of environmentally benign system. To achieve this goal, this work was
73
designed to synthesize and optimize of ZnO-NPs through using of the secreted proteins
74
by the isolated fungus Aspergillus terreus AF-1, in concurrent with investigation of their
75
MIC (minimum inhibitory concentration) and in-vitro cytotoxicity of the biosynthesized
76
ZnO-NPs prior applying of ZnO-NPs onto cotton fabrics. At safe concentration, ZnO-
77
NPs were loaded onto cotton fabrics to also investigate both antibacterial activity and
78
UV-protection properties.
79
M AN U
SC
RI PT
71
2. Materials and Methods
81
2.1.Isolation and Identification of fungal isolate
82
The soil fungus, Aspergillus terreus AF-1 was isolated from contaminated soil dye,
83
Egypt (GPS N: 30o 15 54.51: E: 31o 45 39.95). Isolation of fungi was carried out by
84
plating the inoculum on PDA after serial dilutions of soil sample and incubated at 28± 2
85
°C for 3-4 days. Bacterial contamination was inhibited by supplementing the medium
86
with chloramphenicol at a concentration of 10 µg mL-1 after autoclaving.
87
Morphologically differed colonies were individually picked up and reinoculated on PDA
88
for purification, and then kept at 4 °C for further study [16].
89
Molecular identification was conducted based on amplification and sequencing of
90
internal transcribed spacer (ITS) region. Genomic DNA was extracted using the protocol
91
of Gene Jet Plant genomic DNA purification Kit (Thermo). The ITS region was amplified
AC C
EP
TE D
80
4
ACCEPTED MANUSCRIPT
92
in polymerase chain reaction (PCR) using the genomic DNA as template and primers of
93
ITS1
94
TCCGCTTATTGATATGC-3 ̀). The PCR mixture (50µL) contained Maxima Hot Start
95
PCR Master Mix (Thermo), 0.5µM of each primer, and 1µL of extracted fungal genomic
96
DNA. The PCR was performed in a DNA Engine Thermal Cycler by Sigma Scientific
97
Services Company (Cairo, Egypt) with a hot starting performed at 94ºC for 3 min,
98
followed by 30 cycles of 94ºC for 0.5 min, 55ºC for 0.5 min, and 72ºC for 1 min,
99
followed by a final extension performed at 72ºC for 10 min. The commercial sequencing
100
was conducted using ABI 3730x1 DNA sequencer at GATC Company (Germany). The
101
ITS sequence was compared against the GenBank database using the NCBI BLAST
102
program. Sequences were then compared with ITS sequences in the GenBank database
103
using BLASTN. Multiple sequence alignment was done using ClustalX 1.8 software
104
package (http://wwwigbmc.u-strasbg.fr/BioInfo/clustalx) and a phylogenetic tree was
105
constructed by the neighbor-joining method using MEGA (Version 6.1) software. The
106
confidence level of each branch (1,000 repeats) was tested by bootstrap analysis.
108
-3 ̀)
and
ITS4
(5 ̀-
TCC
TE D
M AN U
SC
RI PT
TCCGTAGGTGAACCTGCGG
EP
107
(5 ̀-
2.2.Biosynthesis of ZnO Nanoparticle using protein secreted fungi Aspergillus terreus AF-1 was grown up in 250 mL Erlenmeyer flask containing 100 mL
110
Czapek Dox (CD) fermentative broth medium for 3 days at pH 6.0, 28±2oC, and shaking
111
of 150 rpm. After incubation period, the fungal biomass was separated using Whatman
112
filter paper No. 1 by filtration method, and washed thrice with sterile distilled H2O to
113
remove any medium components. The harvested fungal biomass (15 g) were re-
114
suspended in 100 mL sterile distilled H2O in an orbital shaker (150 rpm) for 48 h. at
AC C
109
5
ACCEPTED MANUSCRIPT
115
28±2oC. The cell-free filtrate was obtained by separating the fungal biomass using
116
Whatman filter paper No. 1 and used for ZnO-NPs production as the following. Different ratios of Zinc acetate Zn(CH3CO2)2 were mixed and incubated with cell
118
free filtrate at 28±2oC for 24h on orbital shaker (150 rpm). After completion of
119
incubation period, a creamy-white precipitate, mainly Zn(OH)2, was indicated. The latter
120
was separated and then dried at 150 oC for 48h. The bio-transformed product was
121
eventually collected and subjected for further investigation.
2.3.Factors affecting ZnO-NPs production.
M AN U
123
SC
122
RI PT
117
Different variables such as incubation period, Zn (CH3CO2)2 concentrations (0.5mM to
125
2.5mM), and pH (5.0-11) which influencing on the production and distribution of the
126
particle size of ZnO-NPs were studied using UV-visible spectroscopy (JENWAY 6305
127
Spectrophotometer) after resuspension in distilled water.
128
TE D
124
2.4.Characterization of the optimized ZnO-NPs
130
The particle size and shape of the biosynthesized ZnO-NPs were preliminary
131
characterized by using transmission electron microscope (TEM) measurements through
132
using drop coating method in which a drop of solution containing nanoparticles was
133
placed on the carbon-coated copper grids and kept under vacuum desiccation for
134
overnight before loading them onto a specimen holder. For further confirmation, the
135
dynamic light scattering analysis (DLS) was employed in order to investigate the particle
136
size distribution of synthesized nanoparticles as well as check the stability of the
137
nanoparticles by indicating the zeta potential measurement.
AC C
EP
129
6
ACCEPTED MANUSCRIPT
Moreover, the characteristic functional groups present in synthesized nanoparticles
139
molecules were analyzed using Fourier Transform-Infra Red (FT-IR) spectroscopy. The
140
samples were mixed with KBr (binding agent) and were loaded into discs at high
141
pressure. These discs were scanned in the range of 400 to 4000 cm-1 to obtain FT-IR
142
spectra. The crystalline structure of ZnO-NPs was characterized by XRD analysis.
143
Finally, thermal properties of ZnO NPs were measured using Thermal Gravimetric
144
Analysis (TGA/DTA-60H instrument (SHIMADZU) to determine the organic to
145
inorganic contents. Decomposition profiles of TGA were recorded at a heating rate of
146
10.0 0C/min between room temperature and 800.0 0C in nitrogen gas.
M AN U
SC
RI PT
138
147 148 149
2.5.Biological activity of the biosynthesized ZnO-NPs Antibacterial activity of ZnO-NPs
The antibacterial activity of biosynthesized ZnO-NPs was evaluated against Gram
151
positive (Staphylococcus aureus ATCC 6538, Bacillus subtilis ATCC 6633) and Gram
152
negative bacteria (Pseudomonas aeruginosa ATCC 9027, Escherichia coli ATCC 8739)
153
using agar well diffusion method [17]. Each bacterial strain was swabbed uniformly onto
154
individual Mueller Hinton agar plates. In each plate, wells was cut out using a standard
155
cork borer (7 mm diameter). Using a micropipette, 100 µL of Zinc oxide nanoparticles
156
(2000 µg/mL) was added into each well. After incubation at 37 °C for 24 h, the diameter
157
of inhibition zones was measured in mm and the results were recorded. The experiments
158
were performed in three replicates.
159
AC C
EP
TE D
150
Minimum Inhibitory Concentration (MIC)
7
ACCEPTED MANUSCRIPT
MIC of ZnO-NPs against previous Gram positive and Gram negative bacteria were
161
checked by agar well diffusion method. Different concentration of biosynthesized ZnO-
162
NPs (1000, 500, 250 and 125 µg/mL) were made. Each bacterial strain was swabbed
163
uniformly onto individual Mueller Hinton agar plates, and wells were cut out using a
164
standard cork borer (7 mm diameter). A 100 µL of each concentration was poured in to
165
wells and the tested plates were incubated at 37 °C for 24 hours. The minimum
166
concentration of ZnO-NPs showing inhibition zone was considered to be MIC.
167
Experiment was performed in triplicates.
168
In vitro cytotoxicity of ZnO-NPs against cancer and normal cells •
SC
M AN U
169
RI PT
160
Cell culture
The human colorectal adenocarcinoma cells (Caco-2), normal Vero cells (kidney of
171
African green monkey) and normal rat liver epithelial cell (colne-9) were procured from
172
ATCC.
173
•
TE D
170
Cell morphology
Morphological changes in epithelial cells in response to ZnO-NPs, after 24 h of
175
incubation were assessed by light inverted microscope (Nikon, Japan). Cells were
176
cultured in 96-well plates at a density of 1 × 105 cells/well and treated with double fold
177
dilution of biosynthesized ZnO-NPs (1000 µg/mL to 3.9 µg/mL).
179
AC C
178
EP
174
•
MTT assay
180
The cytotoxicity of ZnO-NPs was evaluated by cell viability assay MTT [3-(4, 5-
181
dimethylthiazol-2-yl)-2, 5-diphenyl tetrazolium bromide] using Caco-2 cell, Vero cell &
182
Clone-9 cell. In brief, the cell (1 X 105 cells/mL) grown in 96-well plates and treated with
8
ACCEPTED MANUSCRIPT
different concentration of ZnO-NPs (double-fold dilution) represented as 1000, 500, 250,
184
125, 62.5, 31.25, 15.62, 7.81 and 3.9 µg/mL for 24h at 37oC. The cell were future
185
incubated with MTT (5 mg/mL in phosphate buffered saline) at 37oC / 5% CO2 for 1-5 h.
186
Adding the formazan (MTT metabolic product dissolved in 200 µL DMSO) to 96-well
187
plate. The color intensity was measured at 560 nm using an enzyme linked
188
immunosorbent assay (ELISA) reader [18]. The experiments were performed in
189
triplicates. The percentage cell viability was then calculated with respect to control (cells
190
incubated without zinc oxide nanoparticles) as follows:
SC
RI PT
183
Cell viability % = (sample absorbance / control absorbance) x100.
192
Cell toxicity % =100 – [(sample absorbance / control absorbance) x100].
M AN U
191
193
195
2.6.Application of ZnO-NPs as a precursor for medical textiles •
Zinc oxide nanoparticles loading onto cotton fabrics based textiles
TE D
194
Before being used, cotton fabrics were washed and dried. Experiments were performed
197
on samples with maximum dimension of 30 cm × 15 cm. Cotton fabrics were padded
198
with ZnO-NPs solution at certain safe concentration revealed from both MIC and in-vitro
199
cytotoxicity investigation. For the successive treatment of fabrics with colloidal zinc
200
oxide, the solution was agitated continuously. All samples were immersed in such colloid
201
bath for 5 min then squeezed to 100% wet pick up with laboratory pad at constant
202
pressure. Samples were dried at 80°C for 5 min, followed by curing at 150°C for 2 min.
203
The following treatments were conducted: (1) Control which A] Trypticasene soya broth
204
(TSB) without inoculation by bacterial culture (negative control) B] untreated fabrics
205
emerged in TSB inoculated by bacterial culture (positive control) C] untreated fabrics
AC C
EP
196
9
ACCEPTED MANUSCRIPT
206
emerged in TSB without inoculation (blank) (2) fabrics treated with zinc oxide
207
nanoparticles solution [19].
208
•
Scanning electron microscopy (SEM) for cotton fabrics
SEM was studied using a scanning electron –JSM-5400 instrument (Jeol, Japan). The
210
specimens in the form of fabrics were mounted on the specimen stabs and coated with
211
thin film of gold by the sputtering method.
RI PT
209
213
•
SC
212
Assessment of antimicrobial activity of nanoparticles treated fabric.
