A Simple Label-Free Aptamer-Based Electrochemical Biosensor for the Sensitive Detection of C-Reactive Proteins

The level of C-reactive protein (CRP) in the human body is closely associated with cardiovascular diseases and inflammation. In this study, a label-free functionalized aptamer sensor was attached to an electrode trimmed with in-gold nanoparticles and carboxylated graphene oxide (AuNPs/GO-COOH) to achieve sensitive measurements relative to CRP. Gold nanoparticles were selected for this study due to super stability, remarkably high electrical conductivity, and biocompatibility. In addition, carboxylated graphene oxide was utilized to promote the anchorage of inducer molecules and to increase detection accuracies. The sensing signal was recorded using differential pulse voltammetry (DPV), and it produced a conspicuous peak current obtained at approximately −0.4 V. Furthermore, the adapted sensor manifested a broad linear span from 0.001 ng/mL to 100 ng/mL. The results also demonstrated that this aptamer sensor had superior stability, specificity, and reproducibility. This aptamer-based electrochemical sensor has enormous potential in complex application situations with interfering substances.


Introduction
C-reactive proteins (CRPs) were first revealed in 1930 in the plasma of lung inflammation patients [1]. CRP is a rapid-phase inflammatory protein arising primarily from hepatocytes under the influence of cellular factors such as interleukin (IL)-6 and tumor necrosis element alpha (TNF-α) [2]. As an acute inflammatory mediator in plasma during the inflammation response, CRP plays a regulatory role during inflammation responses by enhancing phagocytosis and activating complement. When the body is exposed to inflammatory stimuli or bacterial infections, the CRP level rises after 4-6 h of activation and increases approximately 1-fold every 8 h, usually peaking at 36-50 h [3]. With the recovery of inflammation, the CRP level declines explosively over 18 to 20 h, approaching the half-life of CRP [4]. It is well-established that CRP concentrations in the body is intimately correlated with heart-related diseases [5,6], cardiovascular diseases [7,8], rheumatoid arthritis [9], cancer [10,11], and inflammation [12]. Recently, the CRP has also been found to be associated with depression [13][14][15][16]. Some studies demonstrated that the epidemiological profile for diagnosing hypo-inflammatory depression can be verified by using the level of C-reactive proteins [17]. Related research also showed that CRP can predict the severity of COVID-19 [18][19][20]. Therefore, it is valuable for detecting CRP accurately.
The current detection methods for CRP include enzyme-linked immunosorbent (ELISA) [21], latex-enhanced immunoturbidimetry [22], single radial immunodiffusion (SRID) [23,24], and immunoscattering turbidimetry [25,26]. However, the limitations of these techniques are also evident: They are vulnerable to interference, time consuming, expensive instruments, and require complex operations, and they are particularly inadequate in the clinical development of effective treatment strategies and timely and rapid CRP detections [27].
surface and the number of immobilized aptamers [55]. Bharti A. et al. used GO-COOH with gold-platinum bimetallic nanoparticles to analyze the microRNA-21 detection [56].
Within this study, we designed an approach for CRP-sensitive tracking: label-free functionalized electrochemical aptamers were immobilized on gold nanoparticles and carboxylated graphene oxide (AuNPs/GO-COOH) composites to achieve sensitive measurements of the CRP. For label-free sensors, molecular imprinting techniques use the target as a template to synthesize polymer chains, which are anchored to an electrode and change conformations upon binding to the target to enable the label-free sensing of the electrochemical platform [57]. There are also electrochemical aptamer sensors that rely on electroactive small molecules, such as methylene blue (MB), to act as electron transfer agents [58]. Combining thiol groups at the ends of the aptamer, the malachite green aptamers (MGAs) bind to the malachite green (MG) to bring the bis-thiolated aptamer within close proximity to the cantilever's surface to create higher surface stress [59]. The proposed label-free aptasensor performs conformation changes when it interacts with the target CRP, resulting in an electrochemical response shift. One end of the DNA aptamer was modified with an amino group, which can be bound to GO-COOH with an amide bond to achieve the stable adhesion of the ligand to the electrode surface. Before binding to CRP, the adaptor was perpendicular to the electrode's surface and was highly flexible. When CRP bound specifically to the aptamer, a rigid aptamer-CRP complex was formed and the aptamer conformation changed, bending toward the electrode's surface and raising the electrical signature. In this work, we first selected the adaptor sequence of the detectors based on their CRP sequence design. Next, the CRP aptamer with a modified amino group was anchored on the superficial face of the bare electrode trimmed with carboxylated graphene oxide. The CRP aptamer was anchored to the electrode composite via the amide bond and demonstrated high stability, specificity, and reproducibility for CRP. In this study, the morphology and electrochemical feedback of the electrodes were evaluated by scanning electron microscopy and differential pulse voltammetry, respectively.

