Introduction

The localized surface plasmon resonance (LSPR) is a spectroscopic phenomenon based on the resonant oscillations of free electrons of various materials including noble metal nanoparticles, Al nanoparticles, conventional semiconductors and 2D materials, when stimulated by incident light1,2,3. Except the size, shape4, 5 and composition of nanoparticles, the frequency and intensity of the LSPR bands are sensitive to the interparticle spacingno and dielectric environment6, 7. Therefore, the response of plasmonic nanoparticles to the refractive index variation of surrounding medium is employed to develop LSPR sensors in broad fields of biology, food, and environment8,9,10,11. However, due to the low detection sensitivity and capacity7, 12, 13 and poor stability, the development of LSPR sensors is limited, especially in practical applications. For example, numerous efforts have been devoted to develop various methods for the detection of E. coli O157:H7, which is a gram-negative enteric bacteria, causing severe intestinal infections in humans14, 15. Traditional methods 16,17,18 such as electrochemical methods and lateral-flow immunochromatography for detecting E. coli O157:H7 are always time-consuming and the sensitivity is not very high19,20,21 and limits their practical use as a commercial product. The objective of the present study is to develop a high performance LSPR sensor for practical application in real sample analysis (E. coli O157:H7) that would achieve high sensitivity and stability.

In recent years, some strategies were suggested to improve the sensitivity and stability of LSPR sensors such as morphology optimization of nanoparticles, surface functionalization and single nanoparticle detection22, 23. Meanwhile, surface functionalization served as a powerful means not only to effectively improve sensitivity and stability of LSPR sensors but also flexibly modify plasmonic nanoparticles with desired functions for further applications24. For example, polymer or biomolecules coated Au nanoparticles LSPR sensors show higher selectivity and stability25.

Homogeneous mesoporous silica has been proven to be a versatile biomaterial to directly improve stability of nanoparticles in complex bio-system, due to its excellent biocompatibility. On the other hand, mesoporous structure26,27,28 provides large-area and easy-decorated surface for maximally capturing the target molecules to improve the sensitivity of LSPR. Since the encapsulated SiO2 determines the refractive index of surrounding environment, the thickness of SiO2 attributed to a vital parameter to affect LSPR sensitivity. However, there is a controversial point about the effect of thickness of SiO2 shell on LSPR sensitivity. For instance, Xu and co-workers synthesize 8 nm mesoporous silica shell coated Au NRs to improve the sensitivity to 325 nm/RIU22. Wang and co-workers used 21 nm silica coated Au NRs to amplify the sensitivity for detecting biomolecules29. Moreover, Huang and co-workers considered that a 2–3 nm silica shell coated on Au NRs induces a highest sensitivity for plasmonic organic photovoltaic devices30. The recent theoretical calculation reveals that ultrathin silica coating (within 3.5 nm) would be ideal for improving the sensitivity31. Therefore, the aim of our present work is to explore the cut-off thickness in a small size, and further amplify the sensitivity of Au NRs maximally for practical application for detection of E. coli O157:H7.

Herein, a series of Au nanorods (Au NRs) with different mesoporous silica shell are synthesized to study the effects of silica shell thickness on the sensitivity of Au NRs LSPR symmetrically. The as-prepared Au NRs@SiO2 with optimal shell thickness showed high sensitivity and used as efficient LSPR biosensor to detect E. coli O157:H7. Au NRs with elongated geometry were selected as plamonic nanoparticles for LSPR sensor due to their tunable and broad spectra range from the visible to near-infrared region24, 32, 33. The thickness of SiO2 on AuNRs was optimized by adjusting the concentration of Cetyltrimethyl Ammonium Bromide (CTAB) and the amount of tetraethyl orthosilicate (TEOS), achieving sensitive Au NRs@SiO2. To verify the performance of Au NRs@SiO2 as LSPR sensors, Au NRs@SiO2 with optimal thickness was modified with specific antibody to selectively detect E. coli O157:H7 in high sensitivity. The detection limit of Au NRs@SiO2 for E. coli O157:H7 is lower than 10 Colony-Forming Units (CFU), which is superior over the values of traditional methods34, 35.

