Detection of HER2 through Antibody Immobilization Is Influenced by the Properties of the Magnetite Nanoparticle Coating

Villegas-Serralta, Enrique; Zavala, Oscar; Flores-Urquizo, Israel Alejandro; García-Casillas, Perla E.; Chapa González, Christian

doi:https://doi.org/10.1155/2018/7571613

Journal of Nanomaterials

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Abstract Introduction Materials and Methods Results and Discussion Conclusions Conflicts of Interest Acknowledgments References Copyright Related Articles

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Advanced Nanomaterials for Biological Applications

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Research Article | Open Access

Volume 2018 | Article ID 7571613 | https://doi.org/10.1155/2018/7571613

Detection of HER2 through Antibody Immobilization Is Influenced by the Properties of the Magnetite Nanoparticle Coating

Enrique Villegas-Serralta,¹Oscar Zavala,²Israel Alejandro Flores-Urquizo,³Perla E. García-Casillas,¹and Christian Chapa González¹

Academic Editor: Jin-Ho Choy

Received28 Jul 2017

Revised27 Dec 2017

Accepted12 Feb 2018

Published02 Apr 2018

Abstract

Considerable effort has been focused on improving the control of size, shape, and surface modifications to detect proteins. The purpose of this study was to compare the efficiencies of aminosilane-coated magnetite (As-M) nanoparticles (NPs), dextran-coated magnetite nanoparticles (Dx-M), and bare nanoparticles for conjugating single-chain variable fragment antibodies (scFvs) with the aim of detecting the human epidermal growth factor receptor 2 (HER2) protein. Dx-M and As-M NPs were characterized using scanning electron microscopy, energy dispersive X-ray spectroscopy, X-ray diffraction, and Raman spectroscopy. Dx-M and As-M were conjugated with a monoclonal scFv for active targeting of the HER2 antigen. Aminosilane surface coating enhanced the scFv conjugation efficiency over twofold compared to that of the dextran-coated magnetite NPs for the detection of HER2 proteins.

1. Introduction

The development of nanomaterials has been widely touted as a revolutionary paradigm shift for biological applications. In recent years, considerable effort has been focused on improving the control of size, shape, and surface modifications to gain better behavior as well as improved functionalization. Magnetic nanoparticles (NPs) have become widely studied due to the rapid increase in the number of applications in the biomedical field, such as magnetic resonance imaging [1], hyperthermia [2], drug delivery [3, 4], gene therapy [5, 6], protein immobilization [7, 8], and immunoassay [9]. Among other applications of magnetic NPs, for the immunoassay, the conjugation of NPs with antibodies is the critical step and severely limited by low efficiency of antibodies grafted on the NP surface.

Although there has been significant work done on the conjugation of chemically synthesized magnetite NPs to antibodies [10–15] there have been relatively few studies comparing the influence of antibody immobilization method in effectiveness of antigen detection. The conjugation of the proteins with magnetic NPs can be done via physical adsorption using polymer coatings, such as dextran, and by covalent immobilization using amino derivatives, such as aminosilane [3]. Dextran is a natural polysaccharide that confers exceptionally high colloidal stability to NPs [16]. 3-(2-aminoethylamino) propyltrimethoxysilane (APTES) is the most frequently used compound to produce the aminosilane coating to enhance protein adhesion [17–20]. Both dextran and aminosilane have been used for the surface modification of NPs to immobilize antibodies and to improve the dispersion of magnetite NPs. Despite the influence on dispersion stability of the NPs, the type of coating has a remarkable influence on the effectiveness of antibody immobilization.

The effectiveness of conjugation has an impact on the detection of bioanalytes, such as cancer biomarkers. Overexpression of human epidermal growth factor receptor 2 (HER2) is common to several types of human carcinomas [21–23], is involved in cell growth, and is a recognized biomarker for breast cancer therapy [24–27]. The aim of this study is to compare aminosilane-coated magnetite (As-M) NPs and dextran-coated magnetite (Dx-M) NPs conjugated with recombinant single-chain variable fragment antibodies (scFvs) to Her2 (anti-HER2) through an adapted enzyme-linked immunosorbent assay (ELISA) in order to choose the most efficient scFv immobilizing agent.

