A serological method to simultaneously detect antibodies against infectious laryngotracheitis virus (ILTV) and infectious bronchitis virus (IBV) is imperative for the differential diagnosis and evaluation of antibodies titers after vaccination.
Method
The microspheres coated with purified recombinant glycoprotein D (gD) of ILTV or nucleocapsid (N) protein of IBV were incubated with serum samples. The simultaneous quantification of ILTV and IBV antibodies were achieved through the interrogation of microspheres by Luminex 200 detection system. .
Results
This xMAP detection demonstrated no nonspecific reactions with avian influenza virus (AIV), avian leukosis virus (ALV), newcastle disease virus (NDV), and Marek’s disease virus (MDV). The results also demonstrated that the xMAP assay was four times more sensitive than the enzyme-linked immunosorbent assay (ELISA) for ILTV detection and two times more sensitive for IBV detection. A total of 90 chicken serum samples from a chicken farm were tested by xMAP and ELISA assays. The results showed that the coincidence rates were 84.44 and 100% for ILTV and IBV detection, respectively.
Conclusion
This study exhibited an opportunity for the differential diagnosis through simultaneous detection of multiplex antibodies in serum and can be used for the multiplex antibodies evaluation after vaccination.
Hinweise
Huanan Wang, Feng Cong and Jianchi Guan contributed equally to this work.
Abkürzungen
AIV
Avian influenza virus
ALV
Svian leukosis virus
IB
Infectious bronchitis
ILT
Infectious laryngotracheitis
MDV
Marek’s disease virus
NDV
Newcastle disease virus
Background
Infectious laryngotracheitis (ILT) and infectious bronchitis (IB) are common respiratory diseases in poultry and are currently present at epidemic levels around the world, including in China, the United States, and India. Because ILT and IB have high incidence and infectivity in chickens at different ages (in days), they have caused huge economic losses to the poultry industry. Both diseases have similar clinical symptoms and pathological changes, leading to significant difficulties in clinical differential diagnosis, especially in cases of mixed infection [1, 2]. In addition, the use of vaccines is the main approach to control of the economically important poultry viral respiratory diseases, such as infectious laryngotracheitis and infectious bronchitis [3]. Therefore, it is important to establish a method to simultaneously detect ILTV and IBV antibodies for the differential diagnosis and immune response evaluation after vaccination.
Infectious laryngotracheitis virus (ILTV), an alphaherpes virus, possesses at least 10 envelope glycoprotein, two main proteins of which are the glycoprotein B (gB) and gD, respectively, which are highly conserved herpesvirus structural glycoproteins [4]. The gD of herpes virus has an important role by binding to the host receptors [1, 5]. The gD protein has been demonstrated to be a candidate antigen for recombinant vaccines [6, 7]. The infectious bronchitis virus (IBV) genome encodes four major structural proteins: the spike glycoprotein (S), the membrane glycoprotein (M), the nucleocapsid (N) protein, and the envelope or small membrane protein (E) [8]. The N protein is thought to be an appropriate diagnostic reagent for antibody detection [9]. In this study, gD and N proteins were selected as antigen molecules for the diagnosis of ILT and IB.
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At present, the methods used for the diagnosis and effect evaluation of vaccine immunity of avian respiratory diseases primarily include virology detection, serological detection, and molecular biological detection. Traditional methods, such as virus isolation, animal inoculation experiments, ELISA, hemagglutination (HA), and hemagglutination inhibition (HI) assays are characterized by complex procedures and long periods of time required for diagnosis. Despite its unique, sensitive, simple features and rapidity, polymerase chain reaction (PCR) is unable to meet the requirements for high-flux quarantine and is not favorable for the urgent screening of bulk samples. Therefore, it is imperative to establish a new technology for the effect evaluation of vaccine immunity and the rapid differentiation or correct identification of important avian respiratory diseases.
