Indirect ELISA based on Hendra and Nipah virus proteins for the detection of henipavirus specific antibodies in pigs

Hendra virus (HeV) and Nipah virus (NiV) belong to the genus Henipavirus in the family Paramyxoviridae. Henipavirus infections were first reported in the 1990’s causing severe and often fatal outbreaks in domestic animals and humans in Southeast Asia and Australia. NiV infections were observed in humans in Bangladesh, India and in the first outbreak in Malaysia, where pigs were also infected. HeV infections occurred in horses in the North-Eastern regions of Australia, with singular transmission events to humans. Bats of the genus Pteropus have been identified as the reservoir hosts for henipaviruses. Molecular and serological indications for the presence of henipa-like viruses in African fruit bats, pigs and humans have been published recently. In our study, truncated forms of HeV and NiV attachment (G) proteins as well as the full-length NiV nucleocapsid (N) protein were expressed using different expression systems. Based on these recombinant proteins, Enzyme-linked Immunosorbent Assays (ELISA) were developed for the detection of HeV or NiV specific antibodies in porcine serum samples. We used the NiV N ELISA for initial serum screening considering the general reactivity against henipaviruses. The G protein based ELISAs enabled the differentiation between HeV and NiV infections, since as expected, the sera displayed higher reactivity with the respective homologous antigens. In the future, these assays will present valuable tools for serosurveillance of swine and possibly other livestock or wildlife species in affected areas. Such studies will help assessing the potential risk for human and animal health worldwide by elucidating the distribution of henipaviruses.


Introduction
Hendra virus (HeV) and Nipah virus (NiV) represent the prototypes of the genus Henipavirus within the family Paramyxoviridae. Henipaviruses first emerged in Southeast Asia and Australia in the 1990's, causing severe febrile illness in domestic animals and humans [1][2][3] foxes of the genus Pteropus have been identified as the major natural reservoir of these zoonotic viruses [4,5]. Virus transmission mainly occurred from bats to intermediate hosts such as pigs or horses, before humans were eventually infected by contact to these intermediate hosts [6][7][8][9]. However, during more recent NiV outbreaks in Bangladesh and India, direct transmission from bats to humans and human-to-human transmission also occurred [10,11]. Both viruses require handling under Biosafety Level 4 (BSL 4) conditions. The diagnostics of acute HeV or NiV infections primarily relies on a direct detection of the viral agent via molecular assays such as real-time RT-PCR, immunohistochemistry or virus isolation [12]. However, since a broad variety of mammalian species have been shown to be susceptible to HeV or NiV infection under experimental conditions, serosurveillance studies in affected areas may play an important role in improving our understanding of the epidemiology of these infections [13][14][15][16][17][18][19][20]. For these studies, simple and cost-efficient serological diagnostic assays are needed that can easily be performed outside a BSL 4 facility. In the past, several strategies have been followed to express recombinant henipavirus proteins that can be handled under BSL 2 conditions either in indirect enzyme-linked immunosorbent assay (ELISA) or in Luminex-based multiplexed microsphere assays [21][22][23][24][25][26][27]. Data in several reports indicated that there are crossreactive antibodies in serum samples from domestic animals and livestock not only in the Southeast Asian / Australian region, but also in geographic areas where henipavirus infections have not been reported, such as Sub-Saharan Africa [28][29][30][31][32]. In areas of Bangladesh where human NiV outbreaks had been observed, serum samples from pigs, cattle and goats have been tested positive for the presence of antibodies against a truncated, soluble form of the NiV glycoprotein (NiV sG) in a Luminex-based microsphere assay [31]. In this study, glycoproteins of HeV and NiV (sHeV G; sNiV G), as well as the NiV nucleocapsid protein (NiV N) were produced for the development of indirect ELISAs. Both viral proteins were selected due to their known immunogenicity. The G proteins were expressed in the eukaryotic parasite Leishmania tarentolae (L. tarentolae), whereas the NiV N protein was expressed in Escherichia coli (E. coli). Since HeV and NiV N proteins share a homology of 92% at the amino acid level [33], we used the NiV N ELISA for initial serum screening regarding the general reactivity of the tested sera with henipaviruses. Subsequently, the serum samples were tested on both G protein based ELISA assays to differentiate between HeV and NiV infections. To evaluate the antigens for their suitability in ELISA, we used a number of henipavirus IgG negative porcine sera and a panel of well characterized sera from experimentally HeV or NiV infected pigs.