Results and Discussion

Au NRs (Fig. 1 and 2A) were synthesized by using the seed-mediated growth method36, which has an aspect ratio of 2.9. As prepared Au NRs showed typical horizontal and longitudinal LSPR bands at 530 nm and 726 nm, respectively (Fig. 2C). The number of Au NRs in solution was estimated to be 2.1 nM according to its extinction coefficient (3.9 ± 0.5 × 109 M−1 cm−1) at the longitudinal plasmon peak (726 nm)37, 38. According to the traditional method (soft-templating method), Au NRs were uniformly coated with mesoporous silica, forming monodispersed core-shell AuNRs@SiO2 nanostructures (Fig. 1 and 2B)39. In the process of silica coating, CTAB formed a bilayer around Au NRs, which served as organic template for the formation of mesoporous silica shell40. Moreover, it was found that the longitudinal LSPR band of Au NRs@SiO2 redshifted clearly compared with Au NRs (Fig. 2C), leading to a lighter pink color (illustration of Fig. 2D).

Figure 1
figure 1

Schematic illustration of the synthesis of Au NRs and Au NRs@SiO2 and the procedure of detection for E. coli O157:H7.

Figure 2
figure 2

SEM (A) and TEM (B) of as-prepared Au NRs and Au NRs@SiO2, respectively; (C) UV-vis spectra of Au NRs (black) and Au@SiO2 (red); (D) Photographs of Au NRs (a) and Au@SiO2 (b).

In order to study systematically the influence of silica thickness on the LSPR of Au NRs@SiO2, Au NRs@SiO2 with different shell thickness were prepared by adjusting the concentration of CTAB and the amount of TEOS. When the additive amount of TEOS was changed from 2 µL to 20 µL, the silica shell thickness increased from 2 nm to 25 nm (Fig. 3). It is noteworthy that the thickness of silica was calculated according to the general theory of statistics by measuring more than 100 particles. Fig. S1 showed the statistical values and statistical distribution of Au NRs@SiO2 with 2 nm SiO2 layer. The thickness of other SiO2 layers on Au NRs@SiO2 (5, 10, 15, 20, 25 nm) were also confirmed by the general theory of statistics. CTAB was used as the template for depositing silica and many previous reports showed that lower concentration of CTAB resulting in thicker silica shell41,42,43. Therefore, by adjusting the concentration of CTAB and the amount of TEOS, Au NRs@SiO2 with different shell thickness could be prepared. The uniform silica shell endows a protective layer on the surface of Au NRs, leading to extremely stable Au NRs dispersion that could keep for three months at room temperature even after removal of CTAB.

Figure 3
figure 3

TEM images of Au NRs@SiO2 with different shell thickness. The thickness of silica were as follows, respectively: (a) 2 nm; (b) 5 nm; (c) 10 nm; (d) 15 nm; (e) 20 nm; (f) 25 nm.

Furthermore, the LSPR properties of Au NRs with different mesoporous silica shell were investigated by UV-vis absorption spectra (Fig. 4). The longitudinal plasmon bands of Au NRs@SiO2 redshifted gradually with increasing the thickness of silica shell (Fig. 4A). The relationship between plasmon shift and thickness of silica is shown in Fig. 4B, indicating that the plasmon band shift showed approximately linearly with increasing shell thickness. This was ascribed to the refractive index variation of silica shell when changing the thickness27. The refractive index of porous silica is much higher than the value of water. When the porous silica was coated onto the surfaces of Au NRs, the refractive index of surrounding environment of Au NRs increased, which was in accordance with previous work44. Therefore, the coating of silica on Au NRs led to redshift of the longitudinal plasmon band, which proved that the Au NRs@SiO2 was much sensitive to the change of surrounding refractive index than Au NRs. This allowed Au NRs@SiO2 could be employed as a LSPR sensor based on the redshift of longitudinal plasmon band induced by coating with mesoporous silica.

Figure 4
figure 4

(A) Normalized extinction spectra of Au NRs@SiO2 with different shell thickness from 2 nm to 20 nm; (B) Linearity curve of plasmon shift vs. the thickness of silica.

