Simultaneous Detection of VEGF and CEA by Time-Resolved Chemiluminescence Enzyme-Linked Aptamer Assay.

BACKGROUND: As two important tumor markers, vascular endothelial growth factor (VEGF) and carcinoembryonic antigen (CEA) have a great value for clinical application in the early diagnosis of cancer. Due to the complex composition of biological samples, the results from combined detection of CEA and VEGF are often taken as a comprehensive indicator in order to make an accurate judgment on a disease. However, most of the current methods can only be used to detect the content of one biomarker. Therefore, it is necessary to explore a simple, rapid, low-cost, and highly sensitive method for the simultaneous detection of CEA and VEGF.
METHODS: Based on specific aptamers and magnetic separation, a time-resolved chemiluminescence enzyme-linked aptamer assay was developed for the simultaneous detections of CEA and VEGF in serum samples.
RESULTS: Under the optimal conditions, the linear range of the calibration curve for VEGF was from 0.5 to 80 ng mL-1, and the limit of detection was 0.1 ng mL-1. The linear range of the calibration curve for CEA was 0.5 to 160 ng mL-1, and the limit of detection was 0.1 ng mL-1. The established method was applied to detect VEGF and CEA in serum samples. The results were consistent with those of commercial kits.
CONCLUSION: The method has high sensitivity and can quickly obtain accurate results, which could greatly improve the measurement efficiency, reduce the cost, and also reduce the volume of sample consumed. It can be seen that the method established in this study has important application value and broad application prospect in clinical diagnosis.

Introduction

Vascular endothelial growth factor (VEGF), which is involved in the regeneration of benign blood vessels and tumor blood vessels,1–3 is a key regulator of embryogenesis and vascular physiological development.4 In mammals, the VEGF family generally consists of five members, ie, placenta growth factor (PlGF), VEGF-A, VEGF-B, VEGF-C, and VEGF-D.5–7 There are four different subtypes of VEGF-A, which includes VEGF121, VEGF165, VEGF189, and VEGF206.8 As the main subtype of the VEGF family, VEGF165 may be abnormally expressed in individuals with cancers or diseases. An example is its high expression in the blood or serum of patients with lung cancer and the low expression in patients with psoriasis and Parkinson’s disease.9 Carcinoembryonic antigen (CEA) is one of the most widely used tumor markers in clinical diagnosis,10 whose main function is to perform the adhesion reaction between cancer cells and stromal collagen, and also plays an important role in the growth and metastasis of tumors. The level of CEA in serum is low in healthy population, but an elevated CEA level can be found in a variety of cancers like that of the breast, colon, and lung.11,12 The development of detection techniques for CEA and VEGF, which are two critical tumor markers, will provide a great application value in the early diagnosis of cancer.13,14

Several methods such as fluorescence immunoassay,15,16 surface plasmon resonance,17 chemiluminescence immunoassay,18,19 electrochemical analysis,20 etc., have been established for the detection of VEGF and CEA. However, most of the current methods can only detect the content of one component.21–23 Due to the complex composition of biological samples, it is difficult to make an accurate judgment of a disease just by detecting the expression level of one marker. As a result, in clinical diagnosis, single-target detection often results in high probability of misdiagnosis.24 Therefore, the development of a simultaneous detection method for the detection of multiple targets has become very important.25 The results from the combined detection of CEA and VEGF are often taken as a comprehensive indicator of a certain type of cancer.26,27 In practical application, in order to achieve the simultaneous detection of VEGF and CEA, a variety of commercial kits must be purchased to analyze these two components, respectively, making the analysis process cumbersome, costly, and also requires large sample volume. Consequently, it is in urgent need to explore a simple, rapid, low-cost, and highly sensitive method to simultaneously detect CEA and VEGF, which will not only improve the accuracy and reliability of early diagnosis of lung cancer but also play an extremely important role in improving the survival rate of patients.

