Sera (n = 279) were collected from patients affected by choroidal nevi (CN; n = 71) and healthy subjects without ocular nevi (HS; n = 208), attending the Eye Clinic of the University Hospital of Ferrara, Italy. Serum samples were collected after routine analysis from discarded samples from the Clinical Laboratory Analysis before incineration.

The two cohorts included patients/individuals of both genders, with the same median age (range = 64–67 years), Table 1.

Anonymously collected sera were coded with indications of age, gender, and pathology only. Written informed consent was obtained from the subjects after explanation of the nature and possible consequences of the study. All patients/subjects signed informed consent at the time of hospital admission. The research followed the tenets of the Declaration of Helsinki. The Ethics Committee, Ferrara, approved the study.

Computer assisted analyses enabled us to identify two specific BKPyV peptides, selected from the late viral region by comparing BKPyV VP1 with the corresponding amino acids from JCPyV and SV40, which are highly homologous to BKPyV, as well as with other, less homologous, polyomaviruses (web site, http://blast.ncbi.nlm.nih.gov; Pietrobon et al., 2017).

Experimental data indicate that the selected BKPyV VP1 peptides, employed as antigens in indirect E.L.I.S.A.s, do not cross-react with JCPyV and SV40 hyperimmune sera (Pietrobon et al., 2017).

The two BKPyV VP1 synthetic peptides are:

Indirect E.L.I.S.A. was developed and standardized to detect specific antibodies against BKPyV in human sera using VP1 L and M synthetic peptides as mimotopes. A human peptide, represented by the neuropeptide S (hNPS), a.a sequence SFRNGVGTGMKKTSFQRAKS, which is BKPyV un-related, was used as a negative peptide in all indirect E.L.I.S.A. reactions (Corallini et al., 2012; Tognon et al., 2016). Peptide coating. Plates were coated with 5 μg of the selected peptide, for each well, diluted in 100 μL of Coating Buffer (Candor Bioscience, Wangen im Allgäu, Germany) at 4°C for 16 h. Peptide blocking. Blocking was made with 200 μL/well of the Blocking Solution (Candor Bioscience, Wangen im Allgäu, Germany) at 37°C for 90 min.

BKPyV viral stock was obtained in infected VERO cells, as previously done (Corallini et al., 2012). Briefly, monolayers of VERO cells grown in T75 tissue culture vessels, with RPMI 1,640 medium with 5% fetal bovine serum (FBS) and 1% penicillin-streptomycin, 90% confluent, were infected at the multiplicity of infection (m.o.i.) of 10⁻⁴ plaque forming unit (P.F.U.)/cell. BKPyV-infected cells were collected 3 weeks after infection. The viral titre, determined by Haemagglutination (HA) assay, was 1.6 × 10⁴ haemagglutinating units (HAU), corresponding to 1.6 × 10⁸ P.F.U./ml (Corallini et al., 2012; Pietrobon et al., 2017).

BKPyV working stock was employed as viral antigens in both HA and HAI assays (Corallini et al., 2012).

BKPyV titre was evaluated by HA with a solution of human erythrocytes, group 0, Rh+. These erythrocytes agglutinate in the presence of a specific concentration of BKPyV virions, i.e., they form a network that maintains red cells in suspension. In the absence of or with a low virion concentration, red cells precipitate and form a red spot on the bottom of the well (Mazzoni et al., 2012; Pietrobon et al., 2017).

Serial dilutions of the viral stock were carried out in plates, 96 round wells (Nunc, CelBio, Milan) in PBS 1x, from 1:10 at 1:5,120 dilution, in 100 μL of final volume. Then, 50 μL of 0.5 or 1% erythrocytes, were added to each viral dilution. Plates were incubated at +4°C and the H.A. titre was read 4 h later when the control, represented by erythrocytes in PBS only, had completely sedimented on the well bottom. The highest dilution of BKPyV, which gives the complete haemagglutination was considered to contain 1 HAU (Portolani et al., 1974; Corallini et al., 2012).