Expression of his-tagged NiV nucleocapsid (N) protein
The NipahN/IRES/CMV plasmid was kindly provided by Dr. Markus Czub (Public Health Agency of Canada, Winnipeg, Manitoba, Canada), and the N-protein coding region was subcloned using the BamH I restriction sites into the pET-30a vector (Novagen), creating the pET-30a/Nipah N plasmid. After confirmation of positive pET-30a/Nipah N clones by sequencing using the commercially available primers T7 FOR promoter-5'-TAA TAC GAC TCA CTA TAG G_3' and T7 Terminator Primer -5'-CCG CTG AGC AAT AAC TAG C-3' 8 (Millipore Sigma) with subsequent comparison to the NiV genome (accession no. AF212302), the plasmid was transformed into the Rosetta (DE3) E. coli bacterial cell line (Novagen) for expression. The inclusion body fraction contained most of the N protein. The harvested inclusion bodies were solubilized using standard methods, and the inclusion body proteins were separated by 10% sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) on large 20 cm PRO-TEAN II xi (Bio-Rad) apparatus. Each gel was washed in Milli-Q water and stained with a solution of 0.2 M copper (II) chloride hydrate for 10 min. The largest band (~62 kDa) was cutout and destained in Towbin's buffer [34]. Destained gel was electro-eluted using the Bio-Rad Model 422 Electro-Eluter according to the manufacturer's instructions. The membrane filter used had a molecular weight cut-off of 15 kDa. After electro-elution for 4 h at a constant current of 10 mA per holder, samples were aliquoted in 100 μl fractions and stored at -20˚C.

Immunoblot analysis of NiV N antigen
The NiV N protein was characterized by immunoblot using standard procedures. Briefly, N antigen was separated by 10% SDS-PAGE. After transfer to a polyvinylidene fluoride (PVDF) membrane, the membrane was blocked with 5% skim milk (Gibco, Germany) diluted in PBS/ 0.05%Tween-20 (PBST) for 1 h at room temperature (RT), and probed overnight at 4˚C with NiV N protein specific monoclonal antibody F45G4 was diluted to 1:2,000 [35]. After washing with PBST, the membrane was incubated for 1 h at RT with an anti-mouse secondary antibody conjugated to horseradish peroxidase (HRP; Sigma-Aldrich) in at a 1:3,000 dilution. The blot was then incubated with SuperSignal West Pico Chemiluminescent Substrate according to the manufacturer's guidelines (Thermo Scientific), and protein detection was visualized on Amersham Hyperfilm ECL ™ film (Fisher Scientific).

Transmission electron microscopy of NiV N antigen
An inclusion body fraction of semi-purified Nipah N antigen was prepared by negative contrast electron microscopy. Specifically, 20 μl of sample was absorbed to formvar-coated carbon-stabilized copper grids and stained with 2% phosphotungstic acid, pH 7.2 (wt/vol). The specimen grids were examined in a Philips CM 120 transmission electron microscope, operating at an accelerating voltage of 80 kV. Micrographs were taken between 28,000X -45,000X using Kodak Electron Microscope Film 4489. The negatives were scanned using an Epson Perfection 3200 photo scanner and enlarged 2.5X.

Expression of HeV and NiV attachment (G) proteins in Leishmania tarentolae (L. tarentolae)
The expression of a truncated soluble HeV G (sHeV G) protein has been described before [36], and the expression of a truncated soluble NiV G (sNiV G) protein in the L. tarentolae system (Jena Bioscience, Germany) was performed accordingly. Briefly, the NiV G sequence was codon optimized for the codon bias of L. tarentolae and the transmembrane domain and cytoplasmic tail were replaced by a double Strep-tag in order to enable affinity chromatography. The sequence product was cloned into the vector pLEXSY-sat2 (Jena Bioscience) using XbaI and NotI restriction sites to yield pLEXSYNiVG. The codon-optimized NiV G sequence was submitted to GenBank (accession No. MF379666). Transfection, clonal selection and subsequent protein purification were carried out as described previously [36]. Purity and size of the protein was evaluated by 10% SDS-PAGE and subsequent Coomassie blue staining. Protein concentration was determined by modified Bradford protein assay based on bovine serum albumin (BSA; GE Healthcare, Germany) as standard and according to the manufacturer's instructions (Sigma Aldrich).