Chemiluminescent enzyme-linked immunoassay (CLEIA) has been widely used in analytical chemistry and food safety owing to its wide dynamic range, low background interference, high sensitivity, and specificity.28–30 The traditional CLEIA is used to mark the catalyst or luminescent agent on the antigen or antibody. After a series of immune reactions, the content of the target is finally detected by measuring chemiluminescence (CL) signal.31,32 This method usually requires a large number of antibodies, which are costly and difficult to preserve. In recent years, the nucleic acid aptamer has become an excellent substitute for antibody because of its advantages of low synthesis cost, stable structure, low immunogenicity, and low toxicity.33–35 As a consequence, after carefully considering its unique properties and advantages, aptamer rather than antibody was selected to specifically recognize the target in this work. Using systematic evolution of ligands by exponential enrichment (SELEX) strategies, a variety of VEGF165 and CEA aptamers have been identified by previous studies.36–38 Referring to the existing studies of VEGF165 and CEA aptamers, the aptamer sequences designed in this study are shown in Table 1.39–42 The VEGF165 and CEA aptamers have been proved to bind to their corresponding targets with high affinity, respectively. And the great dissociation constant (Kd) values of the VEGF165 and CEA aptamers were indeed already demonstrated, with a Kd value of 37.9 nM for VEGF165 and 5 nM for CEA.39,43,44 At the same time, on the basis of the aptamers reported in the previous literatures, we added 10 T-base linkers at the 5ʹ, which can effectively reduce steric hindrance and facilitate the binding of aptamers to the target.

Table 1

Oligonucleotides Used in This Experiment

Oligonucleotide	Sequence (5ʹ to 3ʹ)
Complementary DNA probe1 (cDNA1)	Biotin-TTTTTTTTTTACCCACCATA
Complementary DNA probe2 (cDNA2)	Biotin-TTTTTTTTTTAATTGAATAA
VEGF165 aptamer1 (Apt1-HRP)	HRP-TTTTTTTTTTCAATTGGGCCCGTCCGTATGGTGGGT
CEA aptamer2 (Apt2)	Biotin-TTTTTTTTTTATACCAGCTTATTCAATT

Based on specific aptamers and magnetic separation, we successfully developed a time-resolved chemiluminescence enzyme-linked immunoassay for the simultaneous quantitative detection of CEA and VEGF165 in real human serum samples. The method established in this study was further used for the quantitative analysis of VEGF165 and CEA in serum samples and compared with the extensively used commercial enzyme-linked immunosorbent assay (ELISA) kits. The results showed that there was no significant difference between CLEIA and commercial ELISA kits. The proposed method can quickly obtain accurate results and achieve high sensitivity, a wider detection range, and lower detection limits. It can be seen that the method established in this study has important application value and broad application prospect in clinical diagnosis.

Materials and Methods

Reagents and Materials

Human VEGF165 was purchased from Peprotech Corporation (USA). CEA was obtained from Abcam Corporation (USA). Human CEA ELISA kit was acquired from Huaketai Biotechnology Co. Ltd. (Beijing, China). Human VEGF165 ELISA kit was from Miblo Co. Ltd. (Shanghai, China). Alkaline phosphatase-labeled streptavidin (ALP-SA) was purchased from Beyotime Biotechnology Co. Ltd. (Shanghai, China). Tween-20, Biotin, Dimethyl sulfoxide (DMSO) and Tris (hydroxymethyl) aminomethane-hydrochloric acid (Tris-HCl) were obtained from Solarbio Co. Ltd. (Beijing, China). HCl, NaCl, KCl, and NaOH were acquired from Kemiou Chemical Reagent Co. Ltd. (Tianjin, China). Streptavidin modified magnetic beads (MBs, 300 nm) were from Biomag Biotechnology Co. Ltd. (Wuxi, China). Luminol was acquired from Sigma corporation (USA). 3-(2-Spiroadamatane)-4-methoxy-4-(3-phosphoryloxy)phenyl-1,2-dioxetane (AMPPD) was from Huaxia reagent Co. Ltd. (Chengdu, China). 4-Phenylphenol (BIP) was purchased from Aladdin Co. Ltd. (Shanghai, China). Ultrapure water (18.3 MU cm) was obtained from a Milli-Q system (Waters, Milford, MA, USA) and used for all experiments.

All oligonucleotides employed in the work were synthesized and purified by Sangon Biotechnology Corporation (Shanghai, China) and the sequences are listed in Table 1.

Instruments

Centro LB960 chemiluminescence measuring instrument (Berthold, German) was used for chemiluminescence signal recording in this assay. The morphological images of the detection probes were taken by a scanning electron microscope (Hitachi, Japan). Dynamic light scattering (DLS) measurements were realized by Zetasizer Nano-zs 90 particle size and zeta potential analyzer (Malvern, England).

Solution Preparation

Chemiluminescence substrate A: 1.4 mL of luminol and 28.6 µL of 4-Phenylphenol (BIP) were measured. Then, 0.1 mol L−1 Tris-HCl buffer (pH: 8.5) was used to achieve a final volume of 10 mL.

