Introduction

Researchers have been investigating microbial infections induced by medical implants and surgical instruments, which could lead to serious health complications1,2,3,4. Gram-positive staphylococcus aureus is one of the most common strains of staphylococcus and it is a pathogen capable of causing life-threatening infections (e.g., soft tissue infections), eye infections, pneumonia, meningitis, or even necrotizing fasciitis, and food poisoning5,6,7,8,9,10. Previous studies have suggested that copper ion (Cu2+) can serve as an antimicrobial agent11,12. Many antimicrobial copper alloys have been approved for use in many areas such as mass transit, medical facilities and buildings in the U.S.13.

Combining the merits of both structural and functional materials, antibacterial stainless steel (SS) is a new class of implant materials with broad-spectrum and long-term antibacterial effects. The precipitation of the copper-rich phases on the surface of cu-bearing SS and the Cu2+ released from the surface endow this novel material with broad-spectrum antimicrobial activities14,15,16,17. Some researchers demonstrated that copper kills bacteria by damaging their cell walls and cell membranes11,18,19. Cu2+ possesses strong reduction ability, it can adsorb electrons from bacteria, leading to cell lysis and oxidization of cell nuclei20,21. The reactive oxygen species (ROS) such as superoxide anions were generated by the catalysis of copper, resulting in the fatal damage to important cell constituents and DNA. The exact mechanisms to explain how copper kills bacteria are still under investigation18,22.

Although bacteria may be in the viable but non-culturable (VBNC) state, they can maintain their pathogenicity, and may become infectious when the environment improves23. Previous works indicated that frozen at a low temperature or direct culture following exposure to Cu2+ could induce bacteria into the VBNC state24,25. To prevent missing VBNC cells in cell counting, the live/dead cell staining method was introduced for viability and morphological determinations in addition to cell enumeration using the quantitative polymerase chain reaction (qPCR) method26,27,28,29. The cytotoxicity of the new material was necessarily evaluated30.

The aim of this study was to characterize a potential implant material with a good antibacterial ability and excellent cytotoxicity. In this study, both antibacterial performance and the cytocompatibility of the 317L-Cu SS after antibacterial heat treatment were investigated. The concentration of Cu2+ released from the 317L-Cu SS was also assessed.

Materials and Methods

Bacterial strain, culture medium and SS coupons

The Guide for Chinese Animal Care and Use Committee standards was followed for the animal housing and surgical procedures. All procedures were done in accordance with protocols approved by the Animal Ethics Committee of Chongqing University. The ubiquitous pathogen S. aureus (ATCC 25923) was used in this study. It was routinely subcultured and maintained at 37 °C in the Luria–Bertani (LB) medium (Booute Biotechnology Ltd., Wuhan, Hubei, China) before use. The MC3T3-E1 cell was cultured at 37 °C in the α-minimal essential medium (α-MEM) containing 10% (v/v) fetal bovine serum (Sigma-Aldrich Inc., St. Louis, MO, USA), 50 μg ml−1 gentamicin (Gen-view Scientific Inc., Galveston, TX, USA), 50 μg ml−1 ascorbic acid (Sigma-Aldrich Inc., St. Louis, MO, USA) and 2.5 μg ml−1 fungizone (Gen-view Scientific Inc., Galveston, TX, USA) in a Heracell 150i thermostatic incubator (Thermo Fisher Scientific Inc., Waltham, MA, US) containing 5% (v/v) CO2. The SS alloys used in this study included 317L-Cu SS (composition in Table 1) and commercial medical grade 317L SS (control). The 317L-Cu SS sample was heat treated under the following conditions: a solution treatment at 1100 °C for 0.5 h to distribute Cu evenly in the SS followed by water quenching, and then aging at 700 °C for 6 h in order to obtain the Cu-rich phases in the alloys31. The 317L SS control sample was treated in the same fashion. The heat treated alloys were machined to coin-shaped coupons for testing with a 10 mm diameter and a 1.5 mm thickness. Each coupon was degreased and cleaned by vortexing for 30 s in 10 ml acetone32.

Table 1 Chemical composition of 317L- Cu SS (wt%).