Generation of monoclonal antibody (mAb) 5G1B1 raised against the sHeV G protein
Female BALB/c mice were immunized five times intraperitoneally with 15 μg of recombinant HeV G protein expressed in the L. tarentolae system mixed with an equal amount of GERBU Adjuvant MM (GERBU Biotechnik GmbH) in an interval of 4 weeks. Four days after the final boost, the immunized mice were euthanized and the spleens were removed under aseptic conditions. Splenocytes were harvested in serum-free RPMI-1640 medium (Invitrogen/Thermo Scientific) by using a cell strainer (BD Biosciences). Murine myeloma SP2/0 cells (Cell Culture Collection of the Friedrich-Loeffler-Institut, Germany) and the isolated splenocytes were fused in presence of polyethylene glycol 1500 (Roche Applied Science) following a standard protocol [37,38] by using a cell-to-cell ratio of 4:1. Afterwards, 10.5x10 6 fused spleen cells were seeded in three different cell densities (30,000, 15,000, and 7,500 spleen cells per well, two plates per density) in 96 well flat-bottom plates (Greiner bio-one) and incubated over 10 days at 37˚C, 90% RH, and 5% CO 2 . The complete RPMI-1640 culture medium contained 10% fetal calf serum (Fischer Scientific, #11573397), 1x MEM non-essential amino acids, 2 mM L-glutamine, and 1 mM sodium pyruvate (Invitrogen/Thermo Scientific). For the initial growing phase of the hybridoma cultures, the complete medium was additionally supplemented with 1x BM Condimed H1 (Hybridoma Cloning Supplement, Sigma-Aldrich) as well as 1x HAT Media Supplement (50×) Hybri-Max (Sigma-Aldrich) for selection. Growing cultures were screened for specific antibodies by ELISA using the recombinant protein. Cells from positive cultures were cloned at least twice by limiting dilution (0.1 cells per well) for generating monoclonal antibody producing cell clones [complete RPMI-1640 medium supplemented with 1x HAT Media Supplement (50×) Hybri-Max (Sigma-Aldrich)]. Final clones were adapted to complete RPMI-1640 medium without any further supplements.

Immunofluorescence assay (IFA) for the detection of HeV and NiV G antigens
For immunofluorescence assay (IFA), Vero76 cells (Cell Culture Collection of the Friedrich-Loeffler-Institut, Germany) were either transfected with the pCAGGS HeV G plasmid [36] or with a codon-optimized NiV G expression plasmid (pCAGGS NiV G; GeneArt) using Tran-sIT-LT1 transfection reagent (Mirus Bio). After 48 h, monolayer cultures were fixed with 4% paraformaldehyde solution and permeabilized with 0.2% Triton-X100 (Sigma-Aldrich) in PBS. For the detection of both proteins, undiluted hybridoma supernatant producing the mAb 5G1B1 was used followed by the incubation with Alexa Flour 488-conjugated secondary antimouse antibodies (1:500 in 5% BSA in PBS; 5% BSA/PBS). Fluorescence was visualized using a DMI7 live cell microscope (Leica), a CSU-W1-T spinning disc confocal scanning head (Yokogawa) and an iXon Ultra 888 EMCCD camera (Andor).

Indirect ELISA based on NiV N protein
Electro-eluted NiV N antigen in 0.01 M PBS, pH 7.2 was coated on Nunc F flat bottom polystyrene plates at a concentration of 100 ng/well (100 μl volume). The plates were incubated overnight at 4˚C followed by washing five times using PBST solution. Each well was then blocked using a volume of 100 μl/well of blocking buffer (3% BSA/10% horse serum/0.1% Tween 20 in 0.01 M PBS pH 7.2) buffer. Sterile Donor Horse Serum (lot#CS-C14-500) was purchased in 2002 from CanSera. After incubating the plates at 37˚C for a minimum of 1 h with shaking, the plates were washed as outlined above. Titration experiments revealed a 1:100 dilution of pig serum (both negative and test sera) in blocking buffer as optimal for this ELISA system. (Negative serum samples were submitted to NCFAD for pseudorabies and classical swine fever testing (NCFAD collection of diagnostic samples); test serum samples were collected during the animal studies mentioned in the Ethics statement. After adding 100 μl/well, the plates were incubated at 37˚C for 1 h with shaking, followed by a washing step as outlined previously. A 1:1,000 dilution (in blocking buffer) of rabbit anti-pig IgG secondary antibody conjugated to HRP (100 μl/well) (Intermedico) was then added to the plates for 1 h at 37˚C with shaking. After another washing step, 100 μl/well of enzyme substrate (2,2'-azino-bis(3-ethylbenzothiazoline-6-sulphonic acid)) (ABTS; Roche Diagnostics) was added. After incubating the plates for 15 min at RT in the dark, they were analyzed on a microtiter reader at an absorbance of 405 nm.