Chemiluminescence substrate B: 25.5 µL of H2O2 (30%) was diluted with Milli-Q water to a volume of 25 mL.

Chemiluminescence substrate C: 200 µL of AMPPD was measured and diluted with 0.1 mol L−1 Tris-HCl buffer (pH: 8.5) to a concentration of 1 mg mL−1.

Chemiluminescence substrate D: Chemiluminescence substrate B and chemiluminescence substrate C were mixed in a volume ratio of 1:1.

Principle and Procedure of CLEIA

The principle of CLEIA is shown in Scheme 1.First, the complementary DNA (cDNA1) that has been biotinylated, was modified on streptavidin-modified magnetic beads (MBs) to synthesize the cDNA1-MBs complex. After the addition of the horseradish peroxidase (HRP)-Apt1 (Apt1-HRP) complex and also the VEGF165 detection probe, cDNA1-MBs@Apt1-HRP was formed from the hybridization of the cDNA1-MBs complex with the Apt1-HRP complex. Then, another biotinylated complementary DNA (cDNA2) was modified on the MBs using the same method as described above. After, the addition of the alkaline phosphatase (ALP)-Apt2 (Apt2-ALP) complex and the CEA detection probe led to the synthesis of cDNA2-MBs@Apt2-ALP under the action of base complementation. Then, the two detection probes were mixed in the volume ratio of 1:1 to form the mixed probe. In the presence of VEGF165 and CEA, the two probes specifically bound to the target compounds, to free ALP and HRP labeled on the magnetic beads. Finally, by adding the chemiluminescence substrate, the chemiluminescence system of the Luminol and H2O2 was catalyzed by the remaining HRP on the MBs, while the chemiluminescence system of 3-(2-Spiroadamatane)-4-methoxy-4-(3-phosphoryloxy) phenyl-1,2-dioxetane (AMPPD) was catalyzed by the remaining ALP on the MBs. To achieve the simultaneous detections of CEA and VEGF, chemiluminescence signals were, respectively, recorded at different times according to the kinetic characteristics of the different chemiluminescence reactions catalyzed by HRP and ALP.

Scheme 1

Schematic illustration of the simultaneous detection of VEGF165 and CEA by time-resolved chemiluminescence enzyme aptamer method. (A) cDNA1 and cDNA2 immobilization on MBs and coupling with Apt1-HRP and Apt2-ALP to obtain detection probes respectively. (B) Samples were incubated with the mixed probe solution and Chemiluminescence signals were respectively recorded at different times.

Preparation of cDNA1-MBs@Apt1-HRP

cDNA1 solution (400 nmol L−1) was heated at 95°C for 3 min and then quickly placed at 4°C to cool down to room temperature. After that, 300 µL streptavidin-coated magnetic beads were added to a centrifuge tube and washed twice by Tris-HCl buffer solution with Tween-20 (TBST). Then, excess supernatant was removed by magnetic separation. Next, 300 µL of the prepared cDNA1 suspension (400 nmol L−1) was vortexed with the 300 µL streptavidin-coated magnetic beads at room temperature for 30 min and the mixed solution was washed thrice with TBST. A magnetic separation was performed to remove the supernatant. Then, Apt1-HRP (60 nmol L−1) was added to the centrifuge tube for another 50 min vortexing and the VEGF165 detection probe was obtained after magnetic separation of the supernatant. Finally, cDNA1-MBs@Apt1-HRP was kept in 600 μL of Tris-HCl buffer solution (TBS) at 4°C for subsequent experiments.

Preparation of cDNA2-MBs@Apt2-ALP

The cDNA2 solution (400 nmol L−1) was heated at 95°C for 3 min, and then placed at 4°C to slowly cool to room temperature. Apt2 (100 nmol L−1) and ALP-SA were vortexed at room temperature for 20 min to form Apt2-ALP complex. Three hundred microliters streptavidin-coated magnetic beads were measured into a centrifuge tube and washed twice with TBST. The supernatant was removed by magnetic separation. Next, 300 μL of the prepared cDNA2 suspension (400 nmol L−1) was vortexed with 300 μL of magnetic beads at room temperature for 30 min. A magnetic separation was performed to remove the supernatant and then washed twice with TBST. Then, to obtain the CEA detection probe, the cDNA2-MBs was washed thrice with TBST and vortexed with Apt2-ALP for another 50 min. Finally, after the supernatant had been removed by magnetic separation, cDNA2-MBs@Apt2-ALP was stored in the same way as mentioned above.