2. Materials and Methods

2.1. Synthesis of Magnetite NPs

Magnetite NPs were synthesized by alkaline coprecipitation of two equivalents of ferric chloride (FeCl₃·6H₂O; Mallinckrodt) and one equivalent of ferrous sulfate (FeSO₄·7H₂O; J.T.Baker) in 30% ammonium hydroxide solution (NH₄OH; J.T.Baker) with stirring. The obtained precipitate was centrifuged at 6,000 rpm and washed several times with distilled water until a pH ~ 7 was reached. Finally, the precipitate was dried at 80°C for 24 hours.

2.1.1. scFv Conjugation on Dx-M NPs

For the preparation of Dx-M NPs, dextran (molecular weight 20,000 Da) was dissolved in distilled water. FeCl₃ (0.01 M) and FeSO₄ (0.005 M) were dispersed in 0.05% dextran solution. Synthesis of the NPs was done as previously described. The products were separated with a magnet and washed several times with deionized water. Dx-M was resuspended in phosphate buffer solution (pH 7.4). Then, 500 μL of Dx-M suspension and 500 μL of scFvs were mixed by stirring gently and incubated in a cold room at 4°C for 24 hours. The products were collected with a magnet and washed with buffer.

2.1.2. scFv Conjugation on As-M NPs

The obtained magnetite powder (200 mg) was dispersed in 150 mL of ethanol and sonicated for 15 minutes, before the addition of 3-(2-aminoethylamino) propyltrimethoxysilane (AEPTMS, Sigma-Aldrich). After ultrasonic agitation for 30 min, the suspended NPs were collected by magnetic decantation. The precipitated product (As-M) was washed with ethanol five times and dried at 80°C for 24 hours. The As-M NPs were resuspended in 1.0 mL of 2% glutaraldehyde aqueous solution with stirring for 4 hours at room temperature. Then, a mixture of 500 μL of As-M and 500 μL of scFvs was added and incubated in a cold room at 4°C for 24 hours to allow conjugation to take place. Finally, the solution was dialyzed with phosphate buffered saline (PBS).

2.2. Characterization of NPs

The bare magnetite sample was analyzed in PANalytical X’Pert MRD PRO device with a Cu-kα source (λ = 1.5406 Å) operating at 40 kV and 30 mA and at a scanning rate of 0.1° 2θs⁻¹ from 10 to 80° 2θ. Distances between peaks were compared to the International Centre for Diffraction Data JCDPS, number 5-0664. The average diffracting crystallite size of the prepared NPs was calculated using Scherrer’s equation from the most intense peak. Scanning electron microscopy (SEM) was performed using a JEOL JSM6010LV/PLUS SEM to determine the particle size and morphology of the magnetite nanoparticles. For particle size analysis, the image processing software Scandium was used and 100 particles were analyzed to calculate the mean diameter ± standard deviation (SD). SEM images were made with an accelerating voltage of 20 kV and a working distance of 4 10 mm. Energy dispersive X-ray spectroscopy (EDS) using an Inca apparatus (Oxford Instruments, Oxford, UK) was done for elemental analysis or chemical characterization of the samples. TEM data was also provided to confirm the chemically well-defined magnetite nanoparticles. Hydrodynamic diameters and zeta potentials were analyzed using a dynamic light scattering (DLS) (Nanotrac Wave, Microtrac) operating at 25°C in a scattering angle of 180°; samples were suspended in Triton 2%, pH 7, and sonicated 5 minutes prior to measurement. Fourier transform infrared spectra (FTIR) were recorded using a spectrometer (Nicolet 6700/Thermo Electron) to identify functional groups present in the surface-modified magnetite nanoparticles. Infrared spectra with attenuated total reflection (ATR) were recorded with a resolution of 4 cm⁻¹ and the scan range was set from 4000 to 600 cm⁻¹. Raman spectra were recorded in a WiTec system model Alpha 300 RA equipped with a 785 nm laser source. Raman spectroscopy was used to measure bands of -S-S-, -N-C-N-, and -C-S-, which are likely to be found in proteins (scFvs). These groups are rich in π-electron and, thus, have larger polarizability and totally symmetric vibrational modes that are Raman active but may not be infrared (IR) active and show no IR bands [28]. Because of these differences and considering that water, the natural medium for proteins is a weak Raman scatter; Raman was the method chosen for characterization of antibody-NP conjugate. In addition, for proteins, studies focused on investigating Raman spectra of proteins and the successful design of NP probes has allowed advances in immunoassays [29].