Indirect ELISA based on sHeV and sNiV G proteins
sHeV and sNiV G proteins were diluted in 0.01 M PBS, pH 7.4 and coated on Medisorp 96 well plates at a concentration of 100 ng/well (100 μl volume) and kept at 4˚C overnight. Extracts from untransfected L. tarentolae served as mock antigens in control wells to evaluate unspecific binding of the sera. Plates were blocked with 5% skim milk in 0.01 M PBS for 2 h at 37˚C and washed three times with PBST. Sera were diluted 1:200 in 2.5% skim milk in PBST and added in duplicate to the control and antigen containing wells. After an incubation at 37˚C for 1 h, the plate was washed again three times. Goat-anti-swine IgG HRP conjugate (Dianova) was added in a dilution of 1:10,000 and incubated for 1 h at 37˚C. After four washes with PBST, 3,3',5,5'-Tetramethylbenzidine (TMB) peroxidase substrate (Bio-Rad, Munich) was added to the wells for color development and stopped after 10 min at RT with equal amounts of 1 M sulfuric acid. Absorbance was measured at 450 against 590 nm in a Tecan Infinite 200Pro ELISA Reader (Tecan Deutschland GmbH).

Serum samples and statistical analysis
For the evaluation of the NiV N protein based ELISA, 239 serum samples submitted to NCFAD for pseudorabies and classical swine fever testing (NCFAD collection of diagnostic samples) were used as a negative control panel. For the evaluation of the ELISA assays based on the sHeV and sNiV G proteins, serum samples from 154 pigs from different holdings in Germany (collected during the animal studies mentioned in the Ethics statement) were used as the negative control panel since for both Canada and Germany there is no history of previous henipavirus infection. A panel of 12 sera from pigs experimentally infected with NiV (10 sera) or HeV (2 sera) served as a positive control panel for the initial evaluation of all three ELISAs. These positive sera were collected during experimental NiV and HeV infection trials from different days post infection (dpi), therefore displaying different titers in confirmatory plaque reduction neutralization test (PRNT). Sera were heat inactivated at 56˚C for 60 min prior to analysis in the ELISA. The mean values, standard deviation and diagnostic specificity (D-SP) values were calculated based on the absorbance values of the serum samples. The D-SP was calculated using the following formula: number of negative sera tested minus number of negative sera tested positive divided by number of negative sera tested x 100. When determining the positivity of the pig serum samples tested, we used a cut-off absorbance of three standard deviations above the mean.

Immunoblot analysis of ELISA-positive porcine serum samples
To confirm the specific binding of the ELISA-positive porcine serum samples to the antigens, an exemplary panel of porcine sera was investigated for their reactivity in immunoblot, using a cell lysate of HEK-293T cells (Cell Culture Collection of the Friedrich-Loeffler-Institut, Germany) transfected with a codon optimized NiV G expression plasmid (pCAGGS NiV G) as antigen. Immunoblots were performed as described above for the detection of the N protein.
Briefly, cell lysate was separated by SDS-PAGE and transferred to a nitrocellulose membrane, which was then incubated with porcine sera (dilution 1:200 in 2.5% skim milk in PBST) overnight at 4˚C. Species-specific goat anti-swine antibodies conjugated with HRP (Dianova) were incubated on the membrane for 1 h at RT in a 1:5,000 dilution. MAb 5G1B1 in a dilution of 1:100 served as a positive control for the detection of NiV G antigen expressed in HEK-293T cells.

Plaque reduction neutralization test (PRNT)
The PRNT was performed as published previously using NiV [39], and all procedures with live virus were performed under BSL-4 conditions.

Ethics statement
Manipulations of animals at the Friedrich-Loeffler-Institut mentioned in this report had the specific approval (LALLF 7221.