Simultaneous Detection of VEGF165 and CEA

Thirty microliters of the mixed probe solution, which was obtained by mixing the prepared CEA detection probe and VEGF165 detection probe in a volume of 1:1, was added to each well of a 96-well polystyrene microtiter plate, and then the supernatant was removed by magnetic separation. The standard solution (100 μL) of VEGF165 and CEA prepared with different concentrations was measured into each well and incubated at 25°C for 30 min. After that, the mixed probe was washed thrice with TBST and the supernatant was removed by magnetic separation. Lastly, the chemiluminescence substrate A (100 μL) and chemiluminescence substrate D (100 μL) were added into the microplate, and the CL signal in each well was recorded at 1.0 s and 20 min, respectively, using the CL immunoassay analyzer.

Collection and Detection of Serum Samples

Fasting peripheral blood was collected with a serum separator tube. The blood samples were bathed at 37°C for 30 min and centrifuged at 3000 rpm for 5 min. Then, serum was collected and CEA and VEGF165 in the serum samples were detected according to the established method developed in this work and by commercial ELISA kits. All blood samples were obtained from the First Affiliated Hospital of Zhengzhou University, approved by Life-Science Ethics Review Committee of Zhengzhou University. All blood donors provided informed consent, in accordance with the Declaration of Helsinki.

Results

Characteristics of cDNA1-MBs@Apt1-HRP

Zeta potential and DLS were performed to confirm the conjugation of cDNA1and MBs. As shown in and , the hydrodynamic diameter of MBs was estimated to be 345.3 nm after modification with cDNA1, but only 320.3 nm before modification. The zeta potential changed from −4.16 mV to −16.3 mV, indicating the successful formation of the negative cDNA1 polymerization shell on the surface of MBs, and this led to an increase in electrostatic repulsion between particles and a significant improvement in the stability of MBs (). The results confirmed that the cDNA1-MBs were successfully prepared. In addition, the morphology of the prepared cDNA1-MBs@Apt1-HRP complex was characterized by scanning electron microscopy (SEM). The result showed that MBs were spherical, with a flat surface and their diameter were about 300 nm (Figure 1A). Due to the modification of Apt1-HRP on the MBs, the margin of the cDNA1-MBs@Apt1-HRP complex was not clear (Figure 1B). This primarily indicated that the cDNA1-MBs@Apt1-HRP was successfully prepared.

Figure 1

Scanning electron micrographs of (A) MBs, (B) cDNA1-MBs@Apt1-HRP, (Scale bar was 300 nm) (C) MBs and (D) cDNA2-MBs@Apt2-ALP (Scale bar was 500 nm).

The catalytic activity of HRP in cDNA1-MBs@Apt1-HRP was investigated by mixing different contents of cDNA1-MBs@Apt1-HRP with chemiluminescent substrate (Figure 2A). The chemiluminescence intensity was enhanced with an increase in the dosage of cDNA1-MBs@Apt1-HRP, which indicated that HRP maintained a good catalytic activity in the complex, and that cDNA1-MBs@Apt1-HRP could be used for the detection of VEGF165.

Figure 2

Enzymatic catalytic activity of (A) cDNA1-MBs@Apt1-HRP and (B) cDNA2-MBs@Apt2-ALP.

Characteristics of cDNA2-MBs@Apt2-ALP

After the MBs were modified with cDNA2, the hydrodynamic diameter of the formed cDNA2-MBs showed a significant enhancement from 331.2 nm to 357.9 nm ( and ) and the zeta potential changed from −4.16 mV to −12 mV (). Therefore, both results confirmed that the cDNA2 and MBs were successfully combined. The results from the scanning electron microscopy of MBs and cDNA2-MBs@Apt2-ALP are shown in Figure 1C and D, respectively. Both MBs and cDNA2-MBs@Apt2-ALP were spherical with their diameters around 300 nm. Compared with MBs, the surface of cDNA2-MBs@Apt2-ALP was covered with a layer of material, inferring that the modified Apt2-ALP may be on the surface of the magnetic beads, which indicated that the nanoparticles of cDNA2-MBs@Apt2-ALP were successfully prepared.