HAI tests the ability of a BKPyV immune serum to inhibit the haemagglutination capability of the virus. HAI employs serial dilutions (1:16, 1:32, 1:64, 1:128) of serum to determine the antibody titre. Sera were heated at 56°C for 30 min and treated with NaIO₄ (0.1 M) to remove non-specific inhibitors. Specifically, 30 μL of sera was added to 15 μL of NaIO₄ (1:2), in plates 96 round wells (Nunc, CelBio, Milan) and incubated at RT for 30 min. As a final step, 15 μL of 5% glycerine was added to each serum. Serial dilutions of the serum in PBS 1x, from 1:16 to 1:128, were mixed with 8 HAU of BKPyV as antigen. Mixtures were kept at RT for 1 h. Then, 2 volumes of 0.5% erythrocytes group 0+ were added, and plates were incubated at +4°C for 4 h. As a final step, the HI-antibody titre was determined, as described above (Portolani et al., 1974; Corallini et al., 2012).

The prevalence of BKPyV-positive sera in choroidal nevi (CN) was compared with that in healthy subjects (HS). The statistical tests employed were (i) a one way t-student test to compare serologic profile (OD); (ii) Chi square testing was used to compare binary variables; (iii) Fisher's exact test was used to compare the prevalence of antibodies anti-BKPyV in different groups. The P < 0.05 value was considered statistically significant. All statistical analyses were performed using Prism software (GraphPad, San Diego, CA).

Human sera, from CN patients (n = 71) and three groups of normal subjects, employed as controls indicated as HS1 (n = 87), HS2 (n = 144), and HS3 (n = 208; Table 1), were analyzed for IgG antibodies reacting to BKPyV VP1 mimotopes, known as VP1 L and VP1 M.

To this purpose, an indirect E.L.I.S.A. was employed using synthetic peptides as viral antigens (Pietrobon et al., 2017). These mimotopes correspond to specific BKPyV VP1 antigenic epitopes. As a control reaction, an unrelated BKPyV human synthetic peptide, known as hNPS, was used as a negative control (Corallini et al., 2012).

In the first step of this investigation, the prevalence of BKPyV antibodies was analyzed in 71 CN and 87 HS1 serum samples in a 1:1 ratio cases/controls.

A prevalence of 93.0% (66/71) was found in CN serum samples, which reacted with the VP1 L mimotope, whereas a prevalence of 88.7% (63/71) was reached with the VP1 M peptide (Table 1).

In serum samples from HS1 (n = 87), the prevalence of IgG antibodies against BKPyV VP1 L and VP M was 64.4% (56/87) and 74.7% (65/87), respectively (Table 1).

It is interesting to note that the prevalence of antibodies against BKPyV obtained with the two VP1 peptides L and M did not differ statistically within each group, which was 93.0% for peptide L vs. 88.7% for peptide M in CN group and 64.4% for peptide L vs. 74.7% for peptide M in HS1 group (Table 1). The prevalence detected in HS2 was 70.8% for peptide VP1 L and 71.5% for peptide VP1 M (Table 1), whereas it was ~73%, i.e., VP1 L (72.6%) and VP1 M (73.1%) in HS3 (Table 1).

In our study, sera were considered BKPyV VP1-positive when reacting with both mimotopes/peptides L and M.

When combining the data of BKPyV-positive sera, both for the VP1 L and VP1 M mimotopes, the overall prevalence was 87.3% (62/71) in CN and 62.1% (54/87) in HS1 (Table 1). The difference between the two prevalences, 87.3 vs. 62.1%, of the two cohorts is statistically significant (p < 0.0005).

A similar prevalence of BKPyV antibodies, 63.9 and 64.9%, was obtained in HS, when the number of control samples was double in HS2 (n = 144) and triple in HS3 (n = 208), respectively (Table 1).