A new high-flux detection technology, flexible xMAP (x = Unknown, MAP = Multi-Analyte Profiling) assay, uses variously colored polystyrene beads that is carboxylated to allow covalent coupling of protein. Conjugated beads can be used to capture specific antibodies in serum, and a fluorescent secondary antibody is incubated to bind to the captured serum antibodies. A red laser is used to determine the color of the bead and a green laser to detect fluorescence intensity of bound secondary antibodies through the Luminex 200 detection system [10]. This method is applicable for the simultaneous and rapid detection of multiplex pathogen,s antibodies, with simple operation and high accuracy that are superior to conventional methods. In this study, a method employing Luminex xMAP technology to simultaneously detect ILTV and IBV antibodies in serum was established, optimized and used for the differential diagnosis of IBV and ILTV. This assay can also be used to simultaneous monitoring of IBV and ILTV antibody levels for the evaluation of immunity after vaccination.
Results
Establishment of singleplex xMAP detection for ILTV and IBV
A singleplex xMAP for ILTV was established by testing six concentrations of the ILTV gD envelope protein (2.5 μg, 5 μg, 10 μg, 20 μg, 40 μg, and 80 μg per 5 × 105 magbeads), seen in Table 1. The P/N value is the ratio of MFI (Median Fluorescence Intensity) value between the positive sample and negative sample. The optimal conjugation protein concentration was 2.5 μg per 5 × 105 magbeads for singleplex xMAP detection of ILTV. The mean P/N value under the condition was 10.18.
Table 1
P/N values for ILTV antibody xMAP detection
Serum dilution
Coating antigen dilutions (μg/5 × 105 beads)
Average
2.5
5
10
20
40
80
1:25
16.84
8.41
11.18
10.15
6.87
3.22
9.44
1:50
10.47
6.26
8.54
7.39
4.43
2.70
6.63
1:100
8.30
5.07
5.84
6.11
4.07
2.69
5.35
1:200
5.14
3.88
4.83
4.55
2.97
2.21
3.93
Average
10.18
5.90
7.60
7.05
4.59
2.70
A singleplex xMAP for IBV was established by testing six concentrations of the IBV N envelope protein (3 μg, 6 μg, 12 μg, 24 μg, 48 μg, and 96 μg per 5 × 105 magbeads), seen in Table 2. The P/N value is the ratio of MFI value between the positive sample and negative sample. The optimal conjugation protein concentration was 12 μg per 5 × 105 magbeads for singleplex xMAP detection of IBV. The mean P/N value under the condition was 17.16.
Table 2
P/N values for IBV antibody xMAP detection
Serum dilution
Coating antigen dilutions (μg/5 × 105 beads)
Average
3
6
12
24
48
96
1:50
13.16
14.67
17.53
14.75
16.30
13.30
14.95
1:100
12.23
18.15
16.44
16.07
18.83
17.66
16.57
1:200
13.41
17.07
17.73
14.63
15.16
17.52
15.92
1:400
11.59
14.72
16.93
11.88
12.30
14.90
13.72
Average
12.60
16.15
17.16
14.33
15.65
15.85
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Establishment of duplex xMAP for simultaneous detection of ILTV and IBV
Based on the results in Tables 1 and 2, the optimum serum dilution ratio for ILTV and IBV were 1:25 and 1:100, respectively. When singleplex xMAP assay was performed. To determine the optimal serum dilition ration for simultaneous detection of ILTV and IBV, a serial serum dilutions from the range of 1:25 to 1:200 were prepared and were incubated with ILTV and IBV antigen conjugated microspheres. From the P/N values showed in Fig. 1, it is obvious that the optimal serum dilution ratio for duplex xMAP assay was 1:100.
Fig. 1
Determination of optimal serum dilution ratio for duplex xMAP assay for ILTV and IBV antibodies. ILTV- and IBV-positive and negative sera were diluted at the range from 1:25 to 1:200. MFI Values were obtained after the interrogation of microspheres coated with proteins of ILTV or IBV using Luminex 200 detection system. The P/N values were used to determine the optimal dilution ratio at 1:100 for duplex detection of ILTV and IBV antibodies
×
Determination of threshold
The threshold is considered as the sum of the average plus three times of standard deviation, which is also named cut-off value. To determine the threshold of xMAP assay for ILTV and IBV, 32 special pathogen free chicken serum samples at 1:100 dilution were used to obtain the average MFI value and standard deviation. From the Table 3, it showed that the threshold of ILTV and IBV detection were 154.95 and 266.75, respectively.