Antigen production
Most of the NiV N protein was found in the insoluble fraction harvested from the of E.coli expression system. The protein was harvested by electro-elution from this fraction, and purified by gel electrophoreses. The identity of the harvested protein as NiV N was confirmed by immunoblotting with monoclonal anti-N antibody F45G4. The apparent molecular size of the recombinant NiV N protein corresponded with the expected molecular size of approximately 63 kDa (a 5 kDa histidine tag from the pET-30a vector included) ( Fig 1A). As determined by Bradford analysis, a recovery of 6.72 mg of Nipah N protein was obtained per liter of a starting culture of Nipah N/pET30A transformed Rosetta E. coli. Transmission electron microscopy of a solubilized inclusion body pellet fraction (isolated after 2 h of induction) containing the NiV N protein, detected both clusters and individual herringbone-like structures (Fig 1B). These structures ranged in size from~70-100 nm in length. Upon treatment of these structures with the detergent SDS (i.e. after electro-elution), no herringbone-like structures were apparent. A solubilized inclusion body pellet of the negative controls (isolated after 0 h of induction) did not show any such structures (S1 Fig). To be able to compare the performances of sNiV G and sHeV G in ELISA, a Leishmaniabased expression system was chosen in order to maintain proper glycosylation of the glycoproteins. After transfection of sequence-verified plasmids, four recombinant clones were randomly selected and used for sNiV G protein expression. As previously observed for the expression of the closely related sHeV G protein in L. tarentolae, sNiV G was not efficiently secreted into the growth medium, even though the protein was fused to the secretory signal peptide (SP) of Leishmania mexicana secreted acidic phosphatase (LMSAP). However, we purified nearly 1 mg of recombinant protein per liter of densely grown cell culture lysates as quantified by Bradford protein assay. The electrophoretic analysis of the six elution fractions of the two glycoproteins demonstrated the enrichment and purity of the approximately 70 kDa comprising sHeV G and sNiV G as depicted in Fig 1(C).

Generation and characterization of monoclonal antibodies (mAb) raised against sHeV G
For the generation of monoclonal antibody producing hybridoma clones, BALB/c mice were immunized with the Leishmania-derived sHeV G protein. Growing cultures were screened for specific antibodies by Western Blot using the recombinant sHeV G protein and a commercially available recombinant form of the HeV G protein expressed in mammalian cells (Sino Biological Inc., USA; Panel A in S2 File). One most promising mAb clone designated 5G1B1 was selected eventually and further validated regarding the specific binding by IFA in Vero 76 cells that were either transfected with plasmid-derived HeV G or NiV G. MAb 5G1B1 showed a highly specific detection of the HeV and NiV G proteins in transfected Vero 76 cells (Fig 2). These results indicate a high level of conservation between the targeted epitope of both G proteins. By that we were able to show that 48 h after transfection, NiV and HeV G proteins both accumulated on the cell surface as well as in the cytoplasm. In contrast, no signal was observed in mock transfected cells (Panel B in S2 File).
The reactivity of clone 5G1B1 was also confirmed by Western blot analysis of NiV G protein expressed in HEK-293T cells as well as sHeV G and sNiV G expressed in L. tarentolae (Panel C in S2 File).