Apparatus
The compound-based sensing interface was visually characterized via layer-by-layer modifications using a high-resolution scanning electron microscope (SEM, Nova NanoSEM 430, FEI, Columbia, MD, USA). All electrochemical measurements, including square wave voltammetry (SWV), and differential pulse voltammetry (DPV) were performed on a CHI660E electrochemical workstation (ChenHua, Shanghai, China). The experiments were performed using screen-printed electrodes (SPE, poten, Beijing, China) with both working and auxiliary electrodes of carbon and silver/silver chloride as reference electrodes to form a three-electrode system. All electrochemical measurements were carried out at room temperature (25 ± 2 • C). Square wave voltammetry was applied at a scan rate of 100 mV/s with a range of −1.0 V~−0.2 V. Differential pulse voltammetry was performed with a voltage range of −0.6 V~0 V, an impulse amplitude of 50 mV, and a pulse width of 50 ms.

Reagents and Materials
Sodium tetrachloroaurate dihydrate (NaAuCl 4 -2H 2 O, Aladdin, Beijing, China), sodium sulfate (Na 2 SO 4 , Aladdin, Beijing, China), carboxylated graphene oxide (GO-COOH, XFNANO, Nanjing, China), phosphate buffer (PBS, Aladdin, Beijing, China), 1-(3-dimethylaminopropyl)-3-ethylcarbodiimide hydrochloride (EDC), N-Hydroxysuccinimide (NHS), MES, sodium chloride (NaCl), bovine serum protein (BSA, Genview, Haosogbio, Tianjin, China), Creactive protein (CRP) rabbit mAb (ABclonal, Wuhan, China), PSA standard (China Food and Drug Administration), CA125 standard, proplatelet basic protein (PPBP), and B-type brain natriuretic peptide (BNP) were used. CRP aptamer probes were ordered from Synbio Technologies (Suzhou, China). The DNA aptamer nucleotide sequences are as follows: 5 -(NH2) GCCTGTAAGGTGGTCGGT GTGGCGAGTGTGTTAGGAGAGATTGC-3 [39]. Figure 1 illustrates the preparation process of the SPE/AuNPs/GO-COOH aptamer sensor for the electrochemical detection of CRP. The electrodes were rinsed several times with ultrapure water and then blown dry and set aside for operation. The preparation of a 1% mass fraction of NaAuCl 4 -2H 2 O solution and 0.5 M Na 2 SO 4 nanogold reduction source solution was performed and they were dropwise added on the SPE electrode at a volume ratio of 1:1. The modification of AuNPs continued on the electrode's surface by using square wave voltammetry with a scanning rate of 100 mV/s at −1.0 V~−0.2 V for five turns. It was then rinsed with ultrapure water and air blown until dry. The GO-COOH was decorated on the modified SPE/AuNPs electrode using physisorption at a 2 mg/mL concentration and dried naturally at room temperature. The surface was flushed gently with ultrapure water and then air blown until dry. The CV scan electrode was then used to determine whether GO-COOH was successfully modified relative to the surface. A concentration of 2 mM EDC solution was prepared by mixing 0.4 mg EDC with 1 mL 0.1 M MES and 0.5 M NaCl (pH = 6.0) with shaking. The 0.6 mg NHS was thoroughly mixed with 1 mL PBS to configure the NHS solution with a concentration of 5 mM. The EDC solution and NHS solution were added onto the surface of the modified SPE/AuNPs/GO-COOH electrode dropwise in 1:1 volume and placed at indoor temperature for 15 min to activate carboxyl groups. The modified CRP aptamer was immobilized by amide bonding on the SPE/AuNPs/GO-COOH electrode, which completed carboxyl activation, and then the electrode was placed at room temperature overnight. The SPE/AuNPs/GO-COOH aptamer sensor was closed by adding 1 mg/mL of BSA dropwise to the modified electrode and left for 30 min at 4 • C in a humid environment. At this point, the label-free aptamer sensor modification process had been completed. The specific binding of CRP to the aptamer led to an enhanced current signal as the aptamer changed from a soft structure to a rigid structure, while the orientation shifted from perpendicular to the electrode to curved toward the electrode's surface, as shown in Figure 1.