Table 3
Threshold of ILTV and IBV antibodies detection
ILTV MFI value
IBV MFI value
SPF chicken negative sera
113
101.5
105
93
207.5
198.5
196.5
184
105
97
110
134
192.5
197
222.5
258
68
68
70
74.5
127
132
134.5
149.5
58
67
68
72
116.5
134
135
141.5
106
115.5
75
90
183
152.5
148
134
126
98
104.5
111
140
158.5
164
116
89.5
86
77
86
132.5
150
153
144
48.5
59.5
43
70
119
95
132
87
Average
87.17
154.22
Standard deviation
22.59
37.51
Threshold
154.95
266.75
Specificity of xMAP assay for ILTV and IBV
The results in Figs. 2 and 3 demonstrated that xMAP duplex assay for ILTV and IBV has a high specificity since there were no cross-reactions with serum positive for other avian diseases, such as avian influenza virus (AIV), avian leukosis virus (ALV), newcastle disease virus (NDV), and Marek’s disease virus (MDV).
Fig. 2
Specificity for duplex xMAP assays for ILTV antibody detection. Positive sera for ILTV, IBV, ALV, NDV, MDV, AIV(H5, H7 and H9) were used to determine the specificity of duplex xMAP assay. The specific detection results showed that there were no cross-reactions with positive sera for other avian diseases
Fig. 3
Specificity for duplex xMAP assays for IBV antibody detection. Positive sera for ILTV, IBV, ALV, NDV, MDV, AIV were used to determine the specificity of duplex xMAP assay. The specific detection results showed that there were no cross-reactions with positive sera for other avian diseases
×
×
Repeatability of xMAP assay for ILTV and IBV
Intra-assay repeatability experiments showed that the coefficient of variation (CV) was 5.09% for ILTV and 8.05% for IBV. Inter-assay repeatability experiments showed that the CV was 8.11% for ILTV and 9.48% for IBV. All CVs were less than 10%, indicating that the method has high repeatability. The results were shown in Tables 4 and 5.
Table 4
Repeatability experiment of ILTV antibody detection
ILTV detection
Samples
MFI
Average
Standard deviation
Intra Cv
Repeat Experiment 1
repeat 1
1145.5
1208.33
61.5433
5.09%
repeat 2
1268.5
repeat 3
1211
Negative
111.33
/
/
/
Repeat Experiment 2
repeat 1
1127.5
1143.00
55.8860
4.89%
repeat 2
1205
repeat 3
1096.5
Negative
84.33
/
/
/
Repeat Experiment 3
repeat 1
1046
1028.00
16.3707
1.59%
repeat 2
1024
repeat 3
1014
Negative
75.33
/
/
/
Inter MFI Average
1126.44
Standard deviation
91.30
Inter Cv
8.11%
Table 5
Repeatability experiment of IBV antibody detection
IBV
Samples
MFI
Average
Standard deviation
Intra Cv
Repeat Experiment 1
repeat 1
2096.5
2177.67
75.2103
3.45%
repeat 2
2245
repeat 3
2191.5
Negative
177
/
/
/
Repeat Experiment 2
repeat 1
1770
1884.50
151.6583
8.05%
repeat 2
2056.5
repeat 3
1827
Negative
141.33
/
/
/
Repeat Experiment 3
repeat 1
1842
1832.00
106.3532
5.81%
repeat 2
1721
repeat 3
1933
Negative
127
/
/
/
Inter MFI Average
1964.72
Standard deviation
186.27
Inter Cv
9.48%
Comparison of xMAP assay with ELISA using clinical samples
The sensitivities of xMAP and ELISA were compared using 1:50 to 1:3200 ILTV-positive sera and 1:100 to 1:6400 IBV-positive sera. The results showed that xMAP detected ILTV-positive sera at 1:1600 and IBV-positive sera at 1:3200, while ELISA detected ILTV-positive sera at 1:400 and IBV-positive sera at 1:1600 (see Table 6).