Application of recombinant proteins in ELISA
In order to determine diagnostic specificity of the NiV N ELISA, 239 negative porcine sera submitted to NCFAD for pseudorabies and classical swine fever testing were used as negative control panel. These sera were considered negative due to the lack of evidence for circulation of henipaviruses in Canada. With the cut-off value of the determined optical density at 405 nm (OD 405 ) of 0.32 (average OD 405 value was at 0.124, plus 3 StDev) the diagnostic specificity (D-SP) of the N ELISA was at 99% (Fig 3A). Only two serum samples had OD 405 values above the cut-off, and would undergo confirmatory testing such as Western blot analysis or PRNT to determine whether they are true or false positive results.
For the evaluation of both sHeV G and sNiV G ELISAs, we investigated 154 sera from pigs originating from different holdings in Germany. These sera were considered negative due to the lack of evidence for the circulation of henipaviruses in Germany. The OD 450 average of all tested German pig sera in the sHeV G and sNiV G ELISA was 0.076 and 0.068, respectively, highlighting the generally low background of these tests. Using the average OD 450 plus 3 StDev, cut-off values were calculated as 0.28 for the sHeV G and of 0.26 for the sNiV G ELISA (Fig 3B and 3C). The results obtained for six sera in the sHeV G ELISA and three sera in the sNiV G ELISA slightly exceeded the calculated cut-off values. Six of these samples were tested by Western Blot against a cell lysate of transfected HEK-293T cells expressing the NiV G protein with negative result (Fig 4 and S3 Fig) and were thus considered as false positive. Consequently, a D-SP of 96.1% and 98.0% was determined. Although due to lack of sufficiently characterized samples, this immunoblot assays could not be fully validated, the positive control monoclonal antibody 5G1B1 raised against the sHeV G protein clearly cross-reacted with the NiV G protein expressed in HEK-293T cells in immunoblot test. Sera obtained from HeV or NiV challenge studies also clearly (cross-) reacted with the NiV G protein in the immunoblot (Fig 4). In contrast, two German pig sera (GER11 and GER34) that exceeded the calculated cut-off value in both G based ELISAs, as well as one serum (GER27) that only exceeded the cut-off value in the sHeV G based ELISA did not display any reaction with the antigen in immunoblot analysis. To test the general suitability of our assay system for the detection of henipavirus-infected pigs, we analyzed a set of serum samples that had been collected during NiV and HeV challenge studies and which were determined positive for neutralizing antibodies by PRNT [14,[39][40][41]. These serum samples were first screened using the NiV N based ELISA (Fig 5A), and then tested for their specific reactivity against the sHeV and sNiV G proteins ( Fig 5B). As expected, the recombinant proteins showed stronger reactions with sera from pigs that were infected with the homologous virus: OD 450 values of sera from NiV infected pigs were higher on the sNiV G ELISA as compared to the sHeV G ELISA, and vice versa. All the tested sera however clearly cross-reacted with the sHeV G or the sNiV G antigen, as illustrated in Fig 5B. Selected serum samples were also tested by NiV-PRNT to analyze the correlation between the results obtained by NiV N ELISA, NiV and HeV G ELISAs and NiV-PRNT, which showed an overall good correlation between the G protein based ELISAs and the PRNT (Table 1). For the sHeV G ELISA, one HeV IgG positive serum as well as one NiV IgG positive serum, both collected 28 dpi, were serially diluted for a better comparison of the binding affinities of the sera to the homologous and heterologous G proteins, respectively. For the serum of the HeV challenged pig (NiV-PRNT titer of 1,280), a serum dilution of 1:12,800 still revealed a positive result in the sHeV G ELISA (Fig 5C). The same PRNT titer (1,280) serum from a NiV infected pig displayed a negative result in the sHeV G ELISA in a 1:12,800 dilution, and a very weakly positive OD 450 value at a dilution of 1:6,400 (Fig 5C).