Atomic Absorption Spectroscopy (AAS)

The release of Cu2+ of 317L-Cu SS into a 0.9% (w/v) NaCl solution was measured using an atomic absorption spectrophotometer (Model, Z-2000; Hitachi Ltd., Tokyo, Japan). The detection wavelength and integration time for Cu2+ was 324.8 nm and 5 s, respectively. Five coupons were tested for each time point.

The preparation for antibacterial test

Both 317L and 317L-Cu coupons were placed in a 24-multiwell culture plate. One ml S. aureus suspension with a concentration of 106 CFU ml−1 was deposited into each well containing a coupon. The inoculated plate was incubated in a DNP 9272 incubator (Jinghong Corporation, Shanghai, China) at 37 °C for different periods (0.5 d, 1 d, 3 d and 5 d). All the antibacterial tests were performed under the relative humidity of 90% at 37 °C.

Plate count method

At the end of each test time period, bacterial suspensions from the 24-well plates were diluted to approximately 103 CFU ml−1, and 0.1 ml of the diluted bacterial suspension was streaked on an agar plate (Aoboxing Bio-tech Corporation, Beijing, China). The plates were then incubated at 37 °C for 1 d before counting the bacterial colonies20,33. The antibacterial rate C was calculated based on the following equation:

where A is number of CFUs for 317L SS and B for 317L-Cu SS34,35,36.

Live/dead staining

To elucidate the antibacterial efficacy of 317L-Cu, S. aureus cells after incubation with 317L and 317L-Cu SS coupons were stained with the Live/Dead BacLightTM kit (SYTO9 and propidium iodide (PI); Thermo Fisher Scientific Inc., Waltham, MA, USA). After incubation, a mixture of 10 μmol l−1 SYTO9 and 60 μmol l−1 PI was added to each well. To allow the diffusion of fluorochromes in the biofilm, the specimens were kept stationary in the absence of light at 37 °C for 20 min37. Then, the specimens were incubated for 30 min at room temperature in the dark. After gentle cleaning using 0.9% (w/v) NaCl followed by phosphate buffered saline (PBS) at pH 7.4, the coupons were retrieved for examination under confocal laser scanning microscopy (CLSM, Model C2si+; Nikon Ltd., Tokyo, Japan) equipped with a 40× objective lens with filters appropriate for SYTO9 and PI. Each coupon was mounted on a glass slab for CLSM imaging. The biofilm thickness was obtained using the 3-D scanning mode. The confluent areas with biofilm were randomly measured and 10 views for each sample were recorded for reporting38. All the biofilm thickness data were analyzed with the Nis-Elements Viewer version 4.20 software (Nikon Ltd., Tokyo, Japan)21. The number of sessile cells was quantified from the average of 10 sets of CLSM images using the ImageJ software (National Institutes of Health, Bethesda, MD, USA)39.

DNA extraction and qPCR

Sterile coupons of both 317L SS and 317L-Cu SS were inoculated with 1 ml S. aureus suspension (106 CFU ml−1). After incubation, bacterial suspensions were transferred to 5 ml sterile disposable centrifuge tubes with the DNase I (Takara Bio Inc., Dalian, Liaoning, China) treatment40,41,42. To collect the sessile cells, the coupons were transferred to 15 ml sterile disposable centrifuge tubes containing 10 ml sterile 0.9% NaCl with 20 mmol l−1 EDTA (to chelate free Cu2+) with 2-mm diameter glass beads and vortexed for 30 s. After that, both planktonic and sessile cells were mixed and pelleted by centrifugation. DNA from the pelleted cells was isolated and purified using the Takara Minibest Bacterial Genomic DNA Extraction kit (Version 3.0; Takara Bio Inc., Dalian, Liaoning, China) following the instructions for gram-positive bacteria. The purified DNA was stored at 4 °C before use.

The gene copy numbers of samples were quantified with the qPCR analysis using SYBR® Premix Ex TaqTM (Takara Bio Inc., Dalian, Liaoning, China) following the manufacturer’s instructions43,44. The qPCR to quantify S. aureus was performed with the primers nuc-F (5′ CCT GAA GCA AGT GCA TTT ACG A 3′) and nuc-R (5′ CTT TAG CCA AGC CTT GAC GAA CT 3′) targeted heat-stable nuclease45. The results were analyzed using the 2−ΔΔCT method46.