2.3. ELISA

Aliquots (50 μL) of the homogenized suspensions (scFv-Dx-M, scFv-As-M, and Dx-M) were deposited on the bottom of wells in a 96 well microplate. Next, a permanent magnet was used to immobilize the conjugates at the bottom. The plates were blocked with PBS containing 5% bovine serum albumin (BSA). Successively, anti-HA antibody and horseradish peroxidase (HRP; GE Healthcare Life Sciences) were added and incubated at 37°C for 1 hour. Unbound anti-HA was discarded by washing. All washing steps were performed with 200 μL of PBS–0.05% Tween 20. Finally, 50 μL of 2,2′-Azino-bis(3-ethylbenzthiazoline-6-sulfonic acid) (ABTS, Roche) was added and incubated for 15 minutes at room temperature and the absorbance was read at λ = 405 nm in a Benchmark Plus device (Bio-Rad, Hercules, CA, USA). Each independent experiment was run in triplicate.

2.4. Statistical Analyses

Data are presented as the mean ± standard deviation (SD). Differences between groups were assessed by one-way analysis of variance (ANOVA) followed by Tukey’s Multiple Comparison Analysis test. Values were determined as significant when .

3. Results and Discussion

The X-ray diffraction (XRD) pattern of uncoated magnetite is shown in Figure 1, with the peaks corresponding to the planes for (2 2 0), (3 1 1), (4 0 0), (4 2 2), (5 1 1), and (4 4 0); peaks are matched in position and in relative intensity to the inverse spinel structure of magnetite pattern according to JCPDS 5-0664. The average size of the crystallite was calculated by the Scherrer equation [30–33], in which peak width is inversely proportional to crystallite size. The average crystallite size was 10.1 nm, which is consistent with the size of superparamagnetic particles [34].

SEM revealed the morphological properties of the prepared samples (Figure 2). Monodisperse magnetite NPs were successfully synthesized. While a number of suitable methods have been developed for the synthesis of magnetic NPs, the coprecipitation method yielded magnetite NPs with a relatively uniform and spherical morphology with narrow particle size distribution ( nm) according to SEM measurements. The mean diameter of both coated particles was around 20 nm. Furthermore, the EDS spectrum revealed Fe and O in bare magnetite samples; Fe, O, and C in Dx-M samples; and Fe, O, and Si in As-M samples, consistent with the presence of aminosilane-modified NPs. In all the samples, the carbon signal appeared due to the preparation of the sample; however in Dx-M sample the signal was more intense.

(a)

(b)

(c)

Representative TEM image with corresponding size distribution of magnetite nanoparticles is shown in Figure 3. Well-defined nearly spherically shaped nanoparticles were indeed obtained. Their average size, determined from the statistical sample of over one hundred nanoparticles, was found to be 9.0 nm, while standard deviation of 2.3 nm indicated a reasonably narrow size distribution. Moreover, notice the accurate agreement between the average diameter assessed from both XRD and TEM data confirming the presence of monodomain nanoparticles.