Table 6
Comparison of xMAP and ELISA sensitivity
ILTV detection
IBV detection
Dilution
ELISA S/P
xMAP MFI
Dilution
ELISA S/P
xMAP MFI
1:50
2.9178
+
2205
+
1:100
1.5430
+
2732.5
+
1:100
2.0395
+
1725.5
+
1:200
1.0445
+
2103
+
1:200
1.3866
+
1235
+
1:400
0.6319
+
1960
+
1:400
0.8119
+
806.5
+
1:800
0.3961
+
1161
+
1:800
0.4607
–
486.5
+
1:1600
0.2301
+
779.5
+
1:1600
0.2536
–
277.5
+
1:3200
0.1372
–
428.5
+
1:3200
0.1262
–
145
–
1:6400
0.0828
–
226
–
Cut-off
0.5000
154.95
Cut-off
0.2000
266.75
To compare duplex xMAP assay with ELISA for ILTV/IBV detection, 90 chicken serum samples from a chicken farm in Huizhou, China were used and the results are shown in Table 7. For ILTV, xMAP detected 76 positive cases whereas ELISA detected 69 positive cases; among them, 67 samples were detected positive by xMAP assay and ELISA. All 90 samples were detected as positive for IBV by both methods.
Table 7
Comparison of xMAP and ELISA for ILTV and IBV antibody detection
Detection method
Positive sample
Negative samples
Total coincidence
ILTV
xMAP
76 (67a)
14 (9a)
84.44%
ELISA
69
21
IBV
xMAP
90 (90a)
0 (0a)
100.00%
ELISA
90
0
aIdentical number of detection results for xMAP and ELISA
Discussion
IB, an acute infectious disease characterized by acute watery diarrhea, kidney necrosis, and high mortality, is caused by IBV. Thus far, IB has resulted in economic losses to the poultry industry in various countries [8, 11]. IBV infects chickens at different ages. Chicks infected with IBV are characterized by noisy breathing, panting, sneezing, nasal fluid, and other symptoms; furthermore, laying hens exhibit significantly reduced egg production, broilers exhibits low growth and bad meat quality, and breeding hens exhibit significantly reduced breeding efficiency [12]. ILT is an acute, contact respiratory infectious disease in chickens. Chickens infected with ILT are characterized by nasal fluid, conjunctivitis, panting, coughing, and the production of bloody mucus, as well as swelling, erosion, necrosis, and extensive bleeding in the throat after analysis; laying hens exhibit reduced egg production or even no production, as well as poor egg quality [13]. The disease spreads rapidly and has a wide distribution. The high mortality rate (> 70%) results in huge economic losses to the poultry industry [4]. Given the similar clinical symptoms between ILT and IB, the development of diagnoses for both diseases is significant.
This is the first case report of differential diagnosis of ILTV and IBV with xMAP assay. Luminex xMAP assay is an emerging technology that uses small carboxylated polystyrene microspheres that are internally dyed with both a red and an infrared fluorophore [14]. By changing the ratio of the two fluorophores, it is possible to distinguish up to 100 different color-coded microsphere sets, and each microsphere set may be coupled with a different biological probe. The microspheres are detected and characterized by a dedicated flow cytometer [15]. The Luminex xMAP technology is useful for many different applications. One review describes the use of this technology for the multiplex detection of viral, bacterial, parasitic, and fungal agents using the microsphere-based multiplex nucleic acid assay (MBMNA) and the microsphere-based multiplex immunoassay (MBMI) [16]. MBMIs are typically biochemical tests that allow the detection or measurement of the concentration of a protein in a solution via an antibody or immunoglobulin [17]. MBMIs are often used in the diagnosis of various pathogens, such as human papillomavirus and human cytomegalovirus, to detect antibodies in serum samples [18‐20]. The advantages of this technology are its simple operation, high accuracy, and reduction in the number required experiments and samples because a single test simultaneously identifies a variety of pathogens.