Transmission electron microscopy (TEM)

The S. aureus sessile cell membrane damage due to the biocidal action of 317L-Cu SS was investigated using TEM (Model H-7650; Hitachi Ltd., Tokyo, Japan) with an accelerating voltage of 80 kV. After incubation, the sessile cells were washed off from coupon surfaces with deionized water followed by 15 s of ultrasonication. The sessile cells were collected after centrifugation (6000 g, 5 min at 4 °C). The supernatant was discarded and deionized water was added to resuspend the sessile cells. Then the cells were fixed using osmic acid, dehydrated and placed on a copper grid for TEM observation.

Scanning electron microscopy (SEM)

The surface morphologies of biofilms on 317L SS and 317L-Cu SS coupons were observed under SEM (Model S-3400N; CARL ZEISS Ltd., Oberkochen, BW, Germany) at operating voltage of 20 kV. After incubation, coupons were retrieved and washed three times using 3 ml 0.9% NaCl before being fixed with 2.5% (v/v) glutaraldehyde. Coupons were dehydrated with a graded ethanol series of 50%, 75%, 95% and 100% (v/v)47. The coupons were sputter coated with gold using the JFC-1200 Fine Coater (Jeal Corporation, Tokyo, Japan) before SEM imaging48.

RTCA cytotoxicity assay

Each well was seeded with osteoblast-like 1,000 MC3T3-E1 mouse cells on a 96-well electronic plate (E-Plate View 96; ACEA Biosciences Inc., San Diego, CA, USA)49,50,51. The E-plate was read using the xCELLigence DP system (ACEA Biosciences Inc., San Diego, CA, USA) at 5-min intervals. The value of cellular index (CI) represents the morphological changes and the number of cells which can reflect negative effects on cellular functions. After 20 h of RTCA profiling, the assay was paused, and the plate was removed from the xCELLigence system. The liquid in each well was decanted and replaced with a 0.9% NaCl solution labeled as soaking solution that was exposed to 317L or 317L-Cu for a fixed time period (1 d, 3 d, or 5 d). The plate was monitored for 120 h. For each sample, there were two duplicates. Results were collected using the RTCA software (Version 2.0; ACEA Biosciences Inc., San Diego, CA, USA). The data expressed in CI units were exported to Microsoft Excel software (Microsoft Office Professional Plus 2010; Microsoft, Redmond, WA, USA) for mathematical analysis. The data were normalized to a starting CI of 1.0 at the time point immediately prior to the solution switch and addition of dices52.

Cell morphological analysis

After 140 h of RTCA monitoring, the assay was terminated. A visual assessment of each treatment group was made, and photomicrographs were captured using a digital camera (Digital Sight DS-U3; Nikon Ltd., Tokyo, Japan).

Statistical analysis

Statistical analysis was performed with SPSS 17.0 software. The transition of the number of bacteria between each coupon (by plate count, fluorescence staining and qPCR) and RTCA assay (by NCI) were analyzed by analysis of variance (ANOVA).

Results

Copper ion release curve over time

The Cu2+ released from 317L-Cu SS into the 0.9% NaCl solution was determined using AAS. Figure 1 shows an increased concentration over time with a metal surface area to solution volume ratio of 78.5 m2 m−3. The daily release of Cu2+ from the 317L-Cu matrix was less than 20 ppb cm−2. This low level would not pose any immediate danger to human health53,54.

Figure 1
figure 1

Cu2+ release in 0.9% NaCl by 317L-Cu SS over time.

Antibacterial efficacy of 317L-Cu SS

Figure 2 indicates that the antibacterial rate of 317L-Cu SS reached up to 98.3% when the incubation time reached 1 d, which was consistent with the previously reported results33. The evaluation is considered as an effectively, widely used method. However, as mentioned, the results of this experiment can only determine that the 317L-Cu SS may inhibit the bacterial growth. Obviously, simply using the plate count method cannot guarantee the safety of a potential implant material. Figure 3 presents the plate cultures seeded with the cell suspensions obtained after S. aureus was incubated with the 317L SS and 317L-Cu SS coupons for 0.5 d and 1 d. It was found that after incubation with 317L-Cu SS for 1 d, no cells were detectable on nutrient agar plates. The 3 d and 5 d results (not shown) were identical to Fig. 3d, which confirmed that the good antibacterial performance of 317L-Cu SS showed after 1 d in 0.9% NaCl solution.