Discussion
Henipaviruses first emerged in the 1990's leading to fatalities in Southeast Asian and Australian livestock and human population. HeV and NiV are highly pathogenic zoonotic viruses  (Mock 1-3). Two German pig sera (GER11 and GER34) that exceeded the calculated cut-off value in both G based ELISAs as well as one serum (GER27) that only exceeded the cut-off value in the sHeV G based ELISA were tested exemplarily for reactivity in immunoblot analysis. All sera were diluted as indicated. The monoclonal antibody 5G1B1 was utilized in a dilution of 1:100. of bat origin and have caused several outbreaks with considerable economic and social impact [1,[42][43][44][45]. Serological surveillance to monitor the natural host and other susceptible animals represents a valuable approach to predict potential health risks. We developed a set of indirect ELISAs for swine samples to facilitate risk assessment in the affected areas. Recombinant HeV and NiV G and NiV N proteins were designed and evaluated for use in the ELISAs, as they do not, unlike whole virus antigens, require BSL 4 containment for production. We used a combination of these three recombinant proteins for an optimized detection and specification of antibodies directed against NiV, HeV or other paramyxoviruses in pigs. Although a recombinant NiV N protein expressed in E. coli has been used in serological assays earlier [23,25], the combination of an E. coli derived NiV N protein and both HeV and NiV glycoproteins expressed in L. tarentolae to ensure a mammalian-like glycosylation pattern, helps us assessing and specifying the detected reactivity. While we use the recombinant NiV N protein for an initial screening of pig sera, reactive sera will be further examined using both recombinant glycoproteins. Due to the higher binding affinity to the homologous  G; NiV N). A. Sera from pigs (P) and minipigs (M) were collected at different days post infection (dpi) and tested for the presence of henipavirus specific IgG in the N based assay, with the red line representing the cut-off value. B. Serum reactivity was confirmed and specified in the sHeV G and sNiV G specific ELISAs with the white line representing the cut-off value of the sNiV G based assay and the red broken line representing the sHeV G assay cut-off value. C, D. One HeV IgG positive as well as one NiV IgG positive serum were serially titrated and tested for reactivity in the sHeV G based assay (C) and in the NiV based assay (D) with the red lines representing the cut-off values. https://doi.org/10.1371/journal.pone.0194385.g005 Detection of henipavirus infections in pigs protein, this will ensure the differentiation between antibodies directed against NiV, HeV or other related paramyxoviruses.
Besides the safe production under BSL 2 conditions, recombinant proteins can be produced with a high reproducibility among antigen batches and facilitate standardization of assays [25]. To date, most of the recombinant proteins used in diagnostic assays are expressed in E. coli, baculovirus infected insect cells, or mammalian cells. In this study we used the highly efficient E. coli expression system for the NiV N protein. New expression systems have recently been developed especially for the expression of glycoproteins with mammalian-like glycosylation pattern, such as the eukaryotic parasite L. tarentolae that may serve as a valuable platform for viral protein expression due to their relatively easy maintenance and fast growth as well as high protein yields [46]. Therefore, in this study we used the highly efficient L. tarentolae expression system for the NiV G and HeV G proteins. Due to their immunogenicity, Leishmania-derived hepatitis C virus envelope glycoprotein and influenza virus hemagglutinin have been proposed as promising vaccine candidates [47,48], and a truncated hepatitis E capsid protein was used in an indirect ELISA [49]. In our study, the sHeV G protein produced in L. tarentolae was not only successfully applied in a serological test but was also used to generate monoclonal antibodies. The selected clone 5G1B1 displayed a clear cross-reactivity against the NiV G protein in all conducted assays, including ELISA, IFA and immunoblots, indicating a target epitope in the G protein that is conserved between the two viruses.
In this report, the protein yield of sHeV G and sNiV G of approximately 500 μg-1 mg per liter of densely grown Leishmania cells was within the expected range of the expression system [50]. In a previous study, NiV G was expressed in baculovirus-infected insect cells resulting in a less complexly glycosylated protein while obtaining higher protein yields of 1-2 mg/ml per 1.5 x 10 6 Sf9 cells [21]. For the NiV N, a recovery of 6.72 mg of NiV N protein was obtained per liter of transformed Rosetta E. coli starting culture, which was considerably higher than what has been described in earlier studies using recombinant NiV N protein in E. coli obtaining yields of 1 mg per liter starting culture [25] and 0.8 mg per liter starting culture [51]. In another study, baculovirus-infected Sf9 cells were used for the expression of the recombinant NiV N protein at high yields of 2-3 mg per 1 x 10 6 infected Sf9 cells [23]. Furthermore, when the NiV N protein was expressed in E.coli, the recombinant protein self-assembled into Detection of henipavirus infections in pigs herringbone-like particles as observed before [52]. These results clearly indicate the bacterial expression system to be a quick and relatively easy method for the expression of high yields of recombinant NiV N protein in its native form. The henipavirus G and N proteins were chosen due to their described immunogenicity [53,25]. The henipavirus G protein is responsible for host cell receptor binding and thus a major target for neutralizing antibodies [54,55]. HeV and NiV G proteins share 83% of amino acid sequence homology, whereas the N proteins of both viruses share up to 92% sequence homology, and serological cross-reactivity was confirmed by several studies, making the N protein based assay a good candidate for the initial screening of field sera [56,33,53,35,26,14]. In a recent study by Marsh et al., rabbit antibodies against the N protein of the Cedar virus, another member of the Henipavirus genus, cross-reacted with the HeV N and NiV N in an immunofluorescence assay, although only a 58-59% amino acid sequence identity was observed [57]. These findings further highlight the potential of the N based ELISA as an initial henipavirus screening test. Another group investigated 76 bat sera from 11 different species from Brazil for reactivity in their newly established Nipah N based ELISA [58]. Interestingly, nine bat sera cross-reacted with the Nipah N protein in the ELISA as well as in the confirmatory IFA, indicating the circulation of henipa-like viruses in Brazil.