Protocol of Electrochemical Aptamer Sensor
Tianjin, China), C-reactive protein (CRP) rabbit mAb (ABclonal, Wuhan, China), PSA standard (China Food and Drug Administration), CA125 standard, proplatelet basic protein (PPBP), and B-type brain natriuretic peptide (BNP) were used. CRP aptamer probes were ordered from Synbio Technologies (Suzhou, China). The DNA aptamer nucleotide sequences are as follows: 5′-(NH2) GCCTGTAAGGTGGTCGGT GTGGCGAGTGTGTTAGGAGAGATTGC-3′ [39]. Figure 1 illustrates the preparation process of the SPE/AuNPs/GO-COOH aptamer sensor for the electrochemical detection of CRP. The electrodes were rinsed several times with ultrapure water and then blown dry and set aside for operation. The preparation of a 1% mass fraction of NaAuCl4-2H2O solution and 0.5 M Na2SO4 nanogold reduction source solution was performed and they were dropwise added on the SPE electrode at a volume ratio of 1:1. The modification of AuNPs continued on the electrode's surface by using square wave voltammetry with a scanning rate of 100 mV/s at −1.0 V ~ −0.2 V for five turns. It was then rinsed with ultrapure water and air blown until dry. The GO-COOH was decorated on the modified SPE/AuNPs electrode using physisorption at a 2 mg/mL concentration and dried naturally at room temperature. The surface was flushed gently with ultrapure water and then air blown until dry. The CV scan electrode was then used to determine whether GO-COOH was successfully modified relative to the surface. A concentration of 2 mM EDC solution was prepared by mixing 0.4 mg EDC with 1 mL 0.1 M MES and 0.5 M NaCl (pH = 6.0) with shaking. The 0.6 mg NHS was thoroughly mixed with 1 mL PBS to configure the NHS solution with a concentration of 5 mM. The EDC solution and NHS solution were added onto the surface of the modified SPE/AuNPs/GO-COOH electrode dropwise in 1:1 volume and placed at indoor temperature for 15 min to activate carboxyl groups. The modified CRP aptamer was immobilized by amide bonding on the SPE/AuNPs/GO-COOH electrode, which completed carboxyl activation, and then the electrode was placed at room temperature overnight. The SPE/AuNPs/GO-COOH aptamer sensor was closed by adding 1 mg/mL of BSA dropwise to the modified electrode and left for 30 min at 4 °C in a humid environment. At this point, the label-free aptamer sensor modification process had been completed. The specific binding of CRP to the aptamer led to an enhanced current signal as the aptamer changed from a soft structure to a rigid structure, while the orientation shifted from perpendicular to the electrode to curved toward the electrode's surface, as shown in Figure 1.

CRP Detection
The DPV method was implemented for the electrochemical inspection of SPE/AuNPs/GO-COOH aptamer sensors to establish a relationship between the peak differential pulse current and CRP concentration. The scanning voltage ranged from −0.6 V to 0 V with a pulse amplitude of 50 mV and a pulse width of 50 ms. First, 100 μL of CRP solutions with concentrations of 0.001 ng/mL, 0.01 ng/mL, 0.1 ng/mL, 1 ng/mL, 10 ng/mL, and 100 ng/mL was configured using CRP standards with PBS as the solvent. The gradient concentration of the CRP standard solution was performed for DPV sweeps to establish a

CRP Detection
The DPV method was implemented for the electrochemical inspection of SPE/AuNPs/ GO-COOH aptamer sensors to establish a relationship between the peak differential pulse current and CRP concentration. The scanning voltage ranged from −0.6 V to 0 V with a pulse amplitude of 50 mV and a pulse width of 50 ms. First, 100 µL of CRP solutions with concentrations of 0.001 ng/mL, 0.01 ng/mL, 0.1 ng/mL, 1 ng/mL, 10 ng/mL, and 100 ng/mL was configured using CRP standards with PBS as the solvent. The gradient concentration of the CRP standard solution was performed for DPV sweeps to establish a relationship between peak differential pulse current and CRP concentrations. To investigate the stability of the sensors that we designed, multiple DPV detections were conducted by using 1 ng/mL of the CRP standard solution on the electrodes on the first, third, fifth, and seventh days to observe changes in the results. The SPE/AuNPs/GO-COOH aptamer sensors were preserved in the 4 • C refrigerator when out of use. The selectivity of the aptamer sensors was further verified by detecting possible disturbing substances with 100 µL of 1 ng/mL PSA, 1 ng/mL of CA125, 1 ng/mL of PPBP, and 1 ng/mL of BNP configured as interfering solutions compared with 1 ng/mL of the CRP standard solution for DPV scale verification. Regarding whether the designed sensor is repeatable, we selected five identical electrodes to test the 1 ng/mL CRP solution for multiple repetitions of the DPV detection.