Figure 2
figure 2

The antibacterial efficacy of 317L-Cu SS against S. aureus after incubation at 37 °C for 0.5 d, 1 d, 3 d and 5 d.

Figure 3
figure 3

S. aureus colonies on agar plates inoculated with cell suspensions obtained from S. aureus liquid cultures exposed to 317L SS (a,b) and 317L-Cu SS (c,d) for 0.5 d (a,c) and 1 d (b,d), respectively.

The inhibition of S. aureus biofilm by 317L-Cu SS

Figure 4 shows the epifluorescent images obtained by CLSM showing viable (live) cells with integral membranes as green dots and non-viable (dead) cells with disrupted membranes as red dots. Viable cells were observed in the left column of each row while non-viable cells were observed in the middle column of each row. Viable and non-viable cells were observed simultaneously in 3D mode with the biofilm thickness of each coupon in the right column. In the initial 3 d, there were seldom dead cells on the 317L SS coupon surface, while more dead cells appeared on the 317L-Cu coupon surface after 1 d, indicating the satisfactory biocidal effect of 317L-Cu SS. For 317L-Cu SS, the proportion of non-viable cells increased significantly after 1 d, which corresponded to the Cu2+ release curve in Fig. 1. The result of Fig. 5 also supports that conclusion. The presence of non-viable cells on 317L SS was observed after 5 d, which might be caused by the normal cell death. Compared with 317L SS, the total number of viable and non-viable cells was obviously less on the 317L-Cu coupon surface, demonstrating that with the continuous released of Cu2+, the 317-L Cu possessed a satisfactory biocidal ability. The biofilm thickness values of S. aureus on 317L and 317L-Cu SS surfaces Fig. 6, show significant differences between 317L SS and 317L-Cu SS in each time point (P < 0.05).

Figure 4: CLSM images of the S. aureus biofilm on 317L SS after 0.5 d (a1–a3), 1 d (b1–b3), 3 d (c1–c3) and 5 d (d1–d3) of incubation, and on 317L-Cu SS after 0.5 d (e1–e3), 1 d (f1–f3), 3 d (g1–g3) and 5 d (h1–h3) of incubation.
figure 4

(Left column for stained live cells only, middle column stained dead cells only and the right column for both). (Scale bar = 50 μm).

Figure 5
figure 5

The number of viable bacterial cells stained with SYTO9 vs. time.

Figure 6
figure 6

S. aureus biofilm thickness on a coupon vs. time.

qPCR to quantify the antibacterial efficacy of 317L-Cu SS

The VBNC state can be summarized as a stationary state of microbial life, waiting for a suitable growth environment55. The plate counting method could not distinguish between dead cells and cells in the VBNC state. To verify that cells were killed by 317L-Cu SS rather than in the VBNC state, qPCR was used to evaluate the antibacterial efficacy of 317L-Cu.

Figure 7a shows there were no orders of magnitude difference in viable cells recovered from 317L and 317L-Cu samples before 1 d. In conjunction with Fig. 1, the Cu2+ concentration was 9.25 ppb, probably insufficient to kill the sessile cells. Unlike pure copper, 317L-Cu took 3 d to release adequate Cu2+ to kill the sessile cells21,32. To visualize the data in Fig. 7a better, Fig. 7b was obtained by using the gene copy number before incubation as the basis. As seen in Fig. 7b, the reductions of genomic units (GU) by 2 orders of magnitude after 3 d and 5 d incubation with 317L-Cu SS were achieved. The trend in Fig. 7a is consistent with the results of Live/dead staining analysis shown in Fig. 5. In conjunction with the rationale behind Live/Dead staining and qPCR56,57, it was concluded that the Cu2+ not only led to cell membrane disruption but also gene reduction, confirming the biocidal efficacy of 317L-Cu SS.