To verify the performance of the Au NRs@SiO2 based LSPR biosensor, Au NRs@SiO2 was firstly used to test the surrounding refractive index variations, as shown in Fig. 5. The sensitivity was calculation according to the universal experienced formula45:

$$\bigtriangleup \lambda ={\rm{m}}\cdot \bigtriangleup {\rm{n}}$$
(1)
Figure 5
figure 5

Normalized extinction spectra of Au NRs (A) and Au NRs@SiO2 with 2 nm shell thickness (B) in a mixture of water and glycerol with different volume ratios from 0.9 to 0.1 with the volume ratio of 0.1 interval; (C) Comparison of the refractive index sensitivity of Au NRs (a) and Au NRs@SiO2 with different SiO2 thickness from 2 nm to 20 nm (cross ponding to b to f); (D) Difference in sensitivity of Au NRs and Au NRs@SiO2 with different SiO2 thickness from 2 nm to 20 nm.

Δλ is the difference of the LSPR wavelength before and after coating; m is the sensitivity, Δn is the change in the refractive index.

The refractive index was tuned by adjusting the volume ratio of water and glycerol (from 0.9 to 0.1 with the volume ratio of 0.1 interval), and the refractive indices of the mixture solvents were calculated based on the Lorentz-Lorenz equation, as shown in the experimental details23, 46. Both of Au NRs and Au NRs@SiO2 exhibited band redshift when increasing the volume ratio of glycerol to water (Fig. 5A and B).

The plasmon peaks of Au NRs and Au NRs@SiO2 in mixed solution was plotted against with refractive index, as shown in Fig. 5C. It was found that plasmon absorption shifts linearly to longer wavelength with increasing the refractive index22, 47, 48. In addition, only absorption is considered here and the influence of scattering are neglected due to higher absorption than scattering of nanorods49.

The slope indicated the refractive index sensitivities, as shown in Fig. 5D. The sensitivity values of Au NRs@SiO2 with different thickness were ranged from 110 nm/RIU to 390 nm/RIU. The Au NRs@SiO2 with 2 nm shell exhibited highest sensitivity approaching to 390 nm/RIU, which was much higher than that of previous reports (the reported highest value was 325 nm/RIU)22, 33, 50. The sensitivity of Au NRs@SiO2 had intimate relation with the silica shell and reduced gradually with increasing the shell thickness, which agreed with the results in previous work22, 31. The sensitivity of Au NRs@SiO2 with 2 nm or 5 nm shell was larger than the values of Au NRs and the Au NRs@SiO2 with other thickness. Generally, the improvement in sensitivity can be explained according to the universal experienced formula50,51,52,53

$$\bigtriangleup {\rm{\lambda }}={\rm{m}}({n}_{adsorbate}-{n}_{medium})(1-{e}^{-\frac{2d}{{l}_{d}}})\,$$
(2)

Δλ is the difference of the LSPR wavelength before and after coating; m is the sensitivity; nadsorbate and nmedium are the refractive indexes of the shell and the solution, respectively; d is the thickness of the coating shell and ld is the electromagnetic field decay length of the system, make A equal to \((1-{e}^{-\frac{2d}{{l}_{d}}})\).

When Au NRs coated with thin silica, the change of A was ignored due to the minor change of d. The sensitivity was determined by the value of Δλ/Δn, which resulted in higher sensitivity than Au NRs due to higher change of Δλ than Δn. However, when the silica shell became much thicker, the change of d can’t be ignored, which resulted in the increase of A. Though the value of Δλ increased, the sensitivity decreased following the increase of Δn and A. Therefore, it is not uncommon that the Au NRs@SiO2 with 2 nm shell was with the highest sensitivity for about 390 nm/RIU.

Au NRs@SiO2 with 2 nm of shell thickness showed optimal sensitivity of 390 nm/RIU and can serve as ideal candidate for high-efficiency LSPR sensors. Au NRs@SiO2 was modified with specific antibody to selectively detect E. coli O157:H7. Due to the negative shell, the surface of the Au NRs@SiO2 was negatively charged, which provided opportunity for the electrostatic interaction between Au NRs@SiO2 and the positive antibody (Fig. S2) and simplified the procedure and avoided extra chemical treatment. E. coli O157:H7 samples with different concentration were mixed with antibody-conjugated Au NRs@SiO2 to promote the sufficient incubation. Then the typical plasmon band shifts of Au NRs were measured using UV-vis absorption spectra to detect E. coli O157:H7 (Fig. 6A). After integrated with E. coli O157:H7, the longitudinal plasmon band of Au NRs@SiO2 redshifted gradually and the absorption intensity was decreased gradually when increasing the concentration of E. coli O157:H7 in the range from 0 to 0.5 × 105 CFU (Fig. 6A).