The catalytic activity of ALP in cDNA2-MBs@Apt2-ALP was investigated by mixing different amounts of cDNA2-MBs@Apt2-ALP with chemiluminescence substrate and the changes in chemiluminescence intensity were observed (Figure 2B). As the amount of cDNA2-MBs@Apt2-ALP increased, the chemiluminescence intensity and the relative chemiluminescence units (RLU) continued to rise, suggesting that the prepared CEA detection probe maintained a good catalytic activity of ALP and could be applied in subsequent experiments.

Experimental Conditions Optimization

In order to achieve a better sensing effect, the following parameters were optimized in this assay: Concentration of the Apt1-HRP, dilution ratio of the ALP-SA, concentration of the Apt2, reaction time between aptamers and complementary DNA, and reaction time between detection probes and samples, concentration of the luminol, H2O2, and AMPPD.

As displayed in Figure 3A, with an increase in the concentration of Apt1-HRP, RLU0-RLU increased at the beginning and reached a maximum at 60 nmol L−1. Therefore, 60 nmol L−1 of Apt1-HRP was selected as the optimal concentration. Figure 3B indicated that with a decrease in the dilution rate of ALP-SA from 1:100 to 1:200, the RLU0-RLU increased slightly, and when the dilution ratio of the ALP-SA was lower than 1:200, the signal observably declined. Therefore, we set the dilution ratio of the ALP-SA as 1:200. The results (shown in Figure 3C) also demonstrated that the optimal concentration of the Apt2 was 100 nmol L−1.

Figure 3

Experimental conditions optimization. (A) Optimization of the concentration of the Apt1-HRP. (B) Optimization of the dilution ratio of the ALP-SA. Optimization of the concentration of the the Apt2 (C), luminol (D), H2O2 (E), and AMPPD (F).

Meanwhile, the reaction times between aptamers and complementary DNA, and also between the detection probes and samples were optimized. As shown in , signal intensity at the beginning, increased gradually with an increasing reaction time, but after 50 min and 30 min, respectively, RLU0-RLU decreased steadily. Therefore, the optimal reaction times between aptamers and complementary DNA, detection probes and samples were 50 min and 30 min, respectively.

Because the substrates of the chemiluminescence and the concentration of the luminol, H2O2, and AMPPD can effectively affect the intensity of chemiluminescence, we investigated the optimal concentration of luminol, H2O2, and AMPPD. As shown in Figure 3D–F, the RLU of luminol, H2O2, and AMPPD increased sharply with the concentration and tended to level off after 1.4 mmol L−1, 5 mmol L−1, and 0.5 mg mL−1, respectively. Therefore, 1.4 mmol L−1, 5 mmol L−1, and 0.5 mg mL−1 were chosen as the optimal concentration of luminol, H2O2, and AMPPD, respectively.

Kinetic Characteristics of Different Chemiluminescent Systems

The chemiluminescence kinetic characteristics of the two systems, ALP-AMPPD and HRP-Luminol-H2O2, were investigated (Figure 4). The kinetic characteristics of the HRP-Luminol-H2O2 system are shown in Figure 4A. The system produced a flash-type chemiluminescence, the intensity of which was high in the first 10 s of the reaction and decayed rapidly thereafter. Then, we chose 1.0 s as the time window for detecting HRP-Luminol-H2O2 system. As shown in Figure 4B, the ALP-AMPPD system produced a glow-type chemiluminescence. The chemiluminescence intensity was low at the beginning of the reaction, then increased slowly, reaching the maximum luminous intensity at about 20 min. It then maintained a plateau for a period, and then decreased slowly thereafter. Therefore, 20 min was chosen as the time window for detecting the ALP-AMPPD system.

Figure 4

Kinetics curve of (A) HRP-Luminol-H2O2 and (B) ALP-AMPPD chemiluminescent systems.