Figure 4 shows the hydrodynamic size of M, As-M, and Dx-M samples. The particle size, its distribution, and the surface charge of Fe₃O₄ are very important parameters not only for modifying Fe₃O₄ nanoparticles, but also for biomedical applications. The coating of the nanoparticles can be evaluated by measuring the zeta potential. The results of the mean hydrodynamic diameter, polydispersity index (PDI), and zeta potential of the surface-modified magnetite nanoparticles developed in this study are listed in Table 1. The smallest hydrodynamic diameter of about nm was obtained for bare magnetite nanoparticles. The mean particles size of As-M and Dx-M was found to be, and nm, respectively, suggesting that the AEPTMS coating did induce a significant increase of the mean particles size . Contrastingly, the coating with dextran did not induced a significant increase of the particles diameter . The zeta potential value obtained for M was slightly negative (−1.10 mV); this explains why magnetite nanoparticles do not remain suspended for a long period of time. A zeta potential of −23.10 mV was observed for magnetite nanoparticles coated with AEPTMS. Thus, the use of AEPTMS as a coating also contributed to an increase in colloidal stability. The zeta potential of Dx-M nanoparticles was −8.56 mV, which suggested that the nanoparticles were mainly stabilized by steric repulsion.

(a)

(b)

(c)

The FTIR-ATR comparative spectra of bare and coated Fe₃O₄ nanoparticles, as well as the coating molecules, are displayed in Figure 5. The samples that contain magnetite (M, Dx-M, and As-M) clearly reveal the presence of strong IR absorption band between 500 and 600 cm⁻¹ characteristic to the Fe-O vibration. IR spectra of pure AEPTMS are shown in Figure 5(b) while the IR spectra of As-M are shown in Figure 5(c). The IR spectrum of AEPTMS exhibits absorptions at 2890 cm⁻¹ and 1059 cm⁻¹, which are characteristic peaks of the stretching vibration of C-H and Si-O, respectively. In the spectrum for As-M the peaks for the functional group N-H and silane binding are marked. A displacement of the Si-O peak is observed in the As-M NPs. The peak found at 1383 cm⁻¹ attributed to the stretching vibrations of C-N bond, along with the band at 3360 cm⁻¹ attributed to the H-N-H bending mode of free amino groups, indicates that the AEPTMS has been grafted onto the nanoparticles’ surface. In the same way, Figures 5(d) and 5(e) give the IR absorption spectra of pure dextran and Dx-M, respectively. The very broad band at 3380 cm⁻¹ in both Dx and Dx-M can be attributed to the stretching vibration of O-H. The absorption bands at 2924 cm⁻¹ can be ascribed to the asymmetrical stretching vibration of C-H and the band at 1008 cm⁻¹ belongs to stretching vibrations of C-O-C bond and glycosidic bridge. Regardless of the Fe-O band found in Dx-M, very few differences can be found in the IR spectra of Dx and Dx-M which indicates that dextran coating occurs by physical adsorption.

Nevertheless, to further evaluate the antibody Raman spectroscopy was conducted. Raman spectra of the obtained materials are shown in Figure 6. According to the literature, the modes present at 207, 392, and 470 cm⁻¹ (Figure 6(a)) correspond to magnetite [35] and the band at near 1300 cm⁻¹ is also attributable at magnetite [36, 37]. In the other samples, the spectral bands seen below 800 cm⁻¹ are primarily attributed to presence of magnetite [38] (Figures 6(b), 6(c), 6(e), and 6(f)). The Raman spectrum for the Dx-M included the typical signals for the dextran and weak bands typical of magnetite. For the Raman spectroscopy of the Dx-M, the surface modification of dextran-coated magnetite manifested in the electronic and vibrational properties of the magnetite and resulted in the lowering of the energy (Figure 6(b)). For aminosilane treated surfaces (Figure 6(c)), the characteristic bands at 1117 cm⁻¹ corresponded to Si-O-C, 1348 cm⁻¹ could be attributed to Csp³ bound with or without heteroatoms, 1575 cm⁻¹ was associated with bound Csp², and 3300 cm⁻¹ was related to an amine group. The results were consistent with the presence of aminosilane on the surface of the magnetite NPs. Raman spectroscopy of the antibody (Ab) soluble scFv (Figure 6(d)) was obtained. The test solution contained 1 μg/mL scFv diluted in PBS. The Raman spectra scFv is typical of proteins [38, 39] with bands associated with disulfide bonds (-S-S-, 544 cm⁻¹), polypeptide backbone (Cα-C, 940 cm⁻¹), aromatic amino acids (phenylalanine, tryptophan, and tyrosine, bands from 1000 to 1205 cm⁻¹), C-H deformation (1325 and 1452 cm⁻¹), and amide III (1267 cm⁻¹). The immobilization of the antibodies in both conjugates Dx-M and As-M were consistent with the Raman spectra of Dx-M-Ab (Figure 6(e)) and As-M-Ab (Figure 6(f)); both exhibited bands characteristic of the scFvs. The Raman spectrum for the Dx-M-Ab conjugates included the typical signals for the dextran and weak bands typical of proteins (amide I and phenylalanine aromatic ring near at 1600 cm⁻¹). The Raman band at ≈1550 cm⁻¹ arises from an indole ring vibration that is contributed mainly by Trp in Dx-M-Ab and As-M-Ab samples [20].