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This study describes the establishment and validation of single xMAP and duplex xMAP assays. First, to achieve effective and rapid clinical diagnosis of ILT and IBV, single xMAPs were established for the separate diagnosis of these two diseases after screening to identify the best concentrations of microsphere antigens for ILTV gD and IBV N (2.5 μg/5 × 105 magbeads and and 12 μg/5 × 105 magbeads, respectively), with an optimal serum dilution of 1:100. However, it is not ideal to diagnose only one type of pathogen antibody because more than one disease often affects the respiratory tract in poultry. Given the similar clinical symptoms of ILT and IBV, the differential diagnosis of these two pathogens with two single xMAP assays using one sample wastes time and energy. To achieve the rapid differential diagnosis of clinical samples, it is necessary to establish a duplex xMAP. In addition to ILTV and IBV, AIV and NDV are also common respiratory viruses for poultry. These four diseases have high incidences, and it is difficult to make a differential diagnosis based on clinical symptoms, which are all similar. Figures 2 and 3 showed that our xMAP methods was able to simultaneously detect the antibodies to ILTV or IBV in the sera and had the high specificity. A duplex xMAP can quickly identify ILTV and IBV infection, but it does not indicate possible infection by AIV and NDV. Therefore, based on this study, we propose that quadruplex xMAP should be established in the future for the detection of ILTV, IBV, AIV and NDV as a fast and effective differentiation tool for these four viruses.
Since ELISA was established to detect ILTV antibodies in 1982 [21], it has demonstrated strong advantages, as well as higher sensitivity than virus neutralization tests (VNT), making it widely applicable. ELISA antibody detection of IBV is also feasible at earlier time points [22, 23] and is currently broadly applied in the poultry industry. Single-analyte ELISA does not support the detection of multiple specific antibody responses simultaneously for a single serum sample [24] and possesses other disadvantages, such as the requirement for a relatively large amount of sample, negligible nonspecific binding, and increased background. However, with the development of the poultry industry, requirements dictate that many samples must be detected simultaneously; thus, a new detection method for diagnosis with ILTV and IBV is significant. Luminex xMAP assay represents an alternative for commonly employed indirect tests such as ELISA. The conversion of an ELISA to the xMAP format is uncomplicated, efficient and cost-saving, producing an assay with superior dynamic range and sensitivity [25]. MBMI represents increased sensitivity and the potential to quantify antibodies, antigens, and other substances (e.g., hormones, cytokines, and tumor markers), unlike conventional ELISA tests [26]. Luminex xMAP has also been compared with a western blot assay for antibody detection [27]. The results obtained from both methods showed that the sensitivity of xMAP was 82.7%, while the western blot assay sensitivity was 74.7%. Therefore, xMAP may be more efficient and precise than western blots for the diagnosis of diseases. Although ELISA provides relatively accurate results and has been used for many years, this study demonstrates that xMAP is much more sensitive than ELISA for the diagnosis of ILT, as indicated by the results presented in Table 6. In addition, xMAP may be used for the rapid diagnosis of many samples, saving time and effort. The results presented in Table 7, demonstrate that xMAP is highly accurate, with similar detection results to those obtained by ELISA in positive clinical samples; thus, xMAP is able to be widely applicable.
Conclusions
This study describes how to determine the optimal conditions for establishing duplex xMAP assay based on the singleplex xMAP result, thus providing a reference for establishing multiplex xMAP assay for simultaneous detection of animal pathogen,s.antibodies.
Methods
Antigens and sera
The antigens used for ILTV were a recombinant gD [28], expressed, purified, preserved in our laboratory. For the detection of antibodies against IBV, the recombinant N protein was expressed as GST fusion protein in Escherichia coli BL21 (DE3) cells [29]. The negative sera of SPF chickens and the positive virus serum (ILTV, ALV, NDV, MDV, H5, H7 and H9) were purchased form Harbin Weike Biological Technology Development Company, China. The positive sera (IBV and AIV) were obtained from China Veterinary Culture Collection Center. Ninety of clinical chicken serum samples were collected from a chicken farm in Huizhou, China.