Analytical Performance of the Assay

A time-resolved CLEIA for the simultaneous quantitative detection of CEA and VEGF165 was established under the optimal conditions. Calibration curves were obtained by plotting chemiluminescence RLU values against different concentrations (0.5, 1, 5, 10, 20, 40, 80, 160 ng mL−1) of standard VEGF165 and CEA sample. As observed from Figure 5A, the CL intensity was linear with lgCVEGF165 [Y=0.2603X+4.3684 (Y and X, respectively, denote the lg(RLU0-RLU) and lgCVEGF165, r=0.9882] in the range of 0.5 ng mL−1 and 80 ng mL−1, with the limit of detection (LOD) of 0.1 ng mL−1. Figure 5B also showed that there was a linear intensity when the concentration ranged from 0.5 ng mL−1 to 160 ng mL−1 with a LOD of 0.1 ng mL−1. The linear equation was Y=5032.03X+27732.14 (Y and X, respectively, denote the (RLU0-RLU) and lgCCEA, r=0.9893). The components of serum samples are complex and often contain both VEGF and CEA. In order to evaluate whether this method can be used in actual sample detection, we verified the specificity of the developed method for VEGF165 and CEA detection by measuring the CL signal response of three targets, CEA (50 ng mL−1), VEGF165 (50 ng mL−1) and CEA (50 ng mL−1)+VEGF165 (50 ng mL−1), at 1.0 s and 20 min, respectively. It can be seen that the VEGF165 group and the CEA+VEGF165 group had obvious response at 1.0 s but the signal value of the CEA group was very low (Figure 5C). Significant signal values were observed in the CEA group and the mixed group at 20 min but the VEGF165 group hardly responded to the ALP system (Figure 5D). This means the detection probes had no specific reaction to other target object, indicating that this method had good specificity and could achieve simultaneous detection of VEGF and CEA in samples.

Figure 5

Calibration curves for (A) VEGF165 and (B) CEA determination. The concentrations of VEGF165 and CEA are both 0.5, 1, 5, 10, 20, 40, 80, 160 ng mL−1, respectively. Chemiluminescence signal detected at (C) 1.0 s and (D) 20 min (The concentrations of VEGF165 and CEA are both 50 ng mL−1). The detection results of (E) VEGF165 and CEA (F) in serum samples.

Application in Human Serum Samples

To demonstrate the application of the proposed CLEIA in biological samples, six human serum samples were employed to detect the concentrations of VEGF165 and CEA under the optimum conditions and the results were compared to that of the extensively used ELISA method. The results are summarized in Figure 5 (E-F) and Table 2. Paired sample t test was used to statistically analyze the test results. Furthermore, the results of CEA (t = 0.872, P = 0.423) and VEGF165 (t = −1.118, P = 0.314) in serum samples measured by the new chemiluminescence method were not statistically different from those of commercial ELISA kit, suggesting that the method could be applied to detect VEGF165 and CEA content in serum.

Table 2

Results of Serum Samples Tested with the CLEIA and ELISA Kit

Samples	CCEA (ng mL−1)		CVEGF(ng mL−1)
	CLEIA	ELISA	CLEIA	ELISA
S1	1.70	1.76	1.13	0.83
S2	1.17	1.69	3.45	3.50
S3	1.72	1.95	2.02	2.30
S4	5.51	5.36	0.79	0.69
S5	1.27	1.53	2.29	2.11
S6	3.59	3.30	6.89	6.38

Conclusion

In this work, we have developed a novel and sensitive time-resolved chemiluminescence enzyme-linked immunoassay for the simultaneous quantitative detection of CEA and VEGF165 in human serum samples, based on the different kinetics of chemiluminescence reactions catalyzed by HRP and ALP. The proposed CLEIA revealed wide linear responses (VEGF165: 0.5 ng mL−1-80 ng mL−1, CEA: 0.5 ng mL−1-160 ng mL−1) toward VEGF165 and CEA with low LODs (VEGF165: 0.1 ng mL−1, CEA: 0.1 ng mL−1). More importantly, the proposed method was successfully used for the detection of VEGF165 and CEA in various actual samples and the experimental results were consistent with that of the ELISA kit, indicating that the method had high accuracy. In addition, the assay has many advantages and innovations. First, magnetic beads were selected as solid phase carrier in this study, which, on one hand, achieved rapid separation of reactants from solution, and, on the other hand, enabled biomolecules to be well fixed. Secondly, aptamers with low cost, stable structure, and easy to modify were used to replace the antibodies usually used in traditional CLEIA so as to specifically recognize the target. Meanwhile, the simultaneous detections of CEA and VEGF in serum samples were realized by using the different kinetic characteristics of glow and flash chemiluminescence reaction systems, which did not only save samples but also improved the analysis efficiency. However, there are still several points that need to be improved in the experiment. The limit of detection can be further reduced and also, the sensitivity of multi-component analysis can be improved by using magnetic beads of different materials, by modifying different groups on the magnetic beads, or by blocking the surface of the magnetic beads with some surfactants, etc. Overall, the proposed approach can be used for high-throughput screening and has potential applications in early diagnosis of cancer.