Experimental co-transmission of simian immunodeficiency virus (SIV) and the macaque homologs of the Kaposi sarcoma-associated herpesvirus (KSHV) and Epstein-Barr virus (EBV)

Identification of RV1/RV2-naïve macaques

Initially, the macaque colony at the WaNPRC was screened for animals that were naïve to both macaque RV1 and RV2 rhadinoviruses to serve as recipients in a pilot experimental RFHV transmission. Sera from more than 200 macaques collected during the annual colony-wide health assessment screen were analyzed using a biplexed Luminex-based serological screen detecting macaque IgG antibodies reactive with KSHV virion proteins (RV1 assay, bead set 60) and RRV virion proteins (RV2 assay, bead set 61), as previously described [65]. The anti-RV1 antibody levels ranged from 9 to 2,425 MFI, with a median of 108 MFI, while the anti-RV2 antibody levels ranged from 4 to 2,705 MFI, with a median of 401 MFI (Table 1). Sixteen animals, of which 10 were identified as juveniles less than 13 months of age from the infant colony, had very low seroreactivities in both assays. The RV1 cutoff (mean of nonreactive juvenile sera plus 5 standard deviations) was determined to be 58 MFI, while the RV2 cutoff was 95 MFI [65]. High seroreactivity was observed in 45 macaques that were part of ongoing SIV vaccine studies with RV1 values ranging from 45 to 2,425 MFI with a median of 123 (40/45 positive samples) and RV2 values ranging 447–2,705 MFI with a median of 1,973 (44/45 positive samples) (Table 1)[65]. For comparison, the colony average (67 animals) was 108 MFI (RV1; range 49–448) and 350 MFI (RV2; range 163–1980), while the specific pathogen-free (SPF3; 37 animals) colony average was 99 MFI (RV1; range 30–465) and 475 MFI (RV2; range 42–1079) (Table 1). The SPF3 colony at the WaNPRC had been developed to eliminate cercopithecine herpesvirus 1 (Herpes B), SRV-2 and simian T-cell leukemia virus [67]. From the high RV1 and RV2 serological reactivities detected in the SPF3 colony, it was clear that the macaque RV1 and RV2 rhadinoviruses had not been eliminated from this colony. Two of the juvenile macaques, K04199 (0.5 year of age; RV1: 12 MFI, RV2: 6 MFI) and M04203 (1.0 year of age; RV1: 36 MFI, RV2: 42 MFI) were chosen as naïve recipients for the RFHV transmission experiment. PBMC were obtained from both animals and tested for RV1 and RV2 DNA using highly-sensitive and specific RV1 and RV2 qPCR assays [34, 66]. The assays were negative for both animals, further supporting their naïve status.

Identification of RFHV-positive saliva donors

To identify RFHV-positive saliva donors, multiple saliva samples had been screened from 53 individual macaques at the WaNPRC over 3 years. The macaque population consisted of a mixture of pig-tailed macaques carrying RFHVMn and cynomolgus macaques carrying RFHVMf. Because high rhadinovirus serological reactivity was observed in macaques in ongoing SIV vaccine studies, saliva samples were obtained during regular testing in these studies. The saliva samples were tested for the presence of oral RV1 and RV2 DNA using specific RV1 and RV2 qPCR assays. While the majority of macaques never exhibited detectable levels of oral RV1 and RV2 rhadinovirus DNA in saliva, subsets were positive for oral RV1 (15/53) and RV2 (25/53). The maximal rhadinovirus levels ranged from 104–107 RV1 genomes/mL saliva and 103–108 RV2 genomes/mL saliva (Fig 1A). Fourteen of the 25 RV2 positive macaques had no evidence of oral RV1 DNA, while four of the 15 RV1 positive macaques showed no evidence of oral RV2 DNA (Fig 1B). Two cynomolgus macaques, 01019 and 98039. and one pig-tailed macaque, A02241, were identified as potential RFHV donors. During the course of the screening, all three of these macaques had high levels of RV1 DNA in saliva (Fig 2). Variable levels of oral RV2 DNA were occasionally detected, which were in most cases two logs or more less than RV1.