Figure 7
figure 7

Calculated ratio of gene copy numbers on each coupon (mean values and standard deviations based on triplicate assays within a single qPCR setup): (a) The viable cells recovered and (b) bar chart version of (a) using the gene copy number before incubation as basis.

TEM and SEM to reveal the cell death process

The S. aureus ultrastructure influenced by 317L-Cu SS was assessed by TEM (Fig. 8). The healthy cells were shaped with the unaltered cell structure with the inner and the intact outer curved membrane. The consistent appearance observed in the control group (incubated with 317L SS) shows that S. aureus cells remained undamaged even after 5 d (Fig. 8a)58. When incubated with 317L-Cu SS, partial and complete destructions of cell membranes after 1 d were observed (Fig. 8b,c). These TEM images visually supported the 317L-Cu SS antibacterial ability against S. aureus by destroying its membrane.

Figure 8
figure 8

TEM images showing the deformation process of S. aureus: (a) well defined cells incubated with 317L-Cu SS after 0.5 d, (b) beginning of cell lysis of a cell incubated with 317L-Cu SS after 1 d, and (c) whole cell disintegration incubated with 317L-Cu SS after 3 d. (Scale bar = 0.5 μm).

The surfaces of the 317L and 317L-Cu coupons were also investigated using SEM. Figure 9(a1–a3) shows that after 1 d, 2 d and 3 d, there were no big differences of biofilm coverage on 317L. However, for 317L-Cu, the sessile cell coverage decreased after 3 d compared with 1 d. After 5 d, the sessile cells were much less. This trend was similar to that observed on Cu-bearing CoCrWNi alloys36. The cell integrity found on the 317L-Cu surface (Fig. 9c1–c2) was significantly damaged. This is consistent with the TEM result, indicating a satisfactory biocidal effect of the 317L-Cu SS.

Figure 9
figure 9

SEM images of S. aureus cells on coupons: (a1–a3) 317L SS after 1 d, 3 d and 5 d (scale bar = 1 μm), (b1–b3) 317L-Cu SS after 1 d, 3 d and 5 d (scale bar = 2 μm), and (c1–c2) observation of cell ultrastructure injury at 10000 × amplification for cells on 317L-Cu SS after 3 d (scale bar = 1 μm).

The cytotoxicity of 317L-Cu with mouse cells

RTCA was carried out to compare 317L SS with 317L-Cu SS for their cytotoxicity to MC3T3-E1 mouse cells. A small cell concentration was required to prevent the quick exhaustion of nutrients prematurely. Therefore, based on the preliminary results, 1000 cells per well were seeded in each well on the E-Plate View 96, and the impedance was monitored every 5 min for 141 h. The characteristic RTCA growth profiles of MC3T3-E1 exposed to soaking solutions and SS dice are shown in Fig. 10. The morphological assessment under different treatments was shown in Fig. 11(a–c). At the end of the experiment, MC3T3-E1 grew healthily and there were no significant differences among the three groups59. Initially, the presence of the healthy cells led to an increase in the electrode impedance and the normalized cell index (NCI). When a soaking solution containing 317L and 317L-Cu dices was introduced, the cells might have a change in morphology, and could detach from the electrodes resulting in a change in NCI. In Fig. 10, both soaking solutions and dices did not lead to cell death (CI > 1) after 5 d. Figure 11 reveals a cell growth behavior which proliferated to form a full layer on the E-Plate View 96. No apoptosis cells were observed. The results here suggest that both types of SS did not introduce cytotoxicity to the mouse cells.

Figure 10
figure 10

RTCA profiling of the soaking solution for mouse MC3T3-E1 cells with 1,000 MC3T3-E1 cells per well in α-MEM.

Figure 11
figure 11

Representative photomicrographs of 24-well plates corresponding to 140 h in Fig. 10.

Discussion

The JIS Z2801:2000 industrial standard based on plate count method was used to evaluate the antibacterial properties of antibacterial materials60. The defined antibacterial rate of 317L-Cu could reach up to 98.3% when the incubation time reached 1 d. Furthermore, based on the plate count method, the antibacterial rate was 99.99% at 3 d and 5 d, because there was no colony for the sample incubated with 317L-Cu after 3 d and 5 d. However, 317L-Cu SS was unable to kill the bacteria completely at 3 d and 5 d as indicated by qPCR. It was likely that the plate count approach was affected by the VBNC state of bacteria.