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Coupling of proteins to fluorescent microspheres
Prior to coupling, the recombinant proteins was desalted by gel filtration using MicroBio-Spin 6 columns (Bio-Rad, California, USA) based on the manufacture’s protocol to exchange the buffer from sodium azide or imidazole to PBS. All the antigens were quantified using Pierce BCA protein Quantification Kit (Thermo Scientific, USA). Coupling of proteins to fluorescent microspheres was performed as described by Karanikola et al. [30]. MAP MC10007 beads (Luminex, USA) were coupled by gD protein of ILTV and MAP MC10015 beads (Luminex, USA) were coupled by N protein of IBV. A certain number of beads was transferred to one coupling reaction tube, followed by 100 μL bead wash buffer and suspended in 80 μL bead activation buffer. Then 10 μL of 50 mg/ml EDAC (Sigma-Aldrich) and 10 μL of 50 mg/ml S-NHS (Sigma-Aldrich, Germany) were added in the reaction buffer. The reaction tube was gently vortexed for 20 min at room temperature (RT). PBS (pH 7.4, 150 μL) was added twice and the recombinant protein was added. Incubation was carried out at RT for 2 h. The coupled beads were centrifuged and washed. Ultimately, the beads were stored at 4 °C in 150 μL storage buffer in the darkness.
Methods for bead-based xMAP technology
The xMAP assays were carried out in 96-well polystyrene microplates using Luminex 200 detection system (Luminex, USA). Relevant positive and negative sera have been prepared for the establishment of the singleplex xMAP assay to detect ILTV antibody or IBV antibody in the serum. ILTV gD protein at the following concentrations (2.5 μg, 5 μg, 10 μg, 20 μg, 40 μg, and 80 μg) and IBV N protein at the following concentrations (3 μg, 6 μg, 12 μg, 24 μg, 48 μg, and 96 μg) were coupled with 5 × 105 magbeads to determine the optimum antigen concentration for singleplex xMAP assay. A serious dilution of sera at the range from 1:25 to 1:200 have been made to determine the optimal sample dilution. Cross-reactivity or specificity was evaluated by making the assay with sera from chicken infected with AIV, ALV, NDV, and MDV. Then, a duplex xMAP assay was established based on the result of two separated singleplex xMAP assay. In briefly, a 50 μL aliquot of the simplex beads (50 beads/μL) or the duplex beads (100 beads/μL, 50 beads/μL each kind) was transferred into the wells, added in 50 μL of diluted sera. Incubation was conducted on a plate shaker (800 rpm) at RT for 60 min. The centrifugation was conducted in the magnetic separator for 60 s. The supernatant was removed from each well. Beads were washed 5 times in 100 μL PBS. Each well was added with 100 μL of a biotinylated secondary antibody (goat anti-chicken IgY, Beijing Solarbio Science & Technology, China) at 2 μg/mL. The plate was shaken (800 rpm) for 30 min at RT and washed as described above. Finally, 2 μg/mL of streptavidin-phycoerythrin (SAPE, Life Technologies GmbH) was added to each well at 100 μL/well. The plate was shaken and the supernatant was removed. Finally, 100 μL of assay buffer was added to each well. The plate was shaken for approximately 15 s and analyzed according to the manufacturer’s protocol. All samples were conducted in triplicates in each assay.
ELISA used for comparison
Commercial ILTV and IBV ELISA kit (Biochek, Netherlands) were used to detect presence of ILTV or IBV antibodies in poultry sera. The assay was performed according to the manufacturer’s protocols.
Funding
The study was supported by the Science and Technology Research Program from Department of Science and Technology, Guangdong Province and Guangzhou Municipal (2015B070701003, 2016A040403060, 2017B030314171, 2016201604030059 and 2017A070702001) of the. This study was also supported by the National Key Technology R&D Program (2015BAI07B01).
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Availability of data and materials
All data generated or analyzed during this study are included in this published article. Contact corresponding author for requests.
Ethics approval and consent to participate
Not applicable.
Consent for publication
Our manuscript does not contain any individual person’s data in any form.
Competing interests
The authors declare that they have no competing interests.
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