(a)

(b)

(c)

(d)

(e)

(f)

The conjugated product was verified by ELISA using a magnetic separator (Figure 7). Fifty microliters of the homogenized suspensions (scFv-Dx-M, scFv-As-M, and Dx-M) were used for ELISA using a magnet to immobilize the conjugates (Figure 7) using HRP-conjugated anti-HA. The ABTS assay is a colorimetric assay based on the ABTS cation radical formation. The radical formation is catalyzed by the reduction of HRP in the presence of H₂O₂. Employing this assay, we are able to compare the absorbance generating from the Dx-M-Ab and As-M-Ab conjugates and Dx-M nonconjugate scFv (as the negative control) against a secondary anti-HA antibody. The 2-fold difference in ELISA absorbance between scFv-AsM conjugates and scFv-DxM was indicative of successful conjugation (Figure 8). Based on the results of the evaluation of the ability of anti-HER2 scFv-magnetite conjugate in binding and detecting the studied protein, the chemical modification with aminosilane remarkably improved the protein detection. In addition, the success of binding to HER2 by As-M confirmed the existence of stable chemical bonding between the NPs and antibody. This was not evident in the Dx-M material whose modification occurs primarily by physical adsorption. However, a considerable difference was observed with respect to the first coating. The results allowed us to infer that, despite the washes performed on the aminosilane coating, the continuous antibody coupled to the nanoparticles and was recognized by the secondary anti-HA antibody. The results indicate that this coating is suitable for this type of material bioconjugate.

4. Conclusions

In this study, well-defined magnetite nanoparticles with a narrow size distribution and coated with AEPTMS and dextran were successfully obtained. Furthermore, zeta potential measurements show that the magnetite nanoparticles coated with AEPTMS or dextran are stable in aqueous suspension at pH 7 which makes these nanomaterials suitable for biomedical applications. Surface-modified magnetite nanoparticles containing antibodies were prepared and their antigen recognition ability toward HER2 as a model biomarker was performed. We successfully used this nanomaterial to study how coating changes the efficiency of antibody conjugation and, consequently, how it also affects protein detection in the magnetic bead ELISA. As-M NPs were more efficient in scFv immobilization than Dx-M NPs conjugated with recombinant scFv anti-Her2. This strategy provides an alternative approach to controlling surface functionalization with a view to preparing high-efficiency receptor for specific proteins. The immunoconjugate was proven to have a biomarker-targeting activity. Such As-M might be very useful for biomagnetically targeted detection in several types of human carcinoma.

Conflicts of Interest

The authors declare that there are no conflicts of interest regarding the publication of this article.

Acknowledgments

The authors thank Karla Jacqueline Licona, for her help in preparing the manuscript, and Professor Carlos Rodriguez from UTCJ, for providing the SEM-EDS facilities.

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Copyright © 2018 Enrique Villegas-Serralta et al. This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

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