Figure 6
figure 6

(A) UV-vis spectra of Au NRs@SiO2 after reaction with different concentrations (from 0 to 0.5 × 106 CFU) of E. coli O157:H7 in the 0.01 M PBS solutions (pH = 7.4); (B) Linearity curve for the plot of plasmon shift vs. the logarithm of concentration of E. coli O157:H7 (n = 1, 2, 3, 4, 5, 6).

Au NRs@SiO2 was sensitive to the surrounding refractive. With increasing the concentration of E. coli O157:H7, the refractive index around Au NRs@SiO2 increased, which led to the redshift of the longitudinal plasmon band24. The relationship between plasmon band shift and logarithmic concentration of E. coli O157:H7 is shown in Fig. 6B. It was found that the redshift changed linearly with the logarithmic concentration of E. coli O157:H7, which made it possible to detect E. coli O157:H7 quantitatively. Furthermore, the experiment of the selectivity of the sensor had been done by using Salmonella Typhimurium (S. Typhimurium) with the antibody of E. coli O157:H7 (Fig. S3) to replace E. coli O157:H7. The LSPR band of Au NRs@SiO2 was almost unchanged except some negligible change (around 0.5 nm). The results indicated that the antibody-conjugated Au NRs@SiO2 only bind to E. coli O157:H7 due to the specific recognition.

Conclusion

In summary, a highly sensitive plasmon resonance biosensor based on Au NRs@SiO2 was prepared to detect E. coli O157:H7 quickly and simply. By adjusting the concentration of CTAB and the amounts of TEOS, we synthesized monodisperse Au NRs@SiO2 with serious uniform silica shell. Meanwhile, the refractive index sensitivities of both Au NRs and Au NRs@SiO2 with different thickness of silica shell were investigated and the Au NRs@SiO2 with 2 nm shell was most sensitive compared to others. In addition, the Au NRs@SiO2 with 2 nm shell was used here to detect the E. coli O157:H7 by simply physical adsorption between antibodies and Au NRs@SiO2. The results indicated that the plasmon shift was very sensitive to the change of the concentration of E. coli O157:H7 and monitoring E. coli O157:H7 at concentration lower than 10 CFU in less than 40 min, which meant the LSPR platform based on Au NRs@SiO2 was sensitive, simple, quick for monitoring E. coli O157:H7 without any expensive instruments and this label-free method was promising to applied in detecting pathogenic agents.

Methods

Reagents and materials

Hexadecyltrimethylammonium bromide (CTAB), Sodium borohydride (NaBH4) and Tetraethylorthosilicate (TEOS) were commercially available from Sigma-Aldrich Chemical Co. (St. Louis, MO, USA). L-Ascorbic Acid (AA) was purchased from Energy Chemical in Shanghai. Chloroauricacid (HAuCl4•3H2O, 99.9%), Silver nitrate (AgNO3), ethanol, hydrochloric acid (HCl) and sodium hydroxide were purchased from Sinopharm Chemical Reagent Co. Ltd. (Shanghai). E. coli O157:H7 (1.7 × 108 CFU/mL), Salmonella Typhimurium (S. Typhimurium) (2.48 × 108 CFU/mL) and the murine anti- E. coli O157:H7 monoclonal antibody were purchased from Meridian Life Science, Inc. (Memphis, TN). Phosphate buffer saline (PBS, pH = 7.4) was purchased from Sigma Chemical Company (St. Louis, MO) and was used to dilute the E. coli O157:H7 stock solution (1.7 × 108 CFU/mL) with different concentrations (from 10 to 105 CFU/mL). Other chemicals were purchased from Sinopharm Chemical Reagent Co., Ltd. (China) and used without any further purification.

