1. Introduction
Silver nanoparticles (AgNPs) are widely used in commercial and medical applications, such as in products for disinfectants, water purification and band aids to improve wound healing, due to their antibacterial properties and characteristic features [
1]. AgNPs are particles with sizes between 1 nm and 100 nm that may possess different characteristics related to size, shape, and chemical composition [
2]. Nanoparticles of all types, including silver, may also be used to carry other particles for delivery into specific cells, such as in treatments for cancer [
3] or chronic lung diseases [
4]. The commercial use of AgNPs increases the risk that the particles are spread throughout the environment causing adverse health effects [
1]. Studies have shown that AgNPs may have harmful effects on various cell types [
2]. AgNPs have been shown to directly interact with the extracellular matrix (ECM) and improve its stability in general [
5]. In a previous in vitro study, long-term exposure of lung epithelial cells to AgNPs induced cytotoxicity, epithelial–mesenchymal transition (EMT) and increased collagen deposition [
6,
7], thus implicating a pro-fibrotic response by the AgNPs. Upon damages of the airway epithelial cell layer due to chronic lung disease or chronic exposure of inhaled particles, cells beneath the epithelial basement membrane will become exposed to nanoparticles, triggering an inflammatory response that may promote locally enhanced levels of pro-inflammatory cytokines. Fibroblasts are mesenchymal cells, crucial for maintaining homeostasis of ECM proteins, such as collagens and proteoglycans, components that together act as important reservoirs for cytokines and growth factors [
8,
9]. The ECM provides steady, elastic and durable walls of the alveoli, which are necessary for breathing efficiently and creating low resistance for gas exchange. Fibroblasts are also contributing in inflammation processes and respond to secreted growth factors, chemokines and cytokines, which stimulate a pro-fibrotic fibroblast phenotype that promotes tissue remodeling [
10]. Fibroblasts are involved in the chronic development of lung fibrosis in several severe lung diseases [
9,
11,
12]. However, studies on the effect of AgNPs in fibroblasts have primarily been performed during 24 h of particle exposure, where a cytotoxic effect was observed with smaller AgNPs [
13,
14]. In the present study, which is partly a follow up study to Gliga et al., [
6,
7], we have used AgNPs with different sizes (10 nm and 75 nm) and concentrations (2 μg/mL and 10 μg/mL) up to 72 h to study potential changes on cell viability, ECM synthesis and cytokine profile in human lung fibroblasts and in murine lung tissue slices ex vivo. Our obtained data indicate that AgNPs possess immunomodulatory and proinflammatory effects and are able to stimulate an increased synthesis of procollagen I in human lung fibroblasts. Importantly, AgNPs were also shown to have dose-dependent effects on cell viability observed both in vitro and ex vivo over time, findings that may be of relevance for future biomedical applications.
2. Materials and Methods
Human lung fibroblast cultures: Human fetal lung fibroblasts (HFL-1) (CCL-153, ATCC, Manassas, VA, USA) were cultured in Dulbecco’s modified Eagle medium (DMEM, Sigma Aldrich, St Louis, MO, USA) supplemented with 10% fetal clone serum (FCIII, Thermo Scientific, Waltham, MA, USA), 1% L-glutamine, 0.5% gentamicin and 5 μg/mL amphotericin B (all from Gibco BRL, Paisley, UK) at 37 °C, 10% CO2. HFL-1 was used in passage 16–21. DMEM supplemented with 0.4% FCIII serum was used throughout all experimental conditions to avoid interactions with factors in the serum.
Precision cut lung slices (PCLS): C57/Bl6 mice (female, >10 weeks) (Scanbur research A/S, Karlslunde, Denmark) were sacrificed with an i.p. injection of pentobarbital (0.3 mL of 60 mg/mL). Lungs were filled with pre-warmed low-melting agarose (Sigma Aldrich) solution (0.75% agarose) via a fixed positioned needle inserted into the trachea as previously described [
11]. After 10 min on ice, heart and lungs were removed and put in a tube with minimal essential medium (MEM) supplemented with amino acids (100×), vitamins (100×), sodium pyruvate 1% and glutamine (1%) and PEST (1%). Tubes were placed on ice to allow the agarose to further solidify. Cores of lung tissue were manually cut and then further sectioned into 300 µm thick lung slices using a Krumdieck tissue slicer (Alabama Research and Development, Munford, AL, USA). Slices were incubated at 37 °C, 5% CO
2 overnight, with repeated medium change during the first 4 h. Animal experiments were approved by the local ethics committee for animal research in Malmö/Lund, Sweden (Dnr M103/14).