Characterization of SPE/AuNPs/GO-COOH Aptamer-Sensing Interfaces
We examined the appropriate substances for modifying SPE working electrodes to derive a high electrochemical probe current response. Figure 2A shows the electrodeposition of AuNPs on the electrode's surface using SWV at a scan rate of 100 mV/s with a scan voltage of −1.0 V~−0.2 V. After five scans, extra scans did not enhance the current response significantly, so we performed five SWV scans to deposit AuNPs for the rest of the study. The electrodeposition of gold nanoparticles was achieved by SWV, and the position of the peak appeared at around −0.67 V, implying that AuNPs had been deposited on the electrode's surface with the scanning process of SWV, completing the SPE/AuNPs electrode structural modification. High-resolution scanning electron microscopy (SEM) was used to characterize the preparation process of the sensors, and the apparent differences in the surface morphology characterization of different substances could be observed. As shown in Figure 2B-D, the morphological changes over the surface at the working electrode of this sensor were analyzed by characterizing the modification process of the electrode at each stage during the preparation of the SPE/AuNPs/GO-COOH-modified electrode with SPE as the substrate. Figure 2B-D show the SEM images of SPE, SPE/AuNPs, and SPE/AuNPs/GO-COOH, respectively. The surface of the bare electrode ( Figure 2B) was covered with uneven carbon materials without particle distribution; the SPE/AuNPs ( Figure 2C) were derived by depositing AuNPs onto the working electrode surface of the SPE by the SWV method, which showed a significantly enhanced and homogenous particle distribution compared with ( Figure 2B), which is consistent with the previous results on the structure and size of gold nanoparticles [60]. Features such as high surface area, low charge transfer resistance, and fast electron transfer rates resulted in AuNPs with enhanced electron transfer velocity. From ( Figure 2C), GO-COOH was expected to be a thin film morphology and exhibits wrinkles. When AuNPs and GO-COOH were sequentially revised onto the electrodes, the variation in the surface pattern showed that they could be successfully immobilized onto the electrodes. The layer-by-layer modification provided a sensing platform with excellent stability, selectivity, and reproducibility for adaptors, which together constructed an aptamer sensor with good application performances.

Sensing Detection of CRP
The DPV curves of the SPE/AuNPs/GO-COOH aptamer-based sensor for the detection of CRP standard solutions in the concentration range of 0.001 ng/mL~100 ng/mL are shown in Figure 3A. As the concentration of the CRP standard solution progressively increased, the peak DPV current correspondingly went up, obtaining a satisfactory calibration curve in the 0.001 ng/mL~100 ng/mL range. The fitted curves were plotted according to the difference between the peak of the differential pulse current of the detected CRP solutions under various concentrations and the peak of the detected current under the PBS solution (∆I = I − I PBS ). For the logarithm with respect to the concentration of CRP solutions (log 10 C CRP ), as shown in Figure 3B, a current correlation equation is obtained as follows.
∆I CRP = 0.3579 × log 10 C CRP + 1.5516 Linearity ranged from 0.001 ng/mL to 100 ng/mL, with a correlation coefficient of R 2 = 0.9854. The lower limit of determination was 0.001 ng/mL. Biosensors 2022, 12, x FOR PEER REVIEW 6 of 12

Sensing Detection of CRP
The DPV curves of the SPE/AuNPs/GO-COOH aptamer-based sensor for the detection of CRP standard solutions in the concentration range of 0.001 ng/mL ~ 100 ng/mL are shown in Figure 3A. As the concentration of the CRP standard solution progressively increased, the peak DPV current correspondingly went up, obtaining a satisfactory calibration curve in the 0.001 ng/mL ~ 100 ng/mL range. The fitted curves were plotted according to the difference between the peak of the differential pulse current of the detected CRP solutions under various concentrations and the peak of the detected current under the PBS solution (∆ = − ). For the logarithm with respect to the concentration of CRP solutions ( ), as shown in Figure 3B, a current correlation equation is obtained as follows.
= 0.3579 × + 1.5516 Linearity ranged from 0.001 ng/mL to 100 ng/mL, with a correlation coefficient of R 2 = 0.9854. The lower limit of determination was 0.001 ng/mL.