BKPyV-positive sera tested by indirect E.L.I.S.A., diluted 1/20, had a general cut-off, by spectrophotometric reading, in the range of 0.17–0.19 OD. This value discriminates BKPyV-negative/-positive samples. Our indirect E.L.I.S.A. with BKPyV VP1 mimotopes was set up using rabbit BKPyV hyperimmune serum, which had an OD of up to 1.8, as a positive control. Conversely, the two negative controls, rabbits JCPyV, and SV40 hyperimmune sera, showed an OD of <0.1. A human peptide, represented by the neuropeptide S (hNPS), a.a sequence SFRNGVGTGMKKTSFQRAKS, which is BKPyV un-related, was used as a negative peptide in all indirect E.L.I.S.A. reactions. This negative control, which did not react with human sera under analysis, showed OD values in the 0.01–0.02 range, an OD reading which is expected for human sera tested BKPyV-negative (Pietrobon et al., 2017).

The two indirect ELISAs, with two distinct VP1 mimotopes gave overlapping results, thus confirming the higher prevalence of anti-BKPyV VP1 antibodies in human sera from patients affected by CN compared to controls (Table 1).

Profiles of serum antibody reactivity to BKPyV mimotopes are presented in Figure 1. Immunological data are from samples from CN affected patients and HS. Results are presented as values of optical density (OD) readings at λ 405 nm, of serum samples diluted at 1:20, detected in indirect E.L.I.S.A. In scatter dot plotting, each plot represents the dispersion of OD values to a mean level indicated by the line inside the scatter with Standard Deviation (SD) for each group of subjects analyzed. The mean OD of sera (VP1 L ± Std Error) in CN (0.354 ± 0.024) does not differ from that of HS (0.326 ± 0.008), p > 0.005, whereas the mean OD of sera (VP1 M ± Std Error) in CN (0.326 ± 0.008) is higher than that detected in HS (0.417 ± 0.021), ^***p < 0.001 (Figure 1C). The mean OD of sera (VP1 B+C ± Std Error) in CN (0.329 ± 0.015) is lower than that detected in HS (0.372 ± 0.012), ^*p < 0.05. Statistical analyses were performed using t-test.

The HAI method was also used to test for the presence of BKPyV antibodies in serum samples from CN and HS. To this purpose, sera from 71 CN and 87 HS, which had been serially diluted 1:16; 1:32; 1:64; 1:128, were analyzed by HAI. These serum dilutions were selected based on previous publications reporting that at higher dilutions BKPyV antibodies, which are present at lower titer, agglutinate human erythrocytes with a lower prevalence. Indeed, as shown in a recent publication by Pietrobon et al. (2017), the 1:128 dilution was chosen since other dilutions, such as 1:32 or 1:64, contain antibodies at higher concentrations, which may give rise to false positive reactions; on the other hand higher dilutions could carry antibodies at much lower concentrations giving false negative reactions (Mazzoni et al., 2012; Pietrobon et al., 2017). In our experience, higher dilution than 1:128 is not needed (Mazzoni et al., 2012; Pietrobon et al., 2017).

A prevalence of 91.5% (65/71) BKPyV-positive samples diluted at 1:128 was revealed in CN affected patients, while the prevalence was 64.4% (56/87) in the HS control group. In the HAI assay, the positive neutralization (immune serum) is present in those wells where human erythrocytes form a red botton/dot sedimented on the bottom. In these wells, human sera tested BKPyV-positive. The negative result (non-immune serum) is present in wells where the human erythrocytes are agglutinated by the BKPyV virion activity, thus forming a network of human red cells, which remain in suspension, showing a diffuse rose color in the solution. These sera are BKPyV-negative (data not shown).

As detected using the indirect E.L.I.S.A., the seroprevalence of BKPyV-positive samples among CN patients is higher than that determined in the control group of HS (91.5% vs. 64.4%; p < 0.001); the difference is statistically significant (Table 2).

The concordance of BKPyV antibody prevalence determined using the two different assays is 97%.

Data of this work were enclosed, in part, in the Italian patent application number I0167478/BRE-EC/rp, filed on August 9, 2016. The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.