Ag nanoparticles and characterization: AgNPs in two different sizes; 10 nm Citrate BioPure™ Silver and 75 nm Citrate BioPure™ Silver, were purchased from NanoComposix, Inc. (San Diego, CA, USA) in the form of stock dispersions (1 mg/mL) in aqueous 2 mM citrate. The AgNPs were previously evaluated for their primary size by transmission electron microscopy (TEM) and for their agglomeration in cell medium by photon cross correlation spectroscopy (PCCS) and ultraviolet-visible (UV-vis) spectroscopy. TEM imaging confirmed their primary size, and PCCS/UV-vis analysis showed agglomeration and sedimentation in cell medium over time [
6,
7,
15]. The AgNPs were negative for endotoxin contamination in the limulus amebocyte lysate (LAL) test [
15].
Stimulations with Ag nanoparticles: HFL-1 and PCLS were exposed to AgNPs with different sizes, 10 nm (Ag10) and 75 nm (Ag75), and concentrations 2 μg/mL and 10 μg/mL during 24 h, 48 h or 72 h. Prior to cell exposure, dispersions (1000× and 500× dilutions of Ag10 and Ag75) were prepared fresh in fully supplemented cell culture medium containing 0.4% FCIII. Cells and PCLS that were exposed to cell culture medium containing 0.4% FCIII without any AgNPs were regarded as the untreated controls for the experiments.
Analysis of cytotoxicity and metabolic activity: Cells were cultured in 24-well cell culture plates and exposed to AgNPs for 24 h or 48 h at 37 °C, 10% CO2. Cell medium was extracted and cytotoxicity was analyzed for Lactate Dehydrogenase (LDH) release with a LDH Activity Assay Kit (Roche, Cat. No. 11 644 739 001, Basel, Switzerland) according to the manufacturer’s instructions. Cells treated with 1% Triton-X100 were used as a positive control for cell death. Cell metabolism was measured by incubating the HFL-1 cells and PCLS with Tetrazolium salt (WST-1) (Roche, 11 644 807 001) with subsequent absorbance measurements in the collected cell medium, all according to the manufacturer’s instructions.
Quantification of cell amount: Cell amount was determined at 24 h and 48 h, as previously described [
10]. In short, HFL-1 cells were plated in 96-well culture plates (Cellstar, Monroe, NC, USA) for 6 h and then exposed to AgNPs for 24 h and 48 h. Cells were fixed in 1% glutaraldehyde (Sigma-Aldrich, St. Louis, MO, USA) for 30 min and stained with 0.1% crystal violet (Sigma-Aldrich, St. Louis, MO, USA) for 30 min. Excess staining solution was washed away and cells were permeabilized overnight with 1% Triton X100 at 4 °C (Merck, Darmstadt, Germany). Changes in cell amount were quantified with a spectrophotometer plate reader, measuring absorbance at 595 nm in collected cell suspension.
Transmission Electron microscopy: HFL-1 and PCLS exposed overnight to AgNPs were fixed in buffer containing 0.1 M Sorensen’s phosphate buffer pH 7.4, 1.5% formaldehyde and 1.5% glutaraldehyde at RT for 2 h for TEM. After fixation, the samples were washed twice in 0.1 M Sorensen’s phosphate buffer pH 7.4 before being dehydrated in a graded series of ethanol (50%, 70%, 80%, 90% and twice in 100%). Samples were critical point dried before being mounted and examined in a Jeol JSM-7800F FEG-SEM at Lund University Bioimaging Center (LBIC).