Selectivity, Stability, and Reproducibility Detection of Aptamer Sensors
In this experiment, some possible interfering substances, such as PSA, CA125, PPBP, and BNP, were chosen to evaluate the selectivity of this aptamer sensor. Interference experiments were performed on different electrodes, with one for each piece independently. Selectivity was appraised by recording the signal intensity at 1 ng/mL. DPV was performed for the interfering solutions, with the results shown in Figure 4A. For the current values at −0.4 V, all four interfering solutions, PSA, CA125, PPBP, and BNP, were located below the blank current value, while the DPV scan of the CRP standard solution was greater than the blank current value at −0.4 V. Since the aptamer undergoes conforma-

Selectivity, Stability, and Reproducibility Detection of Aptamer Sensors
In this experiment, some possible interfering substances, such as PSA, CA125, PPBP, and BNP, were chosen to evaluate the selectivity of this aptamer sensor. Interference experiments were performed on different electrodes, with one for each piece independently. Selectivity was appraised by recording the signal intensity at 1 ng/mL. DPV was performed for the interfering solutions, with the results shown in Figure 4A. For the current values at −0.4 V, all four interfering solutions, PSA, CA125, PPBP, and BNP, were located below the blank current value, while the DPV scan of the CRP standard solution was greater than the blank current value at −0.4 V. Since the aptamer undergoes conformational changes upon binding to CRP while the other four interfering proteins are physically adsorbed on the electrode, the current will not be enhanced. Moreover, the current values of the disturbed samples were closer to the blank current values at −0.4 V than those of the CRP. This result also reaffirmed that the sensor was enabled to monitor variations in the current precisely via changes in the aptamer's conformation. The specificity of the developed label-free aptamer sensor was evident from this result. Furthermore, statistical analyses were conducted on the amount of change in the current value at −0.4 V following the DPV scan, which is shown in Figure 4B, where the difference between the interfering substances and PBS currents was negative, and the level of current variation was maintained at a relatively high level. The current response values underwent a significant transformation when the CRP was introduced, with the current becoming positive and the amount of electric current variations being relatively low. These results demonstrated that the aptamer sensor had high selectivity for CRP detections as well as specificity in sophisticated practical scenarios where potential interfering substances were present. An examination of the reproducibility of the SPE/AuNPs/GO-COOH aptamer-based sensor was conducted. Five pieces of aptamer electrodes were arranged in parallel to detect 0.001 ng/mL CRP, while each piece of the electrode was examined repeatedly, as shown in Figure 4D. The current values obtained from the five parallel electrode scans using DPV were compared to the blank control to obtain ΔI. The experiment was repeated three times for each electrode to calculate the standard deviation. In this regard, the five electrodes had close variations in current response ranging from 0.4 to 0.5 μA. This phenomenon represented an acceptable relative deviation of the aptamer sensor during repeated testing with separate electrodes as well as with the same electrode, which collectively demonstrated that the aptamer sensor performed well and was reproducible during CRP detection. The coefficient of variation is Cv = 1%. Therefore, this sensor had the potential to demand practical application scenarios with recurring utilizations. These values were not only based on the choice of the modification material for the electrode's surface but also on the high stability of the DNA aptamer itself and the stability connected to the electrode's surface by the strong bonding of the amino carboxyl group. The reproducibility of the DPV sweeps based on the SPE/AuNPs/GO-COOH aptamer sensors is shown in Figure S2, and the peak currents are essentially close, reflecting that this modified electrode can maintain accurate results via multiple applications. Error analysis plots were obtained by selecting the electrodes on day 1, day 3, day 5, day 7, and day 9 for testing against 1 ng/mL CRP solution (n -3). (D) Reproducibility test plots of five aptamersensing electrodes for multiple assays of 0.001 ng/mL CRP(n -3).