In order to obtain reliable results, live/dead staining have gained increased popularity among researchers in various fields of microbiology29,61. Researchers have used the JIS Z2801:2000 industrial standard in testing growth inhibition of bacteria, live/dead staining was used to determine the bactericidal effect62,63. In this procedure, live/dead staining depends on cytomembrane permeability to differentiate live and dead bacteria based on the assumption that the degradation of cellular DNA is incomplete37,64. Figure 5 shows that there was a 1–2 log reduction in viable cells after 5-d incubation with 317L-Cu SS and there was a significant difference (P < 0.05) between 317L-Cu SS and 317L SS, which was in agreement with previous reports that the cell membranes were the primary targets of contact killing through surface-released Cu2+11. Unfortunately, all staining procedures affect the structural integrity of the bacterial cells considerably65. Ethidium monoazide-quantitative PCR (EMA-qPCR) applies the same principles. It was found to be a poor indicator of cell viability, mainly because high concentrations of the dye can penetrate viable cells66. The qPCR with a prior DNase/PK treatment has been shown to be more practical in comparison with the PMA treatment42. It was able to eliminate the DNA from dead cells to obtain Fig. 7, which clearly proved the antibacterial efficacy of 317L-Cu SS. As mentioned above in the Fig. 3c discussion, there were no colony counts detectable on plates over 1 d. Combined with the analysis of qPCR, it was likely that most cells entered the VBNC state. However after 3 d and 5 d, Fig. 7 shows most bacterial cells were eradicated by the 317L-Cu SS60.

Researchers can directly observe cellular structures on solid surface after incubation using TEM and SEM67,68,69. To further investigate the mechanism of inhibition of Cu2+ on microorganisms, S. aureus was incubated with 317L-Cu SS and studied using TEM and SEM. Figures 8 and 9 clearly show that morphological changes in the injury and death of S. aureus cells after intubation with 317L-Cu SS.

Copper is an essential element but it is cytotoxic at elevated concentrations19. Based on the development of advanced sensor detection technology and cell culture technology, RTCA has been developed for in vitro cytotoxicity tests with reliable data outcome70,71. Here, E-plate was used because it was ideal for simultaneous visual and real-time analysis since these plates provided a viewing window for graphical analysis and electrochemical cytotoxicity test52. Compared with surface modification methods of implants, 317L-Cu SS can be regarded as an approach from the material aspect, which required no addition of the other antibacterial substances72,73. Not only 317L-Cu SS has long-lasting antibacterial effect, but also avoids the failure caused by surface wear or low adhesive force of coating74,75.

The preliminary study for a new type of antimicrobial metal was performed to observe its antibacterial performance, to investigate its antibacterial mechanism and to evaluate its biocompatibility. RTCA has been proved to have the characteristics of high sensitivity, high speed responsibility, real-time dynamic monitoring, label-free analysis76,77. Compared with conventional cell survival assay, RTCA can obtain more comprehensive and reliable data78. Unlike these cited studies, 5 d instead of 1 d was adopted as the incubation time to acquire the preliminary analysis of 317L-Cu cumulative toxicity. The results of three antimicrobial assessments and RTCA confirmed that 317L-Cu SS possessed a satisfactory antibacterial ability against S. aureus after 1 d. SEM and TEM images provided visual confirmations. Although the antimicrobial mechanism of Cu2+ is not fully established in the literature, this work provided additional evidence that Cu2+ led to cell membranes breakage and subsequent cell lysis. 317L-Cu SS possesses strong potential in medical applications to provide a metal surface that is easier to maintain a sanitary surface without antibacterial coatings or biocides. It is potentially a new biocompatible implant material with a good balance of long-term antibacterial ability and mechanical properties.

Additional Information

How to cite this article: Sun, D. et al. An investigation of the antibacterial ability and cytotoxicity of a novel cu-bearing 317L stainless steel. Sci. Rep. 6, 29244; doi: 10.1038/srep29244 (2016).