Analysis of proteoglycans and collagens: Proteoglycan production was determined as previously described [
10]. Briefly, HFL-1 were cultured in 6-well culture plates until confluency. Cells were incubated in low sulphate DMEM (Gibco BRL, Paisley, UK) and exposed to AgNPs or transforming growth factor (TGF-β1) Sigma Aldrich) 10 ng/mL (regarded as positive control) in
35S–containing DMEM supplemented with 0.4% FCIII, 1% glutamine and PEST 1% for 72 h. Proteoglycans in the cell supernatant were purified by ion exchanger DEAE52 and
35S-sulphate incorporation was quantified on a scintillation counter (Wallac; Perkin Ellmer, Boston, MA, USA). Total collagen synthesis was performed using the SircolTM Soluble Collagen assay kit (Biocolor, Carrickfergus, UK) by analyzing the total amount of collagen secreted in the cell supernatant, performed according to the manufacturer’s instructions. The collagen detection limit was 1 μg collagen. Procollagen I α1 synthesis was analyzed in the cell supernatant by ELISA (R&D Systems, Abingdon, UK), following the manufacturer’s instructions. The detection limit for procollagen I α1 was 15.6 pg/mL.
Analysis of growth factors and cytokines: Cell expression of the following interleukins (IL), chemokines and growth factors: IL-6, IL-8, (fibroblast growth factor (FGF-basic, also known as FGF-2), human growth factor (HGF), monokine induced by gamma (MIG), monocyte chemoattractant protein 1 (MCP-1), eotaxin, macrophage inflammatory protein (MIP)-1β, MIP-1α, β-nerve growth factor (NGF), regulated upon activation, normal T cell expressed and secreted (RANTES), platelet derived growth factor (PDGF)-BB and vascular endothelial growth factor (VEGF)-A were determined in cell supernatants collected 72 h post exposure. Analysis was performed with a multiplexed immunoassay on a Bio-Plex 200 Luminex instrument by mixing single-plex assays for the 13 above mentioned growth factors and cytokines (Bio-Rad, Hercules, CA, USA). Undiluted samples were analyzed and sample preparations were performed according to the manufacturer’s instructions. The baseline level of each cytokine measured in cell culture medium containing 0.4% FCIII serum (without any cells) was subtracted from the measured sample concentrations. The calibration curves were fitted using a five-point regression model and results were evaluated in the Bio-Plex Manager Software 6.0 (Bio-Rad). The limit of detection (LOD) for IL-6: 0.3 pg/mL, IL-8: 0.8 pg/mL, FGF-basic: 8.1 pg/mL, HGF: 6.7 pg/mL, MIG: 1.7 pg/mL, MCP-1: 0.7 pg/mL, eotaxin 0.1 pg/mL, MIP-1β: 0.07 pg/mL, MIP-1α: 0.1 pg/mL, β-NGF: 0.2 pg/mL, RANTES: 0.8 pg/mL, PDGF-BB: 2.6 pg/mL and VEGF: 20 pg/mL. Prostaglandin E2 (PGE2) synthesis was measured in the fibroblast medium by a commercially available enzyme immune assay (EIA) kit (Cayman Chemicals, Limhamn, Sweden). LOD for PGE2 was 7.8 pg/mL. All samples were normalized to individual protein amount.
Data presentation and statistical analysis: Data for HFL-1 are presented as mean +/− SEM with n = number of individually performed experiments. For PCLS, n = number of animals used in experiment. Changes in cell metabolism were expressed as % of control and analyzed with one-sample t-test. The non-parametric Wilcoxon test was used to compare statistical differences between two groups. Two-way repeated ANOVA measurement on ranks followed by the non-parametric post hoc test Dunn were used to compare differences in cell behavior in response to AgNP exposure. Differences were considered to be statistical significant at p < 0.05. All analyses were performed using the software program GraphPad Prism 7.0 (San Diego, CA, USA).