Transmission electron microscopy (TEM) was performed on a JEOL JEM-2100F instrument and operated at 200 kV. Scanning electronic microscopy (SEM) measurements were carried out by a JEOL JMS-6700F scanning microscope. UV-vis absorption spectra were collected by virtue of TU-1810 UV-vis spectrophotometer provided by Purkinje General. The surface zeta potential data was performed on a Zeta Potential Analyzer.

The Synthesis of Gold Nanorods

CTAB stabilized gold nanorods were synthesized using the seed-mediated growth method with minor modifications36, 54. First, 0.6 mL of freshly prepared ice-cold aqueous NaBH4 solution (0.01 M), was added into mixed aqueous solution containing 0.25 mL, 0.01 M HAuCl4 and 9.75 mL, 0.1 M CTAB. After string violently for 2 min, the seeds formed and were used within 10~120 min. The growth solution was prepared by mixing the aqueous solution of 4 mL, 0.01 M HAuCl4, 0.8 mL, 0.01 M AgNO3, 80 mL and 0.1 M CTAB firstly. Then 0.64 mL, 0.1 M freshly prepared aqueous ascorbic acid solution was added into the above mixture solution with gentle string, followed by adding 1.6 mL, 0.1 M HCl aqueous solution. After mixing the resultant solution with gentle string, 0.02 mL seed solution was added then mixing it with gentle inversion for 10 s and then left the growth solution undisturbed at least 6 h.

The synthesis of Au NRs@SiO2 with different thicknesses

The synthesis of Au NRs@SiO2 with homogeneous silica thickness was carried out according to the traditional soft-templating method55. The 10 mL of as-prepared Au NRs was washed using deionized water by centrifugation (6500 rpm, 10 min) for 2 times. The supernatant was removed and the pellet was diluted to 10 mL by adding deionized water. Then a certain amount of NaOH (0.1 M) was added to the above solution to adjust the solution PH to 10.6. After the solution was mixed for 20 min, three 2 µL, 4 µL, 6 µL, 10 µL, 15 µL, 20 µL injections of 20% TEOS in ethanol solution was added under gentle stirring at 30 min intervals and the solution was mixed under room temperature for 24 h.

Refractive Index Sensitivity Measurements

Water/glycerol solutions with a percentage of glycerol ranging from 0 to 90% at 10% intervals were used to change the refractive index experienced by the Au NRs and Au NRs@SiO2. The refractive indexes were calculated according to the Lorentz-Lorenz equation as follows:

$$\frac{{n}_{12}^{2}-1}{{n}_{12}^{2}+2}={\phi }_{1}\frac{{n}_{1}^{2}-1}{{n}_{1}^{2}+2}+{\phi }_{2}\frac{{n}_{2}^{2}-1}{{n}_{2}^{2}+2}$$
(3)

Wherein n12 is the refractive index of the mixture, n1 (1.3334) and n2 (1.4746) are the refractive indices of water and glycerol, respectively, φ 1 and φ 2 are their volume fractions. For sensitivity measurements, 3 mL particle samples in solvent with different concentration of glycerol were used. The location of the absorption peak changed response to the concentration variety of glycerol. The LSPR shift showed linearly dependence on the refractive index change and the slope represented the sensitivity of the corresponding sample.

Immobilization of antibodies on Au NRs@SiO2 and Detection of E. coli O157:H7

Firstly, 5 mL of as-prepared Au NRs@SiO2 was washed for 2 times by centrifugation (6500 rpm, 6 min) and redispersed into 5 mL PBS solution (pH 7.4, 0.01 M). Then 1 mL 0.1 µg mL−1 antibodies for E. coli O157:H7 was added into the above solution and stirred for 30 min at room temperature. Then the antibodies conjugated Au NRs@SiO2 was centrifuged for once to remove free antibodies and redispered into 5 mL of PBS (pH 7.4, 0.01 M). 0.5 mL E. coli O157:H7 with different concentrations were mixed with 0.5 mL the as-synthesized antibodies conjugated Au NRs@SiO2. After gentle shaking for 10 min, the mixture was settled for 70 min without disturbance at 37 °C. Then the resultant solution was detected under UV-vis measurement. The selective experiment was similar to the above detecting experiment just replaced the E. coli O157:H7 with S. Typhimurium of equal volume.