CRP Spike Recovery Experiment
In order to investigate the realistic detection capability of this aptamer sensor, CRP standards were added to the artificial serum and diluted to 5 ng/mL, 10 ng/mL, and 20 ng/mL to simulate real samples. The current values were obtained by the DPV, and the results were substituted into the above linear calibration curve to obtain the recoveries The stability of the aptamer sensor based on SPE/AuNPs/GO-COOH was carried out by keeping the sensing electrode in a refrigerator at 4 • C. Via the experiment, we found that the sensor maintained a period of up to nine days at 4 • C. The sensor was removed and used for the DPV detection of 1 ng/mL CRP on the first, third, fifth, seventh, and ninth days, as shown in Figure 4C. The three replicate experiments in Figure 4C used different separate electrodes. A new electrode was used for each experiment. The slight changes in the current response pointed to the fact that the proposed aptamer sensor retained excellent detection capabilities during long-term storage, demonstrating this sensor's high stability. The stability DPV scan results based on the SPE/AuNPs/GO-COOH aptamer sensor are illustrated in Figure S1, where it can be seen that the peak results were between 6 and 7 µA for the first, third, fifth, seventh, and ninth days, with the current peaks close to each other. The coefficient of variation is C v (C v = σ µ ) = 4%. The superior stability of the ensemble sensor can be confirmed.
An examination of the reproducibility of the SPE/AuNPs/GO-COOH aptamer-based sensor was conducted. Five pieces of aptamer electrodes were arranged in parallel to detect 0.001 ng/mL CRP, while each piece of the electrode was examined repeatedly, as shown in Figure 4D. The current values obtained from the five parallel electrode scans using DPV were compared to the blank control to obtain ∆I. The experiment was repeated three times for each electrode to calculate the standard deviation. In this regard, the five electrodes had close variations in current response ranging from 0.4 to 0.5 µA. This phenomenon represented an acceptable relative deviation of the aptamer sensor during repeated testing with separate electrodes as well as with the same electrode, which collectively demonstrated that the aptamer sensor performed well and was reproducible during CRP detection. The coefficient of variation is C v = 1%. Therefore, this sensor had the potential to demand practical application scenarios with recurring utilizations. These values were not only based on the choice of the modification material for the electrode's surface but also on the high stability of the DNA aptamer itself and the stability connected to the electrode's surface by the strong bonding of the amino carboxyl group. The reproducibility of the DPV sweeps based on the SPE/AuNPs/GO-COOH aptamer sensors is shown in Figure S2, and the peak currents are essentially close, reflecting that this modified electrode can maintain accurate results via multiple applications.

CRP Spike Recovery Experiment
In order to investigate the realistic detection capability of this aptamer sensor, CRP standards were added to the artificial serum and diluted to 5 ng/mL, 10 ng/mL, and 20 ng/mL to simulate real samples. The current values were obtained by the DPV, and the results were substituted into the above linear calibration curve to obtain the recoveries and relative standard deviations, as shown in Table 1. The average recovery of 107. 5% and the relative standard deviations were within 10%. The results showed that the sensor was feasible for the determination of CRPs in real samples. In addition, Table 2 summarizes the comparative analytical performance of the various sensors using the aptamers. We calculated the LOD of this biosensor based on a well-known formula, LOD = 10 × ((3.3 SD-intercept)/slope), which is 2.941 × 10 −4 . It can be seen that the proposed label-free electrochemical sensor offers one of the widest linear ranges compared to other types of sensors, although it does not offer the lowest LOD. This feature gives it an advantage in terms of practical applications.

Conclusions
A markerless aptamer transducer was developed to detect CRPs using amide bonds to immobilize the aptamer on carboxyl-containing graphene oxide, immobilizing the aptamer on the electrode's surface. Gold nanoparticles were assigned to amplify the pulse, and carboxylated graphene oxide was used to immobilize the aptamer. SEM was performed to examine the electrode surface modification process. The DPV method was carried out for the sensing detection of the CRP by using this aptamer sensor, exhibiting a wide linear range (0.001 ng/mL to 100 ng/mL). DNA aptamers with amino groups were bound to GO-COOH via amide bonds and oriented perpendicularly to the electrode's surface. When the aptamer recognized the CRP specifically, the aptamer turned into a rigid structure and was accompanied by a conformational change, that is, bending toward the electrode surface so that the current signal was enhanced. The current signal increased with the accumulation of CRP concentrations within a specific range. Subsequently, the stability and reproducibility of the sensor were studied, and the experimental results proved that the sensor could be stored at 4 • C for more than a week. Moreover, there was a slight variation in the results between different electrodes. In addition, the electrochemical sensor maintained superior characteristics in terms of stability, specificity, and reproducibility. The results indicated that this aptamer sensor could be kept for a certain period and reused repeatedly. The sensor had great potential for complex practical application scenarios where potentially interfering substances were present. Distinct from previous sensors, these label-free aptamer sensors do not require additional electroactive small molecules for electron transport. The aforesaid outcomes reveal that the current variations caused by the aptamer's conformation alteration can work as sensors with excellent performances. This sensor has excellent specificity and also provides an idea in the field of future sensor development.

Conflicts of Interest:
The authors declare no conflict of interest.