4. Discussion
In the current study, we evaluated the effect of AgNPs both on tissue level using murine PCLS and on cellular level using human lung fibroblasts. Our obtained data indicate that AgNPs affect cell viability in a concentration-dependent manner, detected both ex vivo and in vitro. Moreover, 10 μg/mL of either Ag10 or Ag75 significantly reduced metabolic activity after 48 h in both HFL-1 and PCLS. The PCLS technique is a well-known methodology for toxicity and pharmacological evaluations [
16,
17,
18,
19,
20]. The advantages of this technology are that the lung slices are viable for several days and have a maintained tissue integrity with intact pulmonary airways, vessels and surrounding lung parenchyma with alveoli, and it is a model system that in more detail mimics in vivo toxicity in comparison to standard cell culture conditions. From one murine lung, several sequential lung slices are obtained which enables inter- and intra-comparisons and significantly reduces the number of animals used in the experimental set up [
11,
19]. The effect of AgNPs on cell viability was further evaluated and confirmed in human cells, with increased cytotoxicity and reduced cell amount after 48 h in HFL-1. Several studies have investigated cytotoxic effects of AgNPs and showed that 24 h of exposure with smaller AgNP size (<10 nm) induced more cytotoxic effects than larger AgNPs seen in different cellular in vitro systems, such as human dermal and pulmonary fibroblasts [
21], human bronchial epithelial cells [
7], the human neural precursor cell line [
22] and human macrophage-like THP cells [
15], which are in line with our results. However, other studies could not identify any effects of AgNPs on cell viability in fibroblasts [
23], and only slight cytotoxic responses were induced in rat PCLS after 24 h of exposure to polyvinylpyrrolidone (PVP)-coated AgNPs (20–30 μg/mL) with a size of 70 nm [
24]. However, these AgNPs appeared to remain on the lung slice surface area [
24] in contrast to our study, where the AgNPs were localized within the slices, as visualized by TEM. These contradictory results could depend on several factors such as how AgNPs were produced, e.g., if or what type of particle coating was used, the size and concentration of the AgNPs and selected exposure times. However, few studies have investigated timepoints that extend 24 h of particle exposure and none have, to our knowledge, looked at the effect of longer AgNP exposure on lung tissue ex vivo. In this study, we evaluated the effects of AgNPs on cell viability after both 24 h and 48 h. Importantly, we could detect reduced metabolic activity both ex vivo and in vitro already after 24 h with 10 μg/mL of Ag10, but the effect was even more pronounced after 48 h. Similar effects were also obtained with 10 μg/mL of Ag75 after 48 h, indicating that the concentration and not the size of the AgNPs triggers to a greater extent the cellular response over time. Several studies points toward the notion that AgNPs and intracellular released Ag ions may affect cell viability through different routes, such as genotoxicity with DNA damages or mitochondrial disruption followed by induction of oxidative stress and reactive oxygen species (ROS) formation, which in turn induce cytotoxicity and cell apoptosis [
7,
25,
26,
27,
28]. In our study, TEM imaging of fibroblasts demonstrated that mitochondria in close proximity to AgNPs had structural changes that may indicate dysfunctional mitochondria, which could further explain and support our findings regarding the pronounced reduction in metabolic activity, as seen in AgNP-exposed HLF-1 and PCLS. However, further studies are warranted to follow up these observations.
AgNPs have also been shown to interact with the ECM [
5] and may stabilize the ECM structures in scaffold constructs [
29]. AgNPs are known to regulate collagen deposition, and AgNP composite nanofibers have been shown to increase collagen production during wound healing [
30,
31] and may thereby indirectly induce tissue remodeling. Larger AgNPs (>20 nm) actively bind to charged components in the ECM, whereas smaller particles may pass through the ECM network and induce more toxic responses [
5]. In a previous long-term study (6 weeks) in human bronchial epithelial cells, it was observed that AgNPs induced pro-fibrotic responses at both gene and protein level, such as increased collagen deposition and epithelial-mesenchymal transition [
6]. In the present study, we could not detect any major changes in ECM synthesis of either proteoglycans (except at 72 h exposure of Ag10, 2 µg/mL) or total amount of collagens by fibroblasts, which are vital components in ECM homeostasis [
8]. However, we analyzed the total amount of soluble proteoglycans and collagens which could be discriminated if changes were present on individual ECM proteins. When we analyzed the effect of AgNPs on one of the most important procollagens for collagen fibrillization, we could identify that the AgNPs induced an increased amount of procollagen I α1 in human lung fibroblasts after 72 h. The growth factor TGF-β1 which is known to induce powerful pro-fibrotic responses in fibroblasts [
11] also significantly increased procollagen I synthesis. Further studies of the ECM proteome with advanced mass spectrometry analysis are warranted to more closely follow potential interactions of AgNPs with individual ECM proteins. The ECM also provides storage for different growth factors and cytokines, where the interplay of AgNPs with the surrounding ECM may be actively involved in remodeling processes. In the present study, we did not show any major effects of AgNP exposure on the secretion of growth factors in lung fibroblasts. However, higher concentrations of both Ag75 and Ag10, reduced HGF levels and exposure for Ag75 showed strong tendencies toward increased PDGF-BB levels, whereas TGF-β1 significantly reduced both PDGF-bb, HGF, and FGF-basic. Collectively, these data indicate that AgNPs and TGF-β1 may induce pro-fibrotic responses through different signaling pathways in human lung fibroblasts.