The antimicrobial behavior of fabrics was evaluated against Gram positive bacteria
215
represented by Staphylococcus aureus ATCC 6538, Bacillus subtilis ATCC 6633 and
216
Gram negative represented by Pseudomonas aeruginosa ATCC 9027 and Escherichia
217
coli ATCC 8739. Squares of 1 cm of each fabric were prepared in aseptic manner and
218
placed in 5 mL TSB inoculated by 100 µL of microbial suspension (adjusted optical
219
density for all bacterial culture at O.D. = 1 nm). The efficiency of the antimicrobial
220
treatment was determined by comparing the reduction in optical density (O.D.630 nm) of
221
the treated samples with that of positive control. Optical density is directly proportional
222
to the number of bacteria in the medium. The bacteriostatic activity was evaluated after
223
24 h and the percent reduction of bacteria was calculated using the following equation:
224
R (%) = [(A - B) / A] × 100
225
Where R= the reduction rate, A = the number of optical density for positive control, and
226
B = the numbers of optical density for treated fabrics.
AC C
EP
TE D
M AN U
214
227 228
•
Ultraviolet protection factor of fabrics
10
ACCEPTED MANUSCRIPT
The ability of treated and untreated fabric to block UV light is given by the ultraviolet
230
protection factor value (UPF). The UPF value was evaluated in the range of 280 – 400
231
nm with difference 10 nm by UV/Visible Spectrophotometer 3101 PC with a software
232
version.
RI PT
229
233 234
•
Statistical analysis: The means of three replications and standard error (SEr ±) were calculated for all the results obtained, and the data were subjected to
236
analysis of variance means by sigma plot 12.5 program.
SC
235
M AN U
237 238
3. Results and discussions
239
3.1.
240
The fungus isolate Aspergillus terreus AF-1 was identified by molecular methods
241
scheme 1. Fungal ITS fragment was identified from PCR and sequencing approaches
242
(Amplification and sequencing of ITS region have resulted in approximately 600 bp).
243
We constructed a maximum-likelihood phylogenetic tree to correlate our ITS
244
sequence with previously described sequences, the results showed that the sequenced
245
ITS fragment was related to the topology of Aspergillus terreus with a similarity of
246
98%.
AC C
EP
TE D
Identification of the isolate Aspergillus terreus AF-1
11
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
247 248
Scheme 1: Phylogenetic analysis of ITS sequences of the fungal strain with the
249
sequences from NCBI. Symbol ■ refers to ITS fragments retrieved from this
250
study. The analysis was conducted with MEGA 6 using neighbor-joining method.
252
TE D
251
3.2. Biosynthesis of ZnO NPs using A. terreus AF-1 Over the past few decades, the green bio-synthesis of metallic nanoparticles and their
254
oxides has been gained an importance suggested as possible alternatives to chemical and
255
physical methods. Proteins and enzymes secreted by fungi have effective role in the
256
reduction of ZnO to ZnO NPs, besides stabilizing these formed nanoparticles [20]. In this
257
context, A. terreus AF-1 was isolated and identified as aforementioned in scheme 1 and
258
then used as a bioreactor for green synthesis of ZnO NPs through harnessing bioactive
259
macromolecules such as proteins and enzymes secreted therefrom. Appearance of a
260
creamy-white precipitate after contacting of biomass filtrate with zinc acetate at the end
261
of reaction indicated the formation of hydrate ZnO (ZnO.H2O). After calcination of the
262
latter, ZnO-NPs were obtained as a white powder.
AC C
EP
253
12
ACCEPTED MANUSCRIPT
263 264
3.3.Factors affecting on the biosynthesis ZnO-NPs
265
Biosynthesis of ZnO-NPs were indicated by UV-visible spectroscopy as represented in
267
Figure 1.
RI PT
266
SC
0.8 0.6 0.4 0.2 0 350
370
269
M AN U
Absorbance
268
390 410 Wave length (nm)
430
450
Figure 1: UV-vis spectrophotometer of the biosynthesized ZnO-NPs and their optical
271
pictures picked during preparation process of: Zinc acetate solution (A), biomass
272
filtrate (B), and white precipitate formed upon addition of zinc acetate to biomass
273
filtrate (C).
EP
274
TE D
270
It was shown that the maximum absorption peak of the formed ZnO-NPs was occurred at
276
wavelength 390 nm, due to its surface plasmon resonance. These observation is in
277
agreement with the earlier studies on the biosynthesis of ZnO-NPs, which indicating that
278
the characterization peak of ZnO-NPs is lied around wavelength of 320-390nm [21].
279
Moreover, the absorption band in Figure 1 is slightly symmetrical with broad in width at
280
wavelength 390nm. These could refer to the formation of spherical ZnO with
281
polydispersed narrow sizes particles.
AC C
275
13
ACCEPTED MANUSCRIPT
Environmental conditions of the mixture of the fungal biomass filtrate and zinc
283
acetate have been the critical component directly affecting the productivity of ZnO-NPs
284
and also the process economics. The physical conditions of this mixture directly monitor
285
the rate of enzyme activity which reflects on the synthesis of ZnO-NPs. Therefore
286
optimization of physical parameters will not only support good growth but also enhance
287
the product yield. Hence, in seek of the optimization of the biosynthesized ZnO-NPs, the
288
UV-visible spectroscopy was used to determine the proper conditions applied during
289
preparation by examining the absorbance of the obtained ZnO-NPs suspensions at
290
wavelength 390 nm. Of these variables under investigation Zinc acetate concentration,
291
pH and incubation period of biomass filtrate with zinc acetate are shown below in Figure
292
2.
M AN U
SC
RI PT
282
AC C
EP
TE D
293
14
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
294
Figure 2: Factors affecting the biosynthesis of ZnO-NPs as a function of absorbance
296
at wavelength 390nm. A) Different zinc acetate concentration, B) Different pH
297
values and C) Different incubation periods
EP
298
TE D
295
Effect of zinc acetate concentration
300
Biosynthesis of ZnO-NPs with different concentrations of zinc acetate solution 0.5mM to
301
2.5mM was studied. Data represented in figure 2A showed that, by increasing the
302
concentration of zinc acetate, the absorbance at wavelength 390nm increases up to 2mM.
303
These evidences indicated the high efficiency of the bio-active molecules (proteins and
304
enzymes) comprised biomass filtrate on formation of ZnO-NPs at high concentration of
305
zinc acetate. Further increasing in the zinc acetate into 2.5mM, the bio-active molecules
AC C
299
15
ACCEPTED MANUSCRIPT
306
unable to protect the formed ZnO from agglomeration which leads to aggregate to bigger
307
sizes and hence, the absorbance decreased significantly [22].
308
Effect of different pH values
310
The effect of varying different pH values from 5 to 11 onto the biosynthesis of ZnO-NPs
311
by A. terreus AF-1 is shown also in Figure 2B, which showed the highest productivity at
312
maximum absorbance was occurred at alkaline pH-10. This could be attributed to the
313
behavior of the bio-active molecules secreted by A. terreus AF-1 in the solution which
314
acting as capping agent of ZnO-NPs is more stable and more reactive at alkaline medium
315
than acidic [23].
316
M AN U
SC
RI PT
309
Effect of incubation periods
318
The incubation period is a critical factor, which not only effect on the secretion of
319
bioactive molecules such as proteins and enzymes, but also effect on the reducing affinity
320
of ZnO to nanoparticles. Therefore, incubation period of the mixed biomass filtrate with
321
zinc acetate of concentration 2.0mM was performed at pH 10. Data illustrated in Figure
322
2C revealed that, the best time for extracellular biosynthesis of ZnO-NPs was obtained
323
when merely the biomass of A.terreus AF-1 has been mixed with zinc acetate for duration
324
of 2 days which the secretion of the bio-active molecules were yielded with highly
325
concentration in the biomass filtrate. After 2 days of incubation age, the bio-active
326
molecules may be, with the missing of the growth ingredients needed, the affinity of
327
fungus biomass to release more of those bio-active molecules was limited and/or most of
328
the secreted molecules tend to degrade or deactivate.
AC C
EP
TE D
317
16
ACCEPTED MANUSCRIPT
329 330
3.4.
Characterizations of ZnO-NPs
TEM measurement was carried out to determine the morphology and the
332
approximate size of the biosynthesized ZnO-NPs. Figure 3A revealed that, ZnO-NPs
333
with spherical shape were formed successfully using A.terreus AF-1 filtrate with well-
334
dispersed narrow sized particles surrounding with capping proteins and enzymes. The
335
average size of the formed ZnO-NPs is lied in the range of 10-45nm.
336
FT-IR analysis was performed to detect any chemical changes in functional groups.
337
Figure 3B is a typical FT-IR for biomass filtrate and ZnO-NPs. Results from biomass
338
filtrate spectra showed that, maximum absorption peak seen at near 1650cm-1 which is
339
related to (C=O) stretching vibration of peptide bonds and the peak near 3300 cm-1 is
340
thought to be N-H bending vibration. On the other side, the maximum spectrum peaks
341
picked from ZnO NPs spectra are seen at 3421, 2937, 2359, 1575, 1401, 1025, 940, 676
342
and 512 cm-1. Indeed, the peak at 512 cm-1 is the characteristic peak related to the
343
absorption of Zn-O bonds, while peak found at 1025cm-1 is corresponding to the C-O
344
stretching in amino acids. Maximum absorption peak at 3421 cm-1 may be attributed to
345
the characteristic absorption of OH- and NH- groups. Furthermore, the intensity of NH-
346
band occurred near 3300 cm-1 were decreased accompanied with shifting of (C=O) amide
347
absorption band to lower wavelength 1544cm-1. This obvious refers to the coordinating
348
bonds occurred between ZnO and proteins secreted fungi. From above results, it is clearly
349
evident that, the proteins secreted biomass filtrate from fungus A. terreus AF-1 have the
350
main role in size reduction of ZnO with narrow size distribution in well stabilized
351
nanoform.
AC C
EP
TE D
M AN U
SC
RI PT
331
17
ACCEPTED MANUSCRIPT
On the other hand, the crystalline nature of ZnO nanoparticles were confirmed by XRD
353
analysis (Figure 3C). XRD spectra showed well defined peaks at 2θ values 31.6°, 34.5°,
354
36.5°, 47.45°, 56.55°, 62.82°, 66.14°, 67.97° and 68.93° corresponding to (100), (002),
355
(101), (102), (110), (103) and (112) of ZnO-NPs, which revealing that the sample was
356
polycrystalline wurtzite structure (Zincite, JCPDS 5-0664).
357
On the other hand, the size and size distribution of ZnO nanoparticles in colloidal
358
solution were analyzed by the making use of DLS technique (Figure 3D). The results
359
represented in Figure 3D make it evident that, the particles obtained were polydispersed
360
mixture with average size of 175.85 nm (95.4%). Considering the presence of the capping
361
proteins and enzymes surrounding particles, the hydrodynamic radius obtained from DLS
362
does not give more information about the individual ZnO-NPs, however, it is considered
363
as a good to measure oval all dimension besides the width of nanoparticles and the
364
polymers which covering the particles. Whereas, the stability of colloidal solution which
365
depending on the surface charge of the formed nanoparticles was determined by zeta
366
potential analysis. In general, the particles keep away each other without any aggregates,
367
when the particles in a colloidal solution have large negative or positive zeta potential
368
values (greater than +30 mV or smaller than −30 mV) [24]. The biosynthesized ZnO-NPs
369
were highly stabled as have a zeta potential found to be -46.6 mV. This high value
370
confirms the high stability of colloidal solution.
371
Moreover, TGA of ZnO-NPs was shown in Figure 3E. The initial weight loss is assigned
372
to be 13.57% which due to water evaporation. The major weight loss occurred between
373
temperature 151 0C – 577 0C, which about 14.62% of the original weight. This weight
374
loss is attributed to the thermal decomposition of the organic compounds presented in the
AC C
EP
TE D
M AN U
SC
RI PT
352
18
ACCEPTED MANUSCRIPT
375
sample under investigation. Whereas, the remaining weight after 800 0C is related to ash
376
containing inorganic Zn. The close examination from the TGA results, it would reveal
377
that, ZnO-NPs were covered with 14.62% of proteins secreted fungi.
RI PT
378
380
AC C
EP
TE D
M AN U
SC
379
381
Figure 3. A) TEM image, B) FTIR spectra, C), XRD pattern, D) Particle size
382
distribution and E) TGA of ZnO-NPs synthesized by Aspergillus terreus AF-1.
383 19
ACCEPTED MANUSCRIPT
384
•
Antibacterial activity of ZnO-NPs.
The critical importance of ZnO-NPs being in their activity against abroad spectrum of
386
human pathogenic bacteria. Therefore, ZnO-NPs synthesized using A. terreus AF-1 were
387
investigated for their antibacterial activity against both Gram positive and Gram negative
388
bacteria. In general, the inhibitory action for biosynthesized ZnO-NPs which represented
389
by diameter of clear zone was more effective against Gram positive than Gram negative
390
bacteria. However, the diameter of clear zone formed due to 100 µL of ZnO-NPs (2000
391
µg/mL) was 20.2±0.2, 19.1±0.2, 14.2±0.2 and 14.1±0.2 for Bacillus subtilis,
392
Staphylococcus aureus, Escherichia coli and Pseudomonas aeruginosa, respectively
393
(Figure 4). The inhibitory action for biosynthesized ZnO-NPs may be due to reacting of
394
nanoparticles with bacterial protein by combining the thiol (-SH) groups, and hence leads
395
to inactivation of proteins and bacterial growth [25]. Gupta, et al., [26] explained the
396
mechanism of nanoparticles in bacterial growth reduction through interact with
397
phosphorous moieties in DNA, which lead to inactivation of DNA replication and hence
398
inhibition of enzymes functions. Whereas, Manke, et al., reported a new mechanism
399
which showing that nanoparticles are lead to changes in biological activities including
400
reactive oxygen species (ROS) thereby cause membrane damage leading too cell death
401
[27]. The exact mechanism of antimicrobial generated by NPs are not completely well
402
understood yet.
404
SC
M AN U
TE D
EP
AC C
403
RI PT
385
3.5.
Minimum Inhibitory Concentration (MIC)
405
The diameter of inhibition zone and its relation to the concentration of nanoparticles were
406
studied by Shaheen and Fouda [28] to confirm the antibacterial activity was dose 20
ACCEPTED MANUSCRIPT
dependent. Therefore, it is compulsory to detect the MIC to ZnO-NPs for each bacterial
408
strain. To this end, different concentrations of ZnO-NPs (1000, 500, 250 and 125 µg/mL)
409
were used. Regards to the data represented graphically in Figure 4, the obtained MIC for
410
Gram Positive Bacillus subtilis, Staphylococcus aureus was 250 µg/mL with clear zone
411
11.0±0.1mm and 10.5±0.2mm respectively. Whereas, the obtained MIC for Escherichia
412
coli and Pseudomonas aeruginosa was 500 µg/mL with inhibition zone 9.2±0.1mm and
413
9.3±0.3mm, respectively.
TE D
M AN U
SC
RI PT
407
EP
414
Figure 4. Antibacterial activity and MIC for ZnO-NPs at different concentrations (2000, 1000,
416
500, 250 and 125 µg/mL) against different human pathogenic bacteria
417 418
AC C
415
3.6.
In vitro cytotoxicity of ZnO-NPs
419
Cell morphology
420
Either variation in cell shape or cell morphology in culture is the first as well as the most
421
notably observation shown after exposure to nanoparticles or any toxic materials.
422
Therefore, the light inverted microscope could be used to monitor the cell shape and 21
ACCEPTED MANUSCRIPT
morphological changes dependent on ZnO-NPs exposure dose. The normal cell line
424
spread continuously on plate and showed epithelial characteristic morphology. The cell
425
exposed to different concentrations of ZnO-NPs gradually lost their phenotypic character.
426
As shown in Figure 5, at high concentration of ZnO-NPs, the cell become partial or
427
complete loss of monolayer, rounding, shrinking or cell granulation when compared to
428
untreated control cells. The light inverted microscope image proved, undoubtedly, that
429
the damage caused in cell morphology is ZnO-NPs dose dependent.
SC
RI PT
423
431
AC C
EP
TE D
M AN U
430
432
Figure 5. Light inverted micrographs proved morphological change for three type of cell
433
lines exposure to different concentration of ZnO-NPs. A) Clone-9 cell. B) Vero cell and
434
C) Caco-2 cell.
22
ACCEPTED MANUSCRIPT
435
MTT assay
437
Viability assays are basic stage in toxicology that explain the cellular response to a
438
toxicant. Also, they give information on the cell death, survival, and metabolic activities
439
[29]. MTT assay is sensitive colorimetric assays for the determination of the number of
440
viability in cell proliferation and cytotoxicity assays. Data represented in Figure 6
441
revealed that, cell mortality for normal and cancer cells were also dose dependent when
442
exposure to different concentrations of ZnO-NPs. Data showed that, the IC50 for normal
443
cell represented by clone-9 and vero cell were 26.85 µg/mL and 27.05 µg/mL,
444
respectively. Whilst, IC50 for cancer cell (Caco-2) was 79.57 µg/mL.
445
treatment of cotton fabrics with ZnO-NPs is highly recommended to be performed at
446
concentration lower than 26.85 µg/mL, in order to keep the process safe for human.
M AN U
SC
RI PT
436
AC C
EP
TE D
447
448
23
Thus, the
ACCEPTED MANUSCRIPT
449 450
Figure 6. Cell mortality for Clone-9 cell, Vero cell and Caco-2 cell at different
451
concentrations of ZnO-NPs synthesized by A. terreus AF-1.
RI PT
452 453 454
3.7.Application of the biosynthesized ZnO-NPs into cotton fabric.
Owing the unique properties of ZnO-NPs towards antibacterial activity and UV-
456
protection, the biosynthesized ZnO-NPs have been used in multifunctional textile fabrics.
457
In the context, ZnO-NPs were applied to cotton fabrics according to method mentioned in
458
our previous works [30]. ZnO-NPs were resuspended in distilled water to get final
459
concentration of 20 µg/mL (20ppm). Moreover, the deposition of ZnO-NPs on cotton
460
fabrics and their chemical composition were demonstrated by SEM-EDX instrument
461
(Figure 7A-D). The deposition of ZnO-NPs was clearly shown in the SEM image of the
462
treated cotton fabrics (Figure 7B), which indicates the homogenously distribution of
463
ZnO-NPs on the cotton fabrics surface whenever compared with control sample (Figure
464
7A) which seemed very smooth surface (Figure 7A). Furthermore, the chemical
465
compositions of the treated cotton fabrics were determined by Energy Dispersive X-ray
466
spectrometer (EDX) as showed in Figure 7C and D. The obtaining results showed that,
467
zinc element in zinc oxide nanoparticles occupied 2% of total number of elements found
468
in the tested sample as concluded from mapping image (Fig. 7C), whereas the weight
469
percent of the Zinc was about 1.03 % as calculated from EDX spectra (Fig. 7D).
AC C
EP
TE D
M AN U
SC
455
24
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
TE D
470
Figure 7. SEM image of: (A) untreated cotton fabrics with ZnO-NPs, (B) treated cotton
472
fabrics with ZnO-NPs, and (C) mapping picture of the surface of treated fabrics with
473
ZnO-NPs. (D) EDX of treated sample with elemental analysis of the ZnO-NPs contents.
475
3.8.Efficiency of the nano-zinc particles as antibacterial agent
AC C
474
EP
471
476
Cotton fabrics treated with nano-sized zinc colloids solution exhibit moderate
477
antibacterial efficiency against both Gram positive and negative bacteria. At 20ppm of
478
nano-zinc oxide colloid solution used for treatment, the reduction of bacterial growth was
479
82.2±0.3 % and 81.9±0.2 % for Staphylococcus aureus and Bacillus subtilis,
480
respectively. While bacterial reduction for gram negative bacteria represented by
25
ACCEPTED MANUSCRIPT
481
Pseudomonas aeruginosa and Escherichia coli were 74.8±0.5 % and 75.4±0.3 %,
482
respectively.
483
3.9.UV-protection of Cotton fabrics loaded by zinc oxide nanoparticles
RI PT
484
The absorption characteristic of the treated cotton fabrics with ZnO-NPs compared with
486
untreated fabrics, which expressed as UPF values and blocking percent for UVA and
487
UVB are represented in Table 1. It can be concluded that, the UPF value for treated
488
cotton fabrics was 16.1 which is a good protection index for the treated fabrics with ZnO-
489
NPs according to Australian/New Zealand Standard AS/NZS 4399:1996 [31], compared
490
with UPF value of 4 for untreated fabrics which consider a bad protection index [31]. UV
491
is the form of invisible radiation emitted from sun and classified into UVA (315-400nm)
492
and UVB (290-315nm) which damages collagen fibres and accelerates skin ageing but
493
UVB is more dangerous than UVA because it is directly destroy DNA and causes skin
494
cancer [32]. Therefore, data presented in Table 1 revealed that, ZnO-NPs loaded cotton
495
fabrics can be blocking UVA and UVB at 76.3% and 85.4%, respectively, when
496
compared to untreated fabrics which blocking at 66.9% and 79% respectively.
M AN U
TE D
EP
498
AC C
497
SC
485
26
ACCEPTED MANUSCRIPT
Table 1. UPF protection values of untreated and treated cotton fabrics with ZnO-NPs. Fabrics
UPF
protection Transmittance (%)
value
UVA
UVB
(315-400nm)
(290-315nm)
4
29.1
14
Treated
16.1
23.7
10.6
UVA
UVB
66.9
79
76.3
85.4
SC
Untreated
500
M AN U
501 502
Blocking (%)
RI PT
499
4. Conclusion
Although lots of chemical and physical methods were frequently used for the synthesis of
504
ZnO-NPs, but these methods possess several disadvantages through either toxic solvents
505
used or undesirable by-products yielded in addition to their high energy consumption.
506
Therefore, the main objectives of the current study were to produce ZnO-NPs by
507
microbial action and to apply these ZnO-NPs to fabricate the multifunctional medical
508
textile fabrics with the safe dose during application. To achieve these goals, the work
509
was designed to bring into synthesis of ZnO-NPs using biological method prolonging
510
with the investigation of their both antibacterial activity and in-vitro cytotoxicity prior
511
applying of ZnO-NPs into cotton fabrics for rendering them UV-protection and
512
antibacterial properties with safe dose. Therefore, the fungus Aspergillus terreus AF-1
513
was successfully used in extracellular biosynthesis of ZnO-NPs using fungus biomass
514
filtrate without addition of any hazardous materials, followed by optimization of the
515
biosynthesized ZnO-NPs and then characterized by UV-Visible spectroscopy,
516
transmission electron microscope (TEM) Fourier Transform-Infra Red (FT-IR)
AC C
EP
TE D
503
27
ACCEPTED MANUSCRIPT
spectroscopy, X-ray diffractometry (XRD) analysis and Dynamic light scattering analysis
518
(DLS). Results from UV-vis. Spectra revealed that ZnO-NPs were successfully
519
synthesized by dint of Aspergillus terreus AF-1 at optimum conditions include incubation
520
period of the biomass filtrate with (2.0mM) zinc acetate for 48h at pH 10. At these
521
conditions, an absorption peak was observed at maximum wavelength 390nm which
522
attributed to the SPR of ZnO-NPs. Further, TEM micrographs confirmed the formation of
523
well-dispersed spherical nanoparticles with an average size of 10-45nm. Furthermore, the
524
particle size analyzer revealed that ZnO-NPs were formed as a polydispersed mixture
525
with average size of 175.8nm, which could be due to presence of covering layer of
526
bioactive secreted molecules surrounding nanoparticles. Thus, the zeta potential was
527
raised to be -46.6 mV, indicating the high stability of the nanoparticles formed.
528
On the other hand, the antibacterial activity and in-vitro cytotoxicity of biosynthesized
529
ZnO-NPs were assessed. Results revealed that, ZnO-NPs have inhibitory action against
530
Gram positive ((Staphylococcus aureus and Bacillus subtilis) more than Gram negative
531
(Pseudomonas aeruginosa and Escherichia coli) bacteria with MIC 250 and 500 µg/mL,
532
respectively. However, ZnO-NPs showed morphological change and cytotoxic effect on
533
Clone-9, Vero and Caco-2 cell line at high concentrations. Below this concentration,
534
ZnO-NPs were loaded onto cotton fabrics to render them both antibacterial activity and
535
UV blocking properties for application in medical purposes. Our results confirmed that,
536
fabrics loaded with biosynthesized
537
bacterial growth of Staphylococcus aureus, Bacillus subtilis, Pseudomonas aeruginosa
538
and Escherichia coli with percent 82.2±0.3, 81.9±0.2, 74.8±0.5
539
respectively with UPF value 16.4 (good UV protection) compared to untreated fabrics.
AC C
EP
TE D
M AN U
SC
RI PT
517
ZnO-NPs had an ability to inhibit pathogenic
28
and 75.4±0.3 %,
ACCEPTED MANUSCRIPT
540 541
5. References
542
EP
TE D
M AN U
SC
RI PT
[1] Albrecht MA, Evans CW, Raston CL. Green chemistry and the health implications of nanoparticles. Green Chemistry. 2006;8:417-32. [2] Rehana D, Mahendiran D, Kumar RS, Rahiman AK. In vitro antioxidant and antidiabetic activities of zinc oxide nanoparticles synthesized using different plant extracts. Bioprocess and Biosystems Engineering. 2017;40:943-57. [3] Rao MD, Gautam P. Synthesis and characterization of ZnO nanoflowers using Chlamydomonas reinhardtii: A green approach. Environmental Progress & Sustainable Energy. 2016;35:1020-6. [4] Mohmed AA, Fouda A, Elgamal MS, Hassan SE-D, Shaheen TI, Salem SS. Enhancing of Cotton Fabric Antibacterial Properties by Silver Nanoparticles Synthesized by New Egyptian Strain Fusarium Keratoplasticum A1-3. Egyptian Journal of Chemistry. 2017;60:63-71. [5] Yuvakkumar R, Suresh J, Nathanael AJ, Sundrarajan M, Hong S. Novel green synthetic strategy to prepare ZnO nanocrystals using rambutan (Nephelium lappaceum L.) peel extract and its antibacterial applications. Materials Science and Engineering: C. 2014;41:17-27. [6] Rasmussen JW, Martinez E, Louka P, Wingett DG. Zinc oxide nanoparticles for selective destruction of tumor cells and potential for drug delivery applications. Expert opinion on drug delivery. 2010;7:1063-77. [7] Navale GR, Thripuranthaka M, Late DJ, Shinde SS. Antimicrobial activity of ZnO nanoparticles against pathogenic bacteria and fungi. JSM Nanotechnol Nanomed. 2015;3:1033-41. [8] Shaheen TI, El-Naggar ME, Abdelgawad AM, Hebeish A. Durable antibacterial and UV protections of in situ synthesized zinc oxide nanoparticles onto cotton fabrics. International journal of biological macromolecules. 2016;83:426-32. [9] Lobiak E, Shlyakhova E, Bulusheva L, Plyusnin P, Shubin YV, Okotrub A. Ni–Mo and Co–Mo alloy nanoparticles for catalytic chemical vapor deposition synthesis of carbon nanotubes. Journal of Alloys and Compounds. 2015;621:351-6. [10] Hasnidawani J, Azlina H, Norita H, Bonnia N, Ratim S, Ali E. Synthesis of ZnO nanostructures using sol-gel method. Procedia Chemistry. 2016;19:211-6. [11] Mănoiu V-S, Aloman A. Obtaining silver nanoparticles by sonochemical methods. UPB Sci Bull B. 2010;72:7. [12] Moghaddam AB, Nazari T, Badraghi J, Kazemzad M. Synthesis of ZnO nanoparticles and electrodeposition of polypyrrole/ZnO nanocomposite film. Int J Electrochem Sci. 2009;4:247-57. [13] Foudaa A, Saad E, Elgamala MS, Mohmedb AA, Salema SS. Optimal factors for biosynthesis of silver nanoparticles by Aspergillus sp. Al Azhar Bulletin of Science, Conf, March 2017. 2017;9th. [14] Singh D, Rathod V, Ninganagouda S, Hiremath J, Singh AK, Mathew J. Optimization and characterization of silver nanoparticle by endophytic fungi Penicillium sp. isolated from Curcuma longa (turmeric) and application studies against MDR E. coli and S. aureus. Bioinorganic chemistry and applications. 2014;2014. [15] Lynch I, Dawson KA, Linse S. Detecting cryptic epitopes created by nanoparticles. Sci Stke. 2006;2006:pe14-pe.
AC C
543 544 545 546 547 548 549 550 551 552 553 554 555 556 557 558 559 560 561 562 563 564 565 566 567 568 569 570 571 572 573 574 575 576 577 578 579 580 581 582
29
ACCEPTED MANUSCRIPT
EP
TE D
M AN U
SC
RI PT
[16] Fouda A, Khalil A, El-Sheikh H, Abdel-Rhaman E, Hashem A. Biodegradation and detoxification of bisphenol-A by filamentous fungi screened from nature. J Adv Biol Biotechnol. 2015;2:123-32. [17] Wang Y, Lu Z, Wu H, Lv F. Study on the antibiotic activity of microcapsule curcumin against foodborne pathogens. International journal of food microbiology. 2009;136:71-4. [18] Philip S, Kundu GC. Osteopontin Induces Nuclear Factor κB-mediated Promatrix Metalloproteinase-2 Activation through IκBα/IKK Signaling Pathways, and Curcumin (Diferulolylmethane) Down-regulates These Pathways. Journal of Biological Chemistry. 2003;278:14487-97. [19] Fouda A, Shaheen TI. Silver Nanoparticles: Biosynthesis, Characterization and Application on Cotton Fabrics. Microbiology Research Journal International. 2017;20:14. [20] Bhuyan T, Mishra K, Khanuja M, Prasad R, Varma A. Biosynthesis of zinc oxide nanoparticles from Azadirachta indica for antibacterial and photocatalytic applications. Materials Science in Semiconductor Processing. 2015;32:55-61. [21] Vennila S, Jesurani SS. Eco-friendly green synthesis and characterization of stable ZnO Nanoparticle using small Gooseberry fruits extracts. International Journal of ChemTech Research. 2017;10:5. [22] Rao CR, Trivedi D. Synthesis and characterization of fatty acids passivated silver nanoparticles—their interaction with PPy. Synthetic Metals. 2005;155:324-7. [23] Yedurkar S, Maurya C, Mahanwar P. Biosynthesis of zinc oxide manoparticles using Ixora coccinea leaf extract—A green approach. Open J Synth Theory Appl. 2016;5:1-14. [24] Meléndrez M, Cárdenas G, Arbiol J. Synthesis and characterization of gallium colloidal nanoparticles. Journal of colloid and interface science. 2010;346:279-87. [25] El-Rafie M, Mohamed A, Shaheen TI, Hebeish A. Antimicrobial effect of silver nanoparticles produced by fungal process on cotton fabrics. Carbohydrate polymers. 2010;80:779-82. [26] Gupta P, Bajpai M, Bajpai S. Investigation of antibacterial properties of silver nanoparticleloaded poly (acrylamide-co-itaconic acid)-grafted cotton fabric. Journal of Cotton Science. 2008. [27] Manke A, Wang L, Rojanasakul Y. Mechanisms of nanoparticle-induced oxidative stress and toxicity. BioMed research international. 2013;2013. [28] Shaheen TI, Fouda A. Green Approach for one-pot Synthesis of Silver Nanorod using Cellulose Nanocrystal and their Cytotoxicity and Antibacterial assessment. International Journal of Biological Macromolecules. 2017. [29] Popescu R, Heiss EH, Ferk F, Peschel A, Knasmueller S, Dirsch VM, et al. Ikarugamycin induces DNA damage, intracellular calcium increase, p38 MAP kinase activation and apoptosis in HL-60 human promyelocytic leukemia cells. Mutation Research/Fundamental and Molecular Mechanisms of Mutagenesis. 2011;709:60-6. [30] El-Rafie MH, Shaheen TI, Mohamed AA, Hebeish A. Bio-synthesis and applications of silver nanoparticles onto cotton fabrics. Carbohydrate polymers. 2012;90:915-20. [31] 4399 AN. Sun protective clothing - evaluation and classification. 1996. [32] Dubrovski PD. Wowen fabric and ultraviolet protection. Woven fabric engineering: InTech; 2010.
AC C
583 584 585 586 587 588 589 590 591 592 593 594 595 596 597 598 599 600 601 602 603 604 605 606 607 608 609 610 611 612 613 614 615 616 617 618 619 620 621 622 623 624
30
ACCEPTED MANUSCRIPT
Highlights Spherical narrow-sized ZnO-NPs were prepared using fungus Aspergillus terreus. Optimization of the biosynthesized ZnO-NPs was performed.
RI PT
Cytotoxicity dose of ZnO-NPs prior application was studied.
AC C
EP
TE D
M AN U
SC
Antibacterial activity and UV-protection of the treated cotton fabrics were investigated at safe ZnO-NPs dose.
S0882-4010(17)31498-5
DOI:
10.1016/j.micpath.2018.09.030
Reference:
YMPAT 3180
To appear in:
Microbial Pathogenesis
Received Date: 13 November 2017 Revised Date:
10 June 2018
Accepted Date: 16 September 2018
Please cite this article as: Fouda A, EL-Din Hassan S, Salem SS, Shaheen TI, In-Vitro cytotoxicity, antibacterial, and UV protection properties of the biosynthesized Zinc oxide nanoparticles for medical textile applications, Microbial Pathogenesis (2018), doi: https://doi.org/10.1016/j.micpath.2018.09.030. 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.
ACCEPTED MANUSCRIPT
1
In-Vitro cytotoxicity, antibacterial, and UV protection properties of the
3
biosynthesized Zinc oxide nanoparticles for medical textile applications
4
Amr Fouda1, Saad EL-Din Hassan1, Salem S Salem1 and Th. I. Shaheen2*
RI PT
2
5 6
1
7
Cairo, 11884, Egypt.
8
2
9
Behouth St. (former El-Tahrir str.), Dokki, P.O. 12622, Giza, Egypt.
SC
Department of Botany and Microbiology, Faculty of Science, Al-Azhar University, Nasr City,
M AN U
National Research Centre (Scopus affiliation ID 60014618), Textile Research Division, El-
10
*Corresponding Author: Dr. Tharwat Ibrahim Shaheen (PhD), Email:
11
[email protected].
12
TE D
13
Abstract
15
Nowadays, medical textiles have become the most essential and developing part in
16
human healthcare sector. This work was undertaken with a view to harness the bio-active
17
macromolecules secreted by fungi e.g. proteins and enzymes in bio-synthesis of ZnO
18
nanoparticles for multifunctional textiles such as antibacterial activity and UV protection
19
with considering the cytotoxicity limitation. Herein, the isolated fungus, Aspergillus
20
terreus, was allowed to produce proteins which has affinity to cape ZnO-NPs. Various
21
factors affecting the behavior of the secreted proteins on the formed nanoparticles were
22
investigated. Thorough characterizations of the protein capped ZnO-NPs were performed
23
by the using of UV-Visible spectroscopy, transmission electron microscope (TEM)
AC C
EP
14
1
ACCEPTED MANUSCRIPT
Fourier Transform-Infra Red (FT-IR) spectroscopy, X-ray diffraction (XRD) analysis and
25
Dynamic light scattering analysis (DLS). Prior treatment of cotton fabrics with ZnO-NPs,
26
the cytotoxicity of the protein capped ZnO-NPs was examined. After that, the
27
antibacterial activity of the ZnO-NPs before and after treating of cotton fabrics, besides,
28
the UV-protection (UPF) properties were investigated. Results obviously demonstrated
29
the ability of the bio-secreted protein to cape and reduce ZnO to spherical ZnO-NPs with
30
particle size lied around 10-45nm, as indicated form UV-vis., spectra TEM, Zeta sizer,
31
FTIR and XRD. Regarding to the results of cytotoxicity, the treatment of the cotton
32
fabrics with ZnO-NPs were performed at safe dose (20ppm). At this dose, ZnO-NPs
33
loaded samples exhibited reasonable antibacterial activity against both Gram positive and
34
Gram negative bacteria; besides, good UV-protection with reasonable increase in UVA
35
and UVB blocking values. Indeed, nanotechnology based microbiological active
36
molecules opens up new opportunities for us to explore novel applications in terms of
37
green technology.
38
Keywords: Zinc oxide nanoparticles; Biosynthesis; Antibacterial; cytotoxicity; UV
39
protection; medical textile.
41 42
SC
M AN U
TE D
EP
AC C
40
RI PT
24
1. Introduction
Bio-Nanotechnology is a correlation of both biology and nanotechnology. Most
43
recently, bio-nanotechnology is growing up day by day as a quickly developing filed with
44
its application in science and technology with the end goal of assembling new materials
45
at the nanoscale level [1, 2]. In recent years, different industries as textile, health, food,
46
chemicals, and cosmetic products incorporated with nanoparticles (NPs). The 2
ACCEPTED MANUSCRIPT
environmental friendly approach for the biosynthesis of nanoparticles is an opportunity to
48
be safely applied in medical fields [3]. Combination of textile technology and medical
49
science has resulted into a new field called medical textiles. New areas of applications for
50
medical textiles have been identified with the development of new either fiber yarns
51
technology or the combined functional biomedical materials such as nanoparticles. Green
52
synthesis of NPs includes synthesis through plants, bacteria, actinomycetes, fungi [4], and
53
algae permit large scale production of NPs free impurities [5].
SC
RI PT
47
Zin oxide nanoparticles (ZnO-NPs) have attracts attention of many researchers for
55
it is biological and chemical behavior which can be returned to their morphology. ZnO-
56
NPs have been used in various biological application as drug delivery and destroying of
57
tumor cell [6], antibacterial and antifungal activity [7], medical textile industry and UV
58
filtering prosperities [8].
M AN U
54
There are several methods for ZnO-NPs synthesis as chemical vapor synthesis [9],
60
sol-gel method [10] sonochemical [11] and thermal decomposition [12]. Processing steps
61
and physical factor as pH, temperature and pressure for these methods are difficult
62
controlling beside producing by-product which may be toxic for ecosystem; therefore,
63
green synthesis of ZnO-NPs is most preferred. Fungi are simple handling and possess
64
different variety of proteins and enzymes in their cell, therefore it is considered excellent
65
candidates for ZnO-NPs synthesis.
EP
AC C
66
TE D
59
Optimization of physic-chemical parameters such as substrate concentration, pH
67
and temperature, agitation rate for medium and incubation period play an important roles
68
in green synthesis of nanoparticles [13, 14]. The activity of ZnO-NPs against tumor cell
3
ACCEPTED MANUSCRIPT
69
due to smaller nanoparticle size, generation of reactive oxygen species (ROS) and highly
70
specific surface area [15]. In the current study, we aimed to fabricate the multifunctional medical textile
72
through using of environmentally benign system. To achieve this goal, this work was
73
designed to synthesize and optimize of ZnO-NPs through using of the secreted proteins
74
by the isolated fungus Aspergillus terreus AF-1, in concurrent with investigation of their
75
MIC (minimum inhibitory concentration) and in-vitro cytotoxicity of the biosynthesized
76
ZnO-NPs prior applying of ZnO-NPs onto cotton fabrics. At safe concentration, ZnO-
77
NPs were loaded onto cotton fabrics to also investigate both antibacterial activity and
78
UV-protection properties.
79
M AN U
SC
RI PT
71
2. Materials and Methods
81
2.1.Isolation and Identification of fungal isolate
82
The soil fungus, Aspergillus terreus AF-1 was isolated from contaminated soil dye,
83
Egypt (GPS N: 30o 15 54.51: E: 31o 45 39.95). Isolation of fungi was carried out by
84
plating the inoculum on PDA after serial dilutions of soil sample and incubated at 28± 2
85
°C for 3-4 days. Bacterial contamination was inhibited by supplementing the medium
86
with chloramphenicol at a concentration of 10 µg mL-1 after autoclaving.
87
Morphologically differed colonies were individually picked up and reinoculated on PDA
88
for purification, and then kept at 4 °C for further study [16].
89
Molecular identification was conducted based on amplification and sequencing of
90
internal transcribed spacer (ITS) region. Genomic DNA was extracted using the protocol
91
of Gene Jet Plant genomic DNA purification Kit (Thermo). The ITS region was amplified
AC C
EP
TE D
80
4
ACCEPTED MANUSCRIPT
92
in polymerase chain reaction (PCR) using the genomic DNA as template and primers of
93
ITS1
94
TCCGCTTATTGATATGC-3 ̀). The PCR mixture (50µL) contained Maxima Hot Start
95
PCR Master Mix (Thermo), 0.5µM of each primer, and 1µL of extracted fungal genomic
96
DNA. The PCR was performed in a DNA Engine Thermal Cycler by Sigma Scientific
97
Services Company (Cairo, Egypt) with a hot starting performed at 94ºC for 3 min,
98
followed by 30 cycles of 94ºC for 0.5 min, 55ºC for 0.5 min, and 72ºC for 1 min,
99
followed by a final extension performed at 72ºC for 10 min. The commercial sequencing
100
was conducted using ABI 3730x1 DNA sequencer at GATC Company (Germany). The
101
ITS sequence was compared against the GenBank database using the NCBI BLAST
102
program. Sequences were then compared with ITS sequences in the GenBank database
103
using BLASTN. Multiple sequence alignment was done using ClustalX 1.8 software
104
package (http://wwwigbmc.u-strasbg.fr/BioInfo/clustalx) and a phylogenetic tree was
105
constructed by the neighbor-joining method using MEGA (Version 6.1) software. The
106
confidence level of each branch (1,000 repeats) was tested by bootstrap analysis.
108
-3 ̀)
and
ITS4
(5 ̀-
TCC
TE D
M AN U
SC
RI PT
TCCGTAGGTGAACCTGCGG
EP
107
(5 ̀-
2.2.Biosynthesis of ZnO Nanoparticle using protein secreted fungi Aspergillus terreus AF-1 was grown up in 250 mL Erlenmeyer flask containing 100 mL
110
Czapek Dox (CD) fermentative broth medium for 3 days at pH 6.0, 28±2oC, and shaking
111
of 150 rpm. After incubation period, the fungal biomass was separated using Whatman
112
filter paper No. 1 by filtration method, and washed thrice with sterile distilled H2O to
113
remove any medium components. The harvested fungal biomass (15 g) were re-
114
suspended in 100 mL sterile distilled H2O in an orbital shaker (150 rpm) for 48 h. at
AC C
109
5
ACCEPTED MANUSCRIPT
115
28±2oC. The cell-free filtrate was obtained by separating the fungal biomass using
116
Whatman filter paper No. 1 and used for ZnO-NPs production as the following. Different ratios of Zinc acetate Zn(CH3CO2)2 were mixed and incubated with cell
118
free filtrate at 28±2oC for 24h on orbital shaker (150 rpm). After completion of
119
incubation period, a creamy-white precipitate, mainly Zn(OH)2, was indicated. The latter
120
was separated and then dried at 150 oC for 48h. The bio-transformed product was
121
eventually collected and subjected for further investigation.
2.3.Factors affecting ZnO-NPs production.
M AN U
123
SC
122
RI PT
117
Different variables such as incubation period, Zn (CH3CO2)2 concentrations (0.5mM to
125
2.5mM), and pH (5.0-11) which influencing on the production and distribution of the
126
particle size of ZnO-NPs were studied using UV-visible spectroscopy (JENWAY 6305
127
Spectrophotometer) after resuspension in distilled water.
128
TE D
124
2.4.Characterization of the optimized ZnO-NPs
130
The particle size and shape of the biosynthesized ZnO-NPs were preliminary
131
characterized by using transmission electron microscope (TEM) measurements through
132
using drop coating method in which a drop of solution containing nanoparticles was
133
placed on the carbon-coated copper grids and kept under vacuum desiccation for
134
overnight before loading them onto a specimen holder. For further confirmation, the
135
dynamic light scattering analysis (DLS) was employed in order to investigate the particle
136
size distribution of synthesized nanoparticles as well as check the stability of the
137
nanoparticles by indicating the zeta potential measurement.
AC C
EP
129
6
ACCEPTED MANUSCRIPT
Moreover, the characteristic functional groups present in synthesized nanoparticles
139
molecules were analyzed using Fourier Transform-Infra Red (FT-IR) spectroscopy. The
140
samples were mixed with KBr (binding agent) and were loaded into discs at high
141
pressure. These discs were scanned in the range of 400 to 4000 cm-1 to obtain FT-IR
142
spectra. The crystalline structure of ZnO-NPs was characterized by XRD analysis.
143
Finally, thermal properties of ZnO NPs were measured using Thermal Gravimetric
144
Analysis (TGA/DTA-60H instrument (SHIMADZU) to determine the organic to
145
inorganic contents. Decomposition profiles of TGA were recorded at a heating rate of
146
10.0 0C/min between room temperature and 800.0 0C in nitrogen gas.
M AN U
SC
RI PT
138
147 148 149
2.5.Biological activity of the biosynthesized ZnO-NPs Antibacterial activity of ZnO-NPs
The antibacterial activity of biosynthesized ZnO-NPs was evaluated against Gram
151
positive (Staphylococcus aureus ATCC 6538, Bacillus subtilis ATCC 6633) and Gram
152
negative bacteria (Pseudomonas aeruginosa ATCC 9027, Escherichia coli ATCC 8739)
153
using agar well diffusion method [17]. Each bacterial strain was swabbed uniformly onto
154
individual Mueller Hinton agar plates. In each plate, wells was cut out using a standard
155
cork borer (7 mm diameter). Using a micropipette, 100 µL of Zinc oxide nanoparticles
156
(2000 µg/mL) was added into each well. After incubation at 37 °C for 24 h, the diameter
157
of inhibition zones was measured in mm and the results were recorded. The experiments
158
were performed in three replicates.
159
AC C
EP
TE D
150
Minimum Inhibitory Concentration (MIC)
7
ACCEPTED MANUSCRIPT
MIC of ZnO-NPs against previous Gram positive and Gram negative bacteria were
161
checked by agar well diffusion method. Different concentration of biosynthesized ZnO-
162
NPs (1000, 500, 250 and 125 µg/mL) were made. Each bacterial strain was swabbed
163
uniformly onto individual Mueller Hinton agar plates, and wells were cut out using a
164
standard cork borer (7 mm diameter). A 100 µL of each concentration was poured in to
165
wells and the tested plates were incubated at 37 °C for 24 hours. The minimum
166
concentration of ZnO-NPs showing inhibition zone was considered to be MIC.
167
Experiment was performed in triplicates.
168
In vitro cytotoxicity of ZnO-NPs against cancer and normal cells •
SC
M AN U
169
RI PT
160
Cell culture
The human colorectal adenocarcinoma cells (Caco-2), normal Vero cells (kidney of
171
African green monkey) and normal rat liver epithelial cell (colne-9) were procured from
172
ATCC.
173
•
TE D
170
Cell morphology
Morphological changes in epithelial cells in response to ZnO-NPs, after 24 h of
175
incubation were assessed by light inverted microscope (Nikon, Japan). Cells were
176
cultured in 96-well plates at a density of 1 × 105 cells/well and treated with double fold
177
dilution of biosynthesized ZnO-NPs (1000 µg/mL to 3.9 µg/mL).
179
AC C
178
EP
174
•
MTT assay
180
The cytotoxicity of ZnO-NPs was evaluated by cell viability assay MTT [3-(4, 5-
181
dimethylthiazol-2-yl)-2, 5-diphenyl tetrazolium bromide] using Caco-2 cell, Vero cell &
182
Clone-9 cell. In brief, the cell (1 X 105 cells/mL) grown in 96-well plates and treated with
8
ACCEPTED MANUSCRIPT
different concentration of ZnO-NPs (double-fold dilution) represented as 1000, 500, 250,
184
125, 62.5, 31.25, 15.62, 7.81 and 3.9 µg/mL for 24h at 37oC. The cell were future
185
incubated with MTT (5 mg/mL in phosphate buffered saline) at 37oC / 5% CO2 for 1-5 h.
186
Adding the formazan (MTT metabolic product dissolved in 200 µL DMSO) to 96-well
187
plate. The color intensity was measured at 560 nm using an enzyme linked
188
immunosorbent assay (ELISA) reader [18]. The experiments were performed in
189
triplicates. The percentage cell viability was then calculated with respect to control (cells
190
incubated without zinc oxide nanoparticles) as follows:
SC
RI PT
183
Cell viability % = (sample absorbance / control absorbance) x100.
192
Cell toxicity % =100 – [(sample absorbance / control absorbance) x100].
M AN U
191
193
195
2.6.Application of ZnO-NPs as a precursor for medical textiles •
Zinc oxide nanoparticles loading onto cotton fabrics based textiles
TE D
194
Before being used, cotton fabrics were washed and dried. Experiments were performed
197
on samples with maximum dimension of 30 cm × 15 cm. Cotton fabrics were padded
198
with ZnO-NPs solution at certain safe concentration revealed from both MIC and in-vitro
199
cytotoxicity investigation. For the successive treatment of fabrics with colloidal zinc
200
oxide, the solution was agitated continuously. All samples were immersed in such colloid
201
bath for 5 min then squeezed to 100% wet pick up with laboratory pad at constant
202
pressure. Samples were dried at 80°C for 5 min, followed by curing at 150°C for 2 min.
203
The following treatments were conducted: (1) Control which A] Trypticasene soya broth
204
(TSB) without inoculation by bacterial culture (negative control) B] untreated fabrics
205
emerged in TSB inoculated by bacterial culture (positive control) C] untreated fabrics
AC C
EP
196
9
ACCEPTED MANUSCRIPT
206
emerged in TSB without inoculation (blank) (2) fabrics treated with zinc oxide
207
nanoparticles solution [19].
208
•
Scanning electron microscopy (SEM) for cotton fabrics
SEM was studied using a scanning electron –JSM-5400 instrument (Jeol, Japan). The
210
specimens in the form of fabrics were mounted on the specimen stabs and coated with
211
thin film of gold by the sputtering method.
RI PT
209
213
•
SC
212
Assessment of antimicrobial activity of nanoparticles treated fabric.
The antimicrobial behavior of fabrics was evaluated against Gram positive bacteria
215
represented by Staphylococcus aureus ATCC 6538, Bacillus subtilis ATCC 6633 and
216
Gram negative represented by Pseudomonas aeruginosa ATCC 9027 and Escherichia
217
coli ATCC 8739. Squares of 1 cm of each fabric were prepared in aseptic manner and
218
placed in 5 mL TSB inoculated by 100 µL of microbial suspension (adjusted optical
219
density for all bacterial culture at O.D. = 1 nm). The efficiency of the antimicrobial
220
treatment was determined by comparing the reduction in optical density (O.D.630 nm) of
221
the treated samples with that of positive control. Optical density is directly proportional
222
to the number of bacteria in the medium. The bacteriostatic activity was evaluated after
223
24 h and the percent reduction of bacteria was calculated using the following equation:
224
R (%) = [(A - B) / A] × 100
225
Where R= the reduction rate, A = the number of optical density for positive control, and
226
B = the numbers of optical density for treated fabrics.
AC C
EP
TE D
M AN U
214
227 228
•
Ultraviolet protection factor of fabrics
10
ACCEPTED MANUSCRIPT
The ability of treated and untreated fabric to block UV light is given by the ultraviolet
230
protection factor value (UPF). The UPF value was evaluated in the range of 280 – 400
231
nm with difference 10 nm by UV/Visible Spectrophotometer 3101 PC with a software
232
version.
RI PT
229
233 234
•
Statistical analysis: The means of three replications and standard error (SEr ±) were calculated for all the results obtained, and the data were subjected to
236
analysis of variance means by sigma plot 12.5 program.
SC
235
M AN U
237 238
3. Results and discussions
239
3.1.
240
The fungus isolate Aspergillus terreus AF-1 was identified by molecular methods
241
scheme 1. Fungal ITS fragment was identified from PCR and sequencing approaches
242
(Amplification and sequencing of ITS region have resulted in approximately 600 bp).
243
We constructed a maximum-likelihood phylogenetic tree to correlate our ITS
244
sequence with previously described sequences, the results showed that the sequenced
245
ITS fragment was related to the topology of Aspergillus terreus with a similarity of
246
98%.
AC C
EP
TE D
Identification of the isolate Aspergillus terreus AF-1
11
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
247 248
Scheme 1: Phylogenetic analysis of ITS sequences of the fungal strain with the
249
sequences from NCBI. Symbol ■ refers to ITS fragments retrieved from this
250
study. The analysis was conducted with MEGA 6 using neighbor-joining method.
252
TE D
251
3.2. Biosynthesis of ZnO NPs using A. terreus AF-1 Over the past few decades, the green bio-synthesis of metallic nanoparticles and their
254
oxides has been gained an importance suggested as possible alternatives to chemical and
255
physical methods. Proteins and enzymes secreted by fungi have effective role in the
256
reduction of ZnO to ZnO NPs, besides stabilizing these formed nanoparticles [20]. In this
257
context, A. terreus AF-1 was isolated and identified as aforementioned in scheme 1 and
258
then used as a bioreactor for green synthesis of ZnO NPs through harnessing bioactive
259
macromolecules such as proteins and enzymes secreted therefrom. Appearance of a
260
creamy-white precipitate after contacting of biomass filtrate with zinc acetate at the end
261
of reaction indicated the formation of hydrate ZnO (ZnO.H2O). After calcination of the
262
latter, ZnO-NPs were obtained as a white powder.
AC C
EP
253
12
ACCEPTED MANUSCRIPT
263 264
3.3.Factors affecting on the biosynthesis ZnO-NPs
265
Biosynthesis of ZnO-NPs were indicated by UV-visible spectroscopy as represented in
267
Figure 1.
RI PT
266
SC
0.8 0.6 0.4 0.2 0 350
370
269
M AN U
Absorbance
268
390 410 Wave length (nm)
430
450
Figure 1: UV-vis spectrophotometer of the biosynthesized ZnO-NPs and their optical
271
pictures picked during preparation process of: Zinc acetate solution (A), biomass
272
filtrate (B), and white precipitate formed upon addition of zinc acetate to biomass
273
filtrate (C).
EP
274
TE D
270
It was shown that the maximum absorption peak of the formed ZnO-NPs was occurred at
276
wavelength 390 nm, due to its surface plasmon resonance. These observation is in
277
agreement with the earlier studies on the biosynthesis of ZnO-NPs, which indicating that
278
the characterization peak of ZnO-NPs is lied around wavelength of 320-390nm [21].
279
Moreover, the absorption band in Figure 1 is slightly symmetrical with broad in width at
280
wavelength 390nm. These could refer to the formation of spherical ZnO with
281
polydispersed narrow sizes particles.
AC C
275
13
ACCEPTED MANUSCRIPT
Environmental conditions of the mixture of the fungal biomass filtrate and zinc
283
acetate have been the critical component directly affecting the productivity of ZnO-NPs
284
and also the process economics. The physical conditions of this mixture directly monitor
285
the rate of enzyme activity which reflects on the synthesis of ZnO-NPs. Therefore
286
optimization of physical parameters will not only support good growth but also enhance
287
the product yield. Hence, in seek of the optimization of the biosynthesized ZnO-NPs, the
288
UV-visible spectroscopy was used to determine the proper conditions applied during
289
preparation by examining the absorbance of the obtained ZnO-NPs suspensions at
290
wavelength 390 nm. Of these variables under investigation Zinc acetate concentration,
291
pH and incubation period of biomass filtrate with zinc acetate are shown below in Figure
292
2.
M AN U
SC
RI PT
282
AC C
EP
TE D
293
14
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
294
Figure 2: Factors affecting the biosynthesis of ZnO-NPs as a function of absorbance
296
at wavelength 390nm. A) Different zinc acetate concentration, B) Different pH
297
values and C) Different incubation periods
EP
298
TE D
295
Effect of zinc acetate concentration
300
Biosynthesis of ZnO-NPs with different concentrations of zinc acetate solution 0.5mM to
301
2.5mM was studied. Data represented in figure 2A showed that, by increasing the
302
concentration of zinc acetate, the absorbance at wavelength 390nm increases up to 2mM.
303
These evidences indicated the high efficiency of the bio-active molecules (proteins and
304
enzymes) comprised biomass filtrate on formation of ZnO-NPs at high concentration of
305
zinc acetate. Further increasing in the zinc acetate into 2.5mM, the bio-active molecules
AC C
299
15
ACCEPTED MANUSCRIPT
306
unable to protect the formed ZnO from agglomeration which leads to aggregate to bigger
307
sizes and hence, the absorbance decreased significantly [22].
308
Effect of different pH values
310
The effect of varying different pH values from 5 to 11 onto the biosynthesis of ZnO-NPs
311
by A. terreus AF-1 is shown also in Figure 2B, which showed the highest productivity at
312
maximum absorbance was occurred at alkaline pH-10. This could be attributed to the
313
behavior of the bio-active molecules secreted by A. terreus AF-1 in the solution which
314
acting as capping agent of ZnO-NPs is more stable and more reactive at alkaline medium
315
than acidic [23].
316
M AN U
SC
RI PT
309
Effect of incubation periods
318
The incubation period is a critical factor, which not only effect on the secretion of
319
bioactive molecules such as proteins and enzymes, but also effect on the reducing affinity
320
of ZnO to nanoparticles. Therefore, incubation period of the mixed biomass filtrate with
321
zinc acetate of concentration 2.0mM was performed at pH 10. Data illustrated in Figure
322
2C revealed that, the best time for extracellular biosynthesis of ZnO-NPs was obtained
323
when merely the biomass of A.terreus AF-1 has been mixed with zinc acetate for duration
324
of 2 days which the secretion of the bio-active molecules were yielded with highly
325
concentration in the biomass filtrate. After 2 days of incubation age, the bio-active
326
molecules may be, with the missing of the growth ingredients needed, the affinity of
327
fungus biomass to release more of those bio-active molecules was limited and/or most of
328
the secreted molecules tend to degrade or deactivate.
AC C
EP
TE D
317
16
ACCEPTED MANUSCRIPT
329 330
3.4.
Characterizations of ZnO-NPs
TEM measurement was carried out to determine the morphology and the
332
approximate size of the biosynthesized ZnO-NPs. Figure 3A revealed that, ZnO-NPs
333
with spherical shape were formed successfully using A.terreus AF-1 filtrate with well-
334
dispersed narrow sized particles surrounding with capping proteins and enzymes. The
335
average size of the formed ZnO-NPs is lied in the range of 10-45nm.
336
FT-IR analysis was performed to detect any chemical changes in functional groups.
337
Figure 3B is a typical FT-IR for biomass filtrate and ZnO-NPs. Results from biomass
338
filtrate spectra showed that, maximum absorption peak seen at near 1650cm-1 which is
339
related to (C=O) stretching vibration of peptide bonds and the peak near 3300 cm-1 is
340
thought to be N-H bending vibration. On the other side, the maximum spectrum peaks
341
picked from ZnO NPs spectra are seen at 3421, 2937, 2359, 1575, 1401, 1025, 940, 676
342
and 512 cm-1. Indeed, the peak at 512 cm-1 is the characteristic peak related to the
343
absorption of Zn-O bonds, while peak found at 1025cm-1 is corresponding to the C-O
344
stretching in amino acids. Maximum absorption peak at 3421 cm-1 may be attributed to
345
the characteristic absorption of OH- and NH- groups. Furthermore, the intensity of NH-
346
band occurred near 3300 cm-1 were decreased accompanied with shifting of (C=O) amide
347
absorption band to lower wavelength 1544cm-1. This obvious refers to the coordinating
348
bonds occurred between ZnO and proteins secreted fungi. From above results, it is clearly
349
evident that, the proteins secreted biomass filtrate from fungus A. terreus AF-1 have the
350
main role in size reduction of ZnO with narrow size distribution in well stabilized
351
nanoform.
AC C
EP
TE D
M AN U
SC
RI PT
331
17
ACCEPTED MANUSCRIPT
On the other hand, the crystalline nature of ZnO nanoparticles were confirmed by XRD
353
analysis (Figure 3C). XRD spectra showed well defined peaks at 2θ values 31.6°, 34.5°,
354
36.5°, 47.45°, 56.55°, 62.82°, 66.14°, 67.97° and 68.93° corresponding to (100), (002),
355
(101), (102), (110), (103) and (112) of ZnO-NPs, which revealing that the sample was
356
polycrystalline wurtzite structure (Zincite, JCPDS 5-0664).
357
On the other hand, the size and size distribution of ZnO nanoparticles in colloidal
358
solution were analyzed by the making use of DLS technique (Figure 3D). The results
359
represented in Figure 3D make it evident that, the particles obtained were polydispersed
360
mixture with average size of 175.85 nm (95.4%). Considering the presence of the capping
361
proteins and enzymes surrounding particles, the hydrodynamic radius obtained from DLS
362
does not give more information about the individual ZnO-NPs, however, it is considered
363
as a good to measure oval all dimension besides the width of nanoparticles and the
364
polymers which covering the particles. Whereas, the stability of colloidal solution which
365
depending on the surface charge of the formed nanoparticles was determined by zeta
366
potential analysis. In general, the particles keep away each other without any aggregates,
367
when the particles in a colloidal solution have large negative or positive zeta potential
368
values (greater than +30 mV or smaller than −30 mV) [24]. The biosynthesized ZnO-NPs
369
were highly stabled as have a zeta potential found to be -46.6 mV. This high value
370
confirms the high stability of colloidal solution.
371
Moreover, TGA of ZnO-NPs was shown in Figure 3E. The initial weight loss is assigned
372
to be 13.57% which due to water evaporation. The major weight loss occurred between
373
temperature 151 0C – 577 0C, which about 14.62% of the original weight. This weight
374
loss is attributed to the thermal decomposition of the organic compounds presented in the
AC C
EP
TE D
M AN U
SC
RI PT
352
18
ACCEPTED MANUSCRIPT
375
sample under investigation. Whereas, the remaining weight after 800 0C is related to ash
376
containing inorganic Zn. The close examination from the TGA results, it would reveal
377
that, ZnO-NPs were covered with 14.62% of proteins secreted fungi.
RI PT
378
380
AC C
EP
TE D
M AN U
SC
379
381
Figure 3. A) TEM image, B) FTIR spectra, C), XRD pattern, D) Particle size
382
distribution and E) TGA of ZnO-NPs synthesized by Aspergillus terreus AF-1.
383 19
ACCEPTED MANUSCRIPT
384
•
Antibacterial activity of ZnO-NPs.
The critical importance of ZnO-NPs being in their activity against abroad spectrum of
386
human pathogenic bacteria. Therefore, ZnO-NPs synthesized using A. terreus AF-1 were
387
investigated for their antibacterial activity against both Gram positive and Gram negative
388
bacteria. In general, the inhibitory action for biosynthesized ZnO-NPs which represented
389
by diameter of clear zone was more effective against Gram positive than Gram negative
390
bacteria. However, the diameter of clear zone formed due to 100 µL of ZnO-NPs (2000
391
µg/mL) was 20.2±0.2, 19.1±0.2, 14.2±0.2 and 14.1±0.2 for Bacillus subtilis,
392
Staphylococcus aureus, Escherichia coli and Pseudomonas aeruginosa, respectively
393
(Figure 4). The inhibitory action for biosynthesized ZnO-NPs may be due to reacting of
394
nanoparticles with bacterial protein by combining the thiol (-SH) groups, and hence leads
395
to inactivation of proteins and bacterial growth [25]. Gupta, et al., [26] explained the
396
mechanism of nanoparticles in bacterial growth reduction through interact with
397
phosphorous moieties in DNA, which lead to inactivation of DNA replication and hence
398
inhibition of enzymes functions. Whereas, Manke, et al., reported a new mechanism
399
which showing that nanoparticles are lead to changes in biological activities including
400
reactive oxygen species (ROS) thereby cause membrane damage leading too cell death
401
[27]. The exact mechanism of antimicrobial generated by NPs are not completely well
402
understood yet.
404
SC
M AN U
TE D
EP
AC C
403
RI PT
385
3.5.
Minimum Inhibitory Concentration (MIC)
405
The diameter of inhibition zone and its relation to the concentration of nanoparticles were
406
studied by Shaheen and Fouda [28] to confirm the antibacterial activity was dose 20
ACCEPTED MANUSCRIPT
dependent. Therefore, it is compulsory to detect the MIC to ZnO-NPs for each bacterial
408
strain. To this end, different concentrations of ZnO-NPs (1000, 500, 250 and 125 µg/mL)
409
were used. Regards to the data represented graphically in Figure 4, the obtained MIC for
410
Gram Positive Bacillus subtilis, Staphylococcus aureus was 250 µg/mL with clear zone
411
11.0±0.1mm and 10.5±0.2mm respectively. Whereas, the obtained MIC for Escherichia
412
coli and Pseudomonas aeruginosa was 500 µg/mL with inhibition zone 9.2±0.1mm and
413
9.3±0.3mm, respectively.
TE D
M AN U
SC
RI PT
407
EP
414
Figure 4. Antibacterial activity and MIC for ZnO-NPs at different concentrations (2000, 1000,
416
500, 250 and 125 µg/mL) against different human pathogenic bacteria
417 418
AC C
415
3.6.
In vitro cytotoxicity of ZnO-NPs
419
Cell morphology
420
Either variation in cell shape or cell morphology in culture is the first as well as the most
421
notably observation shown after exposure to nanoparticles or any toxic materials.
422
Therefore, the light inverted microscope could be used to monitor the cell shape and 21
ACCEPTED MANUSCRIPT
morphological changes dependent on ZnO-NPs exposure dose. The normal cell line
424
spread continuously on plate and showed epithelial characteristic morphology. The cell
425
exposed to different concentrations of ZnO-NPs gradually lost their phenotypic character.
426
As shown in Figure 5, at high concentration of ZnO-NPs, the cell become partial or
427
complete loss of monolayer, rounding, shrinking or cell granulation when compared to
428
untreated control cells. The light inverted microscope image proved, undoubtedly, that
429
the damage caused in cell morphology is ZnO-NPs dose dependent.
SC
RI PT
423
431
AC C
EP
TE D
M AN U
430
432
Figure 5. Light inverted micrographs proved morphological change for three type of cell
433
lines exposure to different concentration of ZnO-NPs. A) Clone-9 cell. B) Vero cell and
434
C) Caco-2 cell.
22
ACCEPTED MANUSCRIPT
435
MTT assay
437
Viability assays are basic stage in toxicology that explain the cellular response to a
438
toxicant. Also, they give information on the cell death, survival, and metabolic activities
439
[29]. MTT assay is sensitive colorimetric assays for the determination of the number of
440
viability in cell proliferation and cytotoxicity assays. Data represented in Figure 6
441
revealed that, cell mortality for normal and cancer cells were also dose dependent when
442
exposure to different concentrations of ZnO-NPs. Data showed that, the IC50 for normal
443
cell represented by clone-9 and vero cell were 26.85 µg/mL and 27.05 µg/mL,
444
respectively. Whilst, IC50 for cancer cell (Caco-2) was 79.57 µg/mL.
445
treatment of cotton fabrics with ZnO-NPs is highly recommended to be performed at
446
concentration lower than 26.85 µg/mL, in order to keep the process safe for human.
M AN U
SC
RI PT
436
AC C
EP
TE D
447
448
23
Thus, the
ACCEPTED MANUSCRIPT
449 450
Figure 6. Cell mortality for Clone-9 cell, Vero cell and Caco-2 cell at different
451
concentrations of ZnO-NPs synthesized by A. terreus AF-1.
RI PT
452 453 454
3.7.Application of the biosynthesized ZnO-NPs into cotton fabric.
Owing the unique properties of ZnO-NPs towards antibacterial activity and UV-
456
protection, the biosynthesized ZnO-NPs have been used in multifunctional textile fabrics.
457
In the context, ZnO-NPs were applied to cotton fabrics according to method mentioned in
458
our previous works [30]. ZnO-NPs were resuspended in distilled water to get final
459
concentration of 20 µg/mL (20ppm). Moreover, the deposition of ZnO-NPs on cotton
460
fabrics and their chemical composition were demonstrated by SEM-EDX instrument
461
(Figure 7A-D). The deposition of ZnO-NPs was clearly shown in the SEM image of the
462
treated cotton fabrics (Figure 7B), which indicates the homogenously distribution of
463
ZnO-NPs on the cotton fabrics surface whenever compared with control sample (Figure
464
7A) which seemed very smooth surface (Figure 7A). Furthermore, the chemical
465
compositions of the treated cotton fabrics were determined by Energy Dispersive X-ray
466
spectrometer (EDX) as showed in Figure 7C and D. The obtaining results showed that,
467
zinc element in zinc oxide nanoparticles occupied 2% of total number of elements found
468
in the tested sample as concluded from mapping image (Fig. 7C), whereas the weight
469
percent of the Zinc was about 1.03 % as calculated from EDX spectra (Fig. 7D).
AC C
EP
TE D
M AN U
SC
455
24
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
TE D
470
Figure 7. SEM image of: (A) untreated cotton fabrics with ZnO-NPs, (B) treated cotton
472
fabrics with ZnO-NPs, and (C) mapping picture of the surface of treated fabrics with
473
ZnO-NPs. (D) EDX of treated sample with elemental analysis of the ZnO-NPs contents.
475
3.8.Efficiency of the nano-zinc particles as antibacterial agent
AC C
474
EP
471
476
Cotton fabrics treated with nano-sized zinc colloids solution exhibit moderate
477
antibacterial efficiency against both Gram positive and negative bacteria. At 20ppm of
478
nano-zinc oxide colloid solution used for treatment, the reduction of bacterial growth was
479
82.2±0.3 % and 81.9±0.2 % for Staphylococcus aureus and Bacillus subtilis,
480
respectively. While bacterial reduction for gram negative bacteria represented by
25
ACCEPTED MANUSCRIPT
481
Pseudomonas aeruginosa and Escherichia coli were 74.8±0.5 % and 75.4±0.3 %,
482
respectively.
483
3.9.UV-protection of Cotton fabrics loaded by zinc oxide nanoparticles
RI PT
484
The absorption characteristic of the treated cotton fabrics with ZnO-NPs compared with
486
untreated fabrics, which expressed as UPF values and blocking percent for UVA and
487
UVB are represented in Table 1. It can be concluded that, the UPF value for treated
488
cotton fabrics was 16.1 which is a good protection index for the treated fabrics with ZnO-
489
NPs according to Australian/New Zealand Standard AS/NZS 4399:1996 [31], compared
490
with UPF value of 4 for untreated fabrics which consider a bad protection index [31]. UV
491
is the form of invisible radiation emitted from sun and classified into UVA (315-400nm)
492
and UVB (290-315nm) which damages collagen fibres and accelerates skin ageing but
493
UVB is more dangerous than UVA because it is directly destroy DNA and causes skin
494
cancer [32]. Therefore, data presented in Table 1 revealed that, ZnO-NPs loaded cotton
495
fabrics can be blocking UVA and UVB at 76.3% and 85.4%, respectively, when
496
compared to untreated fabrics which blocking at 66.9% and 79% respectively.
M AN U
TE D
EP
498
AC C
497
SC
485
26
ACCEPTED MANUSCRIPT
Table 1. UPF protection values of untreated and treated cotton fabrics with ZnO-NPs. Fabrics
UPF
protection Transmittance (%)
value
UVA
UVB
(315-400nm)
(290-315nm)
4
29.1
14
Treated
16.1
23.7
10.6
UVA
UVB
66.9
79
76.3
85.4
SC
Untreated
500
M AN U
501 502
Blocking (%)
RI PT
499
4. Conclusion
Although lots of chemical and physical methods were frequently used for the synthesis of
504
ZnO-NPs, but these methods possess several disadvantages through either toxic solvents
505
used or undesirable by-products yielded in addition to their high energy consumption.
506
Therefore, the main objectives of the current study were to produce ZnO-NPs by
507
microbial action and to apply these ZnO-NPs to fabricate the multifunctional medical
508
textile fabrics with the safe dose during application. To achieve these goals, the work
509
was designed to bring into synthesis of ZnO-NPs using biological method prolonging
510
with the investigation of their both antibacterial activity and in-vitro cytotoxicity prior
511
applying of ZnO-NPs into cotton fabrics for rendering them UV-protection and
512
antibacterial properties with safe dose. Therefore, the fungus Aspergillus terreus AF-1
513
was successfully used in extracellular biosynthesis of ZnO-NPs using fungus biomass
514
filtrate without addition of any hazardous materials, followed by optimization of the
515
biosynthesized ZnO-NPs and then characterized by UV-Visible spectroscopy,
516
transmission electron microscope (TEM) Fourier Transform-Infra Red (FT-IR)
AC C
EP
TE D
503
27
ACCEPTED MANUSCRIPT
spectroscopy, X-ray diffractometry (XRD) analysis and Dynamic light scattering analysis
518
(DLS). Results from UV-vis. Spectra revealed that ZnO-NPs were successfully
519
synthesized by dint of Aspergillus terreus AF-1 at optimum conditions include incubation
520
period of the biomass filtrate with (2.0mM) zinc acetate for 48h at pH 10. At these
521
conditions, an absorption peak was observed at maximum wavelength 390nm which
522
attributed to the SPR of ZnO-NPs. Further, TEM micrographs confirmed the formation of
523
well-dispersed spherical nanoparticles with an average size of 10-45nm. Furthermore, the
524
particle size analyzer revealed that ZnO-NPs were formed as a polydispersed mixture
525
with average size of 175.8nm, which could be due to presence of covering layer of
526
bioactive secreted molecules surrounding nanoparticles. Thus, the zeta potential was
527
raised to be -46.6 mV, indicating the high stability of the nanoparticles formed.
528
On the other hand, the antibacterial activity and in-vitro cytotoxicity of biosynthesized
529
ZnO-NPs were assessed. Results revealed that, ZnO-NPs have inhibitory action against
530
Gram positive ((Staphylococcus aureus and Bacillus subtilis) more than Gram negative
531
(Pseudomonas aeruginosa and Escherichia coli) bacteria with MIC 250 and 500 µg/mL,
532
respectively. However, ZnO-NPs showed morphological change and cytotoxic effect on
533
Clone-9, Vero and Caco-2 cell line at high concentrations. Below this concentration,
534
ZnO-NPs were loaded onto cotton fabrics to render them both antibacterial activity and
535
UV blocking properties for application in medical purposes. Our results confirmed that,
536
fabrics loaded with biosynthesized
537
bacterial growth of Staphylococcus aureus, Bacillus subtilis, Pseudomonas aeruginosa
538
and Escherichia coli with percent 82.2±0.3, 81.9±0.2, 74.8±0.5
539
respectively with UPF value 16.4 (good UV protection) compared to untreated fabrics.
AC C
EP
TE D
M AN U
SC
RI PT
517
ZnO-NPs had an ability to inhibit pathogenic
28
and 75.4±0.3 %,
ACCEPTED MANUSCRIPT
540 541
5. References
542
EP
TE D
M AN U
SC
RI PT
[1] Albrecht MA, Evans CW, Raston CL. Green chemistry and the health implications of nanoparticles. Green Chemistry. 2006;8:417-32. [2] Rehana D, Mahendiran D, Kumar RS, Rahiman AK. In vitro antioxidant and antidiabetic activities of zinc oxide nanoparticles synthesized using different plant extracts. Bioprocess and Biosystems Engineering. 2017;40:943-57. [3] Rao MD, Gautam P. Synthesis and characterization of ZnO nanoflowers using Chlamydomonas reinhardtii: A green approach. Environmental Progress & Sustainable Energy. 2016;35:1020-6. [4] Mohmed AA, Fouda A, Elgamal MS, Hassan SE-D, Shaheen TI, Salem SS. Enhancing of Cotton Fabric Antibacterial Properties by Silver Nanoparticles Synthesized by New Egyptian Strain Fusarium Keratoplasticum A1-3. Egyptian Journal of Chemistry. 2017;60:63-71. [5] Yuvakkumar R, Suresh J, Nathanael AJ, Sundrarajan M, Hong S. Novel green synthetic strategy to prepare ZnO nanocrystals using rambutan (Nephelium lappaceum L.) peel extract and its antibacterial applications. Materials Science and Engineering: C. 2014;41:17-27. [6] Rasmussen JW, Martinez E, Louka P, Wingett DG. Zinc oxide nanoparticles for selective destruction of tumor cells and potential for drug delivery applications. Expert opinion on drug delivery. 2010;7:1063-77. [7] Navale GR, Thripuranthaka M, Late DJ, Shinde SS. Antimicrobial activity of ZnO nanoparticles against pathogenic bacteria and fungi. JSM Nanotechnol Nanomed. 2015;3:1033-41. [8] Shaheen TI, El-Naggar ME, Abdelgawad AM, Hebeish A. Durable antibacterial and UV protections of in situ synthesized zinc oxide nanoparticles onto cotton fabrics. International journal of biological macromolecules. 2016;83:426-32. [9] Lobiak E, Shlyakhova E, Bulusheva L, Plyusnin P, Shubin YV, Okotrub A. Ni–Mo and Co–Mo alloy nanoparticles for catalytic chemical vapor deposition synthesis of carbon nanotubes. Journal of Alloys and Compounds. 2015;621:351-6. [10] Hasnidawani J, Azlina H, Norita H, Bonnia N, Ratim S, Ali E. Synthesis of ZnO nanostructures using sol-gel method. Procedia Chemistry. 2016;19:211-6. [11] Mănoiu V-S, Aloman A. Obtaining silver nanoparticles by sonochemical methods. UPB Sci Bull B. 2010;72:7. [12] Moghaddam AB, Nazari T, Badraghi J, Kazemzad M. Synthesis of ZnO nanoparticles and electrodeposition of polypyrrole/ZnO nanocomposite film. Int J Electrochem Sci. 2009;4:247-57. [13] Foudaa A, Saad E, Elgamala MS, Mohmedb AA, Salema SS. Optimal factors for biosynthesis of silver nanoparticles by Aspergillus sp. Al Azhar Bulletin of Science, Conf, March 2017. 2017;9th. [14] Singh D, Rathod V, Ninganagouda S, Hiremath J, Singh AK, Mathew J. Optimization and characterization of silver nanoparticle by endophytic fungi Penicillium sp. isolated from Curcuma longa (turmeric) and application studies against MDR E. coli and S. aureus. Bioinorganic chemistry and applications. 2014;2014. [15] Lynch I, Dawson KA, Linse S. Detecting cryptic epitopes created by nanoparticles. Sci Stke. 2006;2006:pe14-pe.
AC C
543 544 545 546 547 548 549 550 551 552 553 554 555 556 557 558 559 560 561 562 563 564 565 566 567 568 569 570 571 572 573 574 575 576 577 578 579 580 581 582
29
ACCEPTED MANUSCRIPT
EP
TE D
M AN U
SC
RI PT
[16] Fouda A, Khalil A, El-Sheikh H, Abdel-Rhaman E, Hashem A. Biodegradation and detoxification of bisphenol-A by filamentous fungi screened from nature. J Adv Biol Biotechnol. 2015;2:123-32. [17] Wang Y, Lu Z, Wu H, Lv F. Study on the antibiotic activity of microcapsule curcumin against foodborne pathogens. International journal of food microbiology. 2009;136:71-4. [18] Philip S, Kundu GC. Osteopontin Induces Nuclear Factor κB-mediated Promatrix Metalloproteinase-2 Activation through IκBα/IKK Signaling Pathways, and Curcumin (Diferulolylmethane) Down-regulates These Pathways. Journal of Biological Chemistry. 2003;278:14487-97. [19] Fouda A, Shaheen TI. Silver Nanoparticles: Biosynthesis, Characterization and Application on Cotton Fabrics. Microbiology Research Journal International. 2017;20:14. [20] Bhuyan T, Mishra K, Khanuja M, Prasad R, Varma A. Biosynthesis of zinc oxide nanoparticles from Azadirachta indica for antibacterial and photocatalytic applications. Materials Science in Semiconductor Processing. 2015;32:55-61. [21] Vennila S, Jesurani SS. Eco-friendly green synthesis and characterization of stable ZnO Nanoparticle using small Gooseberry fruits extracts. International Journal of ChemTech Research. 2017;10:5. [22] Rao CR, Trivedi D. Synthesis and characterization of fatty acids passivated silver nanoparticles—their interaction with PPy. Synthetic Metals. 2005;155:324-7. [23] Yedurkar S, Maurya C, Mahanwar P. Biosynthesis of zinc oxide manoparticles using Ixora coccinea leaf extract—A green approach. Open J Synth Theory Appl. 2016;5:1-14. [24] Meléndrez M, Cárdenas G, Arbiol J. Synthesis and characterization of gallium colloidal nanoparticles. Journal of colloid and interface science. 2010;346:279-87. [25] El-Rafie M, Mohamed A, Shaheen TI, Hebeish A. Antimicrobial effect of silver nanoparticles produced by fungal process on cotton fabrics. Carbohydrate polymers. 2010;80:779-82. [26] Gupta P, Bajpai M, Bajpai S. Investigation of antibacterial properties of silver nanoparticleloaded poly (acrylamide-co-itaconic acid)-grafted cotton fabric. Journal of Cotton Science. 2008. [27] Manke A, Wang L, Rojanasakul Y. Mechanisms of nanoparticle-induced oxidative stress and toxicity. BioMed research international. 2013;2013. [28] Shaheen TI, Fouda A. Green Approach for one-pot Synthesis of Silver Nanorod using Cellulose Nanocrystal and their Cytotoxicity and Antibacterial assessment. International Journal of Biological Macromolecules. 2017. [29] Popescu R, Heiss EH, Ferk F, Peschel A, Knasmueller S, Dirsch VM, et al. Ikarugamycin induces DNA damage, intracellular calcium increase, p38 MAP kinase activation and apoptosis in HL-60 human promyelocytic leukemia cells. Mutation Research/Fundamental and Molecular Mechanisms of Mutagenesis. 2011;709:60-6. [30] El-Rafie MH, Shaheen TI, Mohamed AA, Hebeish A. Bio-synthesis and applications of silver nanoparticles onto cotton fabrics. Carbohydrate polymers. 2012;90:915-20. [31] 4399 AN. Sun protective clothing - evaluation and classification. 1996. [32] Dubrovski PD. Wowen fabric and ultraviolet protection. Woven fabric engineering: InTech; 2010.
AC C
583 584 585 586 587 588 589 590 591 592 593 594 595 596 597 598 599 600 601 602 603 604 605 606 607 608 609 610 611 612 613 614 615 616 617 618 619 620 621 622 623 624
30
ACCEPTED MANUSCRIPT
Highlights Spherical narrow-sized ZnO-NPs were prepared using fungus Aspergillus terreus. Optimization of the biosynthesized ZnO-NPs was performed.
RI PT
Cytotoxicity dose of ZnO-NPs prior application was studied.
AC C
EP
TE D
M AN U
SC
Antibacterial activity and UV-protection of the treated cotton fabrics were investigated at safe ZnO-NPs dose.