We calculated specificities of 99%, 96% and 98% for our ELISA based on NiV N, HeV G and NiV G. In recent studies using the NiV N protein, a specificity of 98.7% was calculated based on a sample panel of 1709 porcine positive and negative samples [59], while a specificity of 98.4% was determined by testing a set of 133 positive and negative human samples [25].
The observed broad cross-reactivity of antibodies against the N protein within the known members of the genus Henipavirus, however, necessitates additional serological assays specific for HeV or NiV, the viruses of human and animal health interest. Therefore, we developed a second ELISA based on either the sHeV or sNiV G proteins, in order to determine the specific reactivity of the serum.
We observed a considerable cross-reactivity of the sera against the heterologous antigens in ELISA which is in accordance with the cross-reactive NiV-PRNT results obtained from a HeV challenge study in pigs [14]. Interestingly, the cross-reactivity is not always correlated with cross-protection. For several animal models such as cats, African green monkeys and ferrets, animals that were pre-vaccinated with HeV G proteins were clearly cross-protected against a NiV challenge [60][61][62][63]. In pigs, however, a recent study revealed a lack of cross-protectivity and only low cross-neutralizing activity when vaccinated with one of the G proteins and challenged with the heterologous virus [64].
The ELISAs used in our study clearly discriminated sera from experimentally infected pigs collected at different dpi and sera from uninfected henipavirus negative pigs. However, since the number of available positive porcine field sera is very limited, the sensitivity of the assays can only be estimated. In addition, that applies equally to the confirmatory tests that were only validated by using serum samples from experimentally infected animals, while positive field sera were inaccessible for validation purposes. Therefore, the occurrence of false negative results when testing field sera cannot be completely ruled out for any of these tests. To finally validate the newly established assays, testing field sera of well-known origin would be desirable.
The recombinant proteins which were expressed in different expression systems obviously displayed the relevant antigenic epitopes necessary for the recognition in ELISA. A low number of assumed negative sera (i.e. originating from Canada or Germany, with no henipavirus activity) were reactive in individual ELISAs. These sera were further investigated by immunoblot or by NiV-PRNT [39], and no specific reaction was detected with the NiV G antigen expressed in eukaryotic HEK-293T cells or in the PRNT. Interestingly, there is recent serological and molecular evidence for the presence of a diverse group of henipa(-like) viruses in different geographic regions around the world [28,29,65,66,31,67], even with reports about a potential spillover into the human population of Sub-Saharan Africa [68]. Although the collected data suggests a close antigenic relationship between the G proteins of HeV and NiV and that of the putatively circulating African henipavirus, it is noteworthy that these findings have not been linked to disease reports yet, and virus isolates are still missing. Chowdhury et al. tested a panel of serum samples from livestock located in a human NiV outbreak area with a considerable number of positive results in the applied Luminex assay using HeV and NiV G proteins as antigens [31]. Although none of the detected antibodies displayed neutralizing activities, the results emphasize the need for further surveillance, based on reliable serological diagnostics to better predict a potential risk to human health in the future. In the future, the newly established assays will be expanded and adapted to other mammalian species in different regions where henipa (-like) viruses have been assumed to occur. In our study, henipavirus G and N protein based ELISAs proved to be suitable assays for the detection of henipavirus specific antibodies in experimentally infected pigs. However, due to lack of availability of field sera and only a low number of available positive experimental sera, the ELISAs could not be fully validated in terms of diagnostic sensitivity. For their application in serological and epidemiological studies in pigs, it would be desirable to determine the assays' detection limits in the early stage of infection. Nonetheless, these newly established tools will be highly valuable for a serological screening of different animal species in regions where natural reservoir hosts are abundant. Western blot analysis of 5G1B1 reactivity against commercially obtained HeV G/Fc (Sino Biologicals). The monoclonal antibody hybridoma supernatant 5G1B1 was utilized in a dilution of 1:10 and 1:100. Other hybridoma supernatants were tested but did not reveal positive signal in Western blot. B. Immunofluorescence analysis of monoclonal antibody 5G1B1 reactivity against Mock-transfected Vero76 cells. Vero 76 cells were transfected with the pCAGGS plasmid. For immunostaining, the newly generated cross-reactive monoclonal antibody 5G1B1 was used followed by mouse specific Alexa-Fluor 488-labeled secondary antibodies. Nuclei were stained with Hoechst. Fluorescence was visualized by a DMI7 live cell microscope (Leica), magnification 630 x. C. Western blot analysis of 5G1B1 reactivity against Leishmania-derived sHeV or NiV G. The monoclonal antibody hybridoma supernatant 5G1B1 was utilized in a dilution of 1:100. (TIF) S3 Fig. Immunoblot analysis of reactivity of additional serum samples against plasmid derived NiV G. Serum sample from a NiV infected pig was collected at 7 dpi served as a positive control. Six German pig sera that exceeded the calculated cut-off values in or or both G based ELISAs were tested for reactivity in immunoblot analysis. All sera were diluted as indicated. The monoclonal antibody 5G1B1 was utilized in a dilution of 1:100. (TIF)