We also investigated the effect of AgNPs on different cytokines secreted by the fibroblasts after 72 h of exposure. Others have shown that AgNPs may induce both pro- and anti-inflammatory responses in different in vitro systems, such as upregulation of IL-8 secretion by macrophage-like cells [
32] and by neutrophils [
33]. AgNPs may also interfere with toll-like receptor signaling in cellular innate immunity responses [
15]. We demonstrated that IL-8 and RANTES, which belong to the same cytokine family, were upregulated by Ag75 and to same extent by Ag10. RANTES, also known as CCL5, is chemotactic for leukocytes, such as T cells, eosinophils and basophils, whereas IL-8 is a well-known chemokine, attracting neutrophils to inflammatory sites. IL-8 may also promote angiogenesis [
5]. IL-8 is also reported to be upregulated during oxidative stress, linking to the reduced metabolic activity induced by 10 μg/mL of Ag10 and Ag75 in HFL-1 seen in this study. In the present study, 2 μg/mL of Ag75 reduced secretion of MCP-1, which is a chemoattractant for monocytes, and 2 μg/mL of Ag10 and Ag75 reduced secretion of IL-6. IL-6 is known as an important pro-inflammatory cytokine that recruits immune cells. IL-6 is also recognized as a myokine, important for repair processes in the tissue [
34].
In vivo studies on rats have shown that intratracheal installation of 75–150 µg of PVP-coated Ag50 caused a reversible inflammation, and that 300 µg caused DNA damage and neutrophilic granulocytes [
35]. Our findings imply that fibroblasts exposed by AgNPs become activated and recruit immune cells as a proinflammatory response. Of note, previous studies in dermal fibroblasts have shown that PDGF-BB, MCP-1, eotaxin and RANTES may increase type I collagen production [
36], findings that may explain the upregulation of procollagen I as a response to the enhanced release of PDGF-BB and RANTES observed in the present study. The proinflammatory enzyme cyclooxygenase 2 (COX-2) has been shown to be induced by dermal fibroblasts after 24 h of exposure to AgNPs (10 nm, 25 ppm) [
14]. To follow up these results, we examined the down-stream mediator PGE
2, which is generated via COX, and 10 μg/mL of Ag10 significantly induced PGE
2 secretion from the fibroblasts.
Although we observed toxic effects of AgNPs both ex vivo and in vitro, this study has some limitations. Our in vitro experiments were performed with a primary fetal cell line (HFL-1) and not using primary cells derived from healthy individuals. The promising results from this study showing a shift in cytokine profile warrants further investigation by co-culturing and investigating fibroblast interactions with inflammatory cells. In order to further increase clinical translatability, human lung slices can also be examined in addition to the murine PCLS, however, this was not feasible in this experimental set up.
In conclusion, our data indicate that immunomodulatory responses are induced by both sizes (Ag10 and Ag75) already at a relatively low dose (2 µg/mL) in human lung fibroblasts. AgNPs significantly affected cell viability both ex vivo in lung tissue slices and in vitro in HFL-1, with significantly reduced viability after 48 h of exposure to higher concentrations (10 μg/mL) of both Ag10 and Ag75. To translate our observed findings to the in vivo situation, previous studies have indicated that daily work exposure of AgNPs over a period of 74 working weeks would correspond to a total cellular deposition equal to the concentration of 10 μg/mL [
7]. The used concentrations in this experimental set up are quite high but within the range to be reached after exposure during an acute working accident or after many years of daily exposure. The ECM and cytokine profiles in human lung fibroblasts were clearly influenced by the exposure to AgNPs, promoting increased procollagen I synthesis and a proinflammatory cascade of cytokine release. Hence, careful characterization of AgNPs is of importance, including timepoints beyond 24 h for future applications in nanomaterials, and being aware of toxic effects as well as the ability to influence the ECM and the immune responses over time.