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Fig 1. qPCR Screen for RV1 and RV2 Rhadinovirus DNA in Saliva.

Saliva was obtained from macaques at the WaNPRC undergoing routine health screening and tested for the presence of RV1 and RV2 rhadinovirus DNA. A) The highest RV1 and RV2 DNA levels detected during longitudinal screening. B) Correlation of RV1 and RV2 viral loads for the animals in panel A showing a positive level of DNA for either RV1 or RV2.

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Fig 2. Longitudinal Analysis of RV1 and RV2 Rhadinovirus DNA in Saliva of Donor Macaques.

The RV1 and RV2 DNA levels in longitudinal saliva samples of donor macaques A) cynomolgus macaque 01019, B) cynomolgus macaque 98039 and C) pig-tailed macaque A02241. Saliva collected on week 0 was used in the experimental transmission studies, as indicated. The level of LCV in the week 0 saliva of 01019 is shown in panel A.

Experimental infection of naïve juvenile macaques with RFHV-positive saliva

Saliva was obtained from the two cynomolgus donors, 01019 (saliva “A”) and 98039 (saliva “C”). The 01019 and 98039 saliva samples contained 1.7 × 106 and 4.4 × 104 RV1 genomes per ml of saliva, respectively, with no detectable levels of RV2 DNA (Fig 2A, B). The 01019 saliva sample was also screened with a qPCR assay developed to detect macaque lymphocryptoviruses (LCV) [60], and was found to contain 6.6 × 10⁴ LCV genomes per ml (Fig 2A). The saliva was prepared as described in Materials and Methods and injected intravenously into the naïve juvenile pig-tailed recipients M04230 (01019 saliva “A”) and K04199 (98039 saliva “C”). Saliva was also obtained from the pig-tailed macaque donor A02441 (saliva “B”), which contained 1.2 × 10⁵ RV1 genomes per ml. This saliva was inoculated directly into the cheek pouches of both juvenile recipients (Fig 3). Thus, intravenously injected saliva would contain cynomolgus macaque viruses, while the cheek pouch inoculated saliva would contain pig-tailed macaque viruses. Saliva and blood samples were collected from the experimentally infected macaques weekly and/or bi-weekly and blood cells were counted. DNA was isolated from both saliva and peripheral blood mononuclear cells (PBMC) and RV1 and RV2 viral loads were determined by qPCR.

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Fig 3. Timeline of Experimental Infections.

The outlines of the experimental infections and treatment is shown for naïve juveniles A) K04199 and B) M04203, as described in the text and subsequent figure legends.

Experimental transmission of salivary RFHVMn and SIV to K04199

The K04199 juvenile pig-tailed macaque was injected i.v. with cell-free saliva “C” from the cynomolgus macaque 98039 that had high titers of RFHVMf DNA and received whole saliva “B” into the cheek pouches from the pig-tailed macaque A02441 that had high titers of RFHVMn DNA. Analysis of saliva by RV1 qPCR revealed a low-level signal (153 RV1 genomes/ml saliva) by 10 weeks post infection (Fig 4A). The RV2 qPCR was negative during this time frame (Fig 4B). To enhance the infection, K04199 received an additional i.v. injection of cell-free saliva “A” from the cynomolgus macaque 01019, which had high titers of RFHVMf DNA in saliva. By week 16, the RV1 qPCR assay detected 2.3 million RV1 genomes/ml saliva. By week 18, however, the RV1 DNA levels were undetectable. The animal remained negative for RV2 during this time frame. Serological analysis of the bi-weekly blood samples revealed continuous baseline levels of anti-RV1 and anti-RV2 virion IgG antibodies from weeks 0 to 23 post infection (Fig 4A, B).

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Fig 4. Experimental Rhadinovirus Infection in Juvenile Macaque K04199.

The naïve juvenile pig-tailed macaque K04199 was inoculated intravenously with diluted, filtered saliva from the 98039 cynomolgus macaque donor (Saliva C) containing high levels of the RV1 rhadinovirus (RFHVMf), and was inoculated into the cheek pouches (cp) with whole saliva from the A02441 pig-tailed macaque (Saliva B) containing high levels of RFHVMn. Subsequently, K04199 was inoculated on week 12 with diluted, filtered saliva from the 01019 cynomolgus macaque donor (Saliva A) containing high levels of RFHVMf. Saliva and blood were collected weekly and/or biweekly. A) The RV1 genome levels were determined using the RV1 qPCR assay and the RV1 antibody levels were determined using the RV1 Luminex assay. B) the RV2 genome levels were determined using the RV2 qPCR assay and the RV2 antibody levels were determined using the RV2 Luminex assay. C) The SIV cDNA levels were determined using the SIV qPCR assay and the SIV antibody levels were determined using the SIV Luminex assay. D) The absolute number of cells in the lymphocyte subsets was determined, as indicated. K04199 developed clinical signs of SIV-induced AIDS and was terminated on week 23. MFI = mean fluorescent intensity.

The amplification product from the RV1 qPCR assay on the week 16 saliva sample was sequenced yielding a 100% match with the RFHVMn sequence and an 87% match with the RFHVMf sequence. These results indicate that the K04199 pig-tailed macaque had been experimentally infected with RFHVMn, the pig-tailed macaque RV1 rhadinovirus, from the A02441 whole saliva that had been inoculated into the cheek pouches of K04199. No evidence of an RFHVMf infection from the i.v. injection of cell-free saliva from the cynomolgus macaque donors 98039 or 01019 was detected.

Since the donor macaques were all long-term non-progressors in previous SIV vaccine studies and had been challenged with SIVmneB3718, we tested the longitudinal series of PBMC from K04199 for the presence of SIV using a SIV-specific qPCR assay [68]. A peak of SIV DNA (6,600 SIV genomes/10⁶ PBMC) was detected 2 weeks after the initial saliva infection. The SIV levels were undetectable by week 4 and remained undetectable until week 17, at which time the SIV DNA level increased to 51,000 SIV genomes/10⁶ PBMC. SIV DNA remained at this level for 2 weeks at which time K04199 showed symptoms of simian AIDS. Using a Luminex-based serological assay for SIV [67], low levels of IgG antibodies to SIV virion proteins were detected by week 4 (264 MFI), peaking at week 8 (377 MFI) and dropping to baseline levels thereafter. By week 23, K04199 developed clinical signs and hematological changes meeting the end-point criteria for AIDS protocols, and euthanasia was performed. Necropsy and histopathological examination revealed AIDS-associated pathologies, including involution of lymphoid tissues, notably thymus and spleen, pneumonia due to Pneumocystis sp. and orchitis. Blood counts showed a continual drop in the level of CD4⁺/CD8⁻ T-cells from 1,700 cells/ml on Day 0 to 212 cells/ml on Day 22 (Fig 4D).

Experimental transmission of salivary RFHVMf to M04203

The M04203 juvenile pig-tailed macaque was injected i.v. with cell-free saliva “A” from the cynomolgus macaque 01019 that had high titers of RFHVMf DNA and received whole saliva “B” from the pig-tailed macaque A02441 that had high titers of RFHVMn DNA (Fig 3B). Analysis of M04203 saliva and PBMC by RV1 qPCR 4 weeks post infection revealed a low level of RV1 DNA in saliva (1,300 RV1 genomes/ml saliva) and a much greater level in PBMC (319,000 RV1 genomes/10⁶ cells) (Fig 5A). RV1 DNA in saliva and PBMC from weeks 6–10 post infection was below the level of detection. By week 16, RV1 DNA levels increased to 2,300,000 RV1 genomes/ml saliva with 27,000 RV1 genomes/10⁶ cells in PBMC. The high saliva levels maintained for two weeks, while the PBMC levels dropped to an undetectable level by week 17. During the first 16 weeks, the anti-RV1 virion antibodies remained at baseline levels but started rising sharply by week 18, reaching 3,300 MFI by week 20 (Fig 5A). During this timeframe and for the rest of the experiment, no RV2 genomes were detected by qPCR in either saliva or PBMC, and no specific anti-RV2 virion antibody response was observed. The amplification product from the RV1 qPCR assay on the week 16 saliva sample was sequenced yielding a 100% match with the RFHVMf sequence and an 87% match with the RFHVMn sequence. These results indicate that the M04203 pig-tailed macaque had been experimentally infected with RFHVMf following i.v. injection of the cynomolgus macaque RV1 rhadinovirus from the cell-free saliva of 01019. From weeks 20 to 26, the RV1 qPCR assays of both PBMC and saliva were negative and the anti-RV1 virion antibody level remained high, above 3,500 MFI.

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Fig 5. Experimental Rhadinovirus Infection in Juvenile Macaque M04203.

The naïve juvenile pig-tailed macaque M04203 was inoculated intravenously (i.v.) with diluted filtered saliva from the 01019 cynomolgus macaque donor (Saliva “A”) containing high levels of RFHVMf and low levels of MfaLCV and was inoculated into the cheek pouches with whole saliva from pig-tailed macaque A02241 (Saliva “B”), which had high levels of RFHVMn. M04203 received a second iv inoculation of saliva from 01019 (Saliva “A”) 44 weeks after the initial infection. Subsequently, whole saliva from 01019 (Saliva “A”) was administered to the cheek pouch at week 52. To activate rhadinovirus infections, M04203 was treated with daily injections of cyclosporine for 3 weeks (week 26–29) to induce immune suppression, as indicated (green bar). The animal was subsequently infected with SRV-2B and SIVMne, which have previously been associated with rhadinovirus activation and associated pathologies (see text). Saliva and blood were collected weekly and/or bi-weekly. A) The RV1 genome levels were determined using the RV1 qPCR assay and the RV1 antibody levels were determined using the RV1 Luminex assay. B) the LCV genome levels were determined using the LCV qPCR assay and the LCV antibody levels were determined using the LCV Luminex assay. C) The SRV2 cDNA levels were determined using the SRV2 qPCR assay and the SRV2 antibody levels were determined using the SRV2 Luminex assay. D) The SIV cDNA levels were determined using the SIV qPCR assay and the SIV antibody levels were determined using the SIV Luminex assay.

Identification of MfaLCV co-infection in M04203

To determine whether M04203 had been co-infected with LCV from the 01019 saliva, the saliva and PBMC samples from M04203 were screened with the LCV qPCR assay. LCV DNA was detected in the PBMC 12 weeks after the initial saliva infection (142 LCV genomes/10⁶ PBMC) and in the saliva 16 weeks after infection (27,438 LCV genomes/ml saliva) (Fig 5B). LCV DNA was continually detected in PBMC and saliva reaching 3.6 × 10³ LCV genomes/10⁶ PBMC and 1.7 × 10⁷ genomes/ml saliva by week 26. The amplification product from the LCV qPCR assay on the week 16 saliva sample was sequenced yielding a 100% match with the MfaLCV sequence. These results indicate that the M04203 pig-tailed macaque had been experimentally co-infected with both RFHVMf, the cynomolgus macaque RV1 rhadinovirus, and MfaLCV, the cynomolgus macaque LCV, via the i.v. injected cell-free saliva “A” sample from 01019. To further study the LCV infection, we developed a Luminex-based serological assay to detect macaque antibodies that cross-react with EBV virion proteins, as described in Materials and Methods. No anti-LCV virion antibodies were detected at day 0, but by week 26, low levels of anti-LCV antibodies were observed (720 MFI) (Fig 5B).

Identification of SIV co-infection in M04203

Since SIV was detected in K04199 from the saliva inoculation, which resulted in high levels of SIV DNA by week 17 and clinical signs of AIDS by week 23, we screened the PBMC samples of M04203 for evidence of a saliva-induced SIV infection. High levels of SIV DNA (2.9 × 10⁴ genomes/10⁶ PBMC) were detected in PBMC at week 16, coinciding closely with the appearance of SIV DNA in K04199 at week 17. However, unlike K04199, which continued to have high levels of SIV DNA in PBMC from week 17 to week 23, at which time it was sacrificed with clinically evident AIDS, M04203 had no detectable SIV DNA during this timeframe (Fig 5A) and showed no evidence of AIDS-associated clinical signs. Analysis of blood cells revealed consistent levels of circulating B-cells (CD20+) and T-cells (CD4+8−, CD8+4−, CD4+8+, CD3+, CD2+) through week 16 (Fig 6). However, immediately after the appearance of RFHVMf and MfaLCV DNA in saliva and PBMC and SIV DNA in PBMC on week 16, the absolute number of B-cells and T-cells dropped precipitously reaching a minimum on week 20 (Fig 6), at which time the strong anti-RV1 virion antibody and weaker anti-LCV antibody responses initiated (Fig 5A).

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Fig 6. Longitudinal Analysis of Lymphocyte Subsets in M04203.

The absolute number of cells in lymphocyte subsets was determined from the blood samples in the experimental infection of M04103 shown in Fig 5.

Cyclosporine-induced immunosuppression of M04203

Previously, cyclosporine has been used to immunosuppress macaques, resulting in a high incidence of lymphomas and post-transplant lymphoproliferative disorders associated with macaque homologs of EBV [54, 69–71]. To examine the effect of immunosuppression on the RFHVMf and MfaLCV infections, M04203 was treated daily from weeks 26–29 with cyclosporine A intramuscularly at 15 Mgs/Kg (Fig 3B). Although no RV1 DNA was detected in PBMC or saliva from week 26–32, the titer of anti-RV1 virion antibodies continued to rise increasing from 3,607 (week 26) to 4,741 MFI (week 32) (Fig 5A). This suggests that the immunosuppressive effect of cyclosporine on T-cells may have caused a low-level reactivation of the latent RFHVMf infection resulting in the expression of sufficient RFHMf virion proteins to increase the level of anti-virion antibodies, without evidence of DNA replication. While the level of antibodies to MfaLCV virion proteins continued to increase during this timeframe, no obvious effects were observed on the levels of LCV DNA in saliva or PBMC, which continued to be high (Fig 5B). A sharp peak of anti-SIV antibodies was detected after the cyclosporine treatment reaching a maximum at week 30 (762 MFI) (Fig 5D).

Co-infection of M04203 with SRV-2B

Previous studies have shown that simian retrovirus 2 (SRV-2) infection has an immunosuppressive effect on macaques and a high percentage of naturally infected animals at the WaNPRC developed high levels of RV1 and RV2 rhadinovirus infections in conjunction with rhadinovirus-associated malignancies [34, 60, 72, 73]. To examine the effect of SRV-2 on the RFHVMf and MfaLCV infections, M04203 was injected i.v. on week 32 with infectious SRV-2B (1 × 10⁷ viral genomes) that had been isolated from a naturally infected macaque (T81273) at the WaNPRC (Fig 3B). The SRV-2B strain of SRV-2 was previously associated with the long-term development of RFHV-associated retroperitoneal fibromatosis (RF) [74]. An SRV-2B-specific qPCR assay was developed to quantitate viral loads (see Materials and Methods), and antibodies to SRV-2 were quantitated using a Luminex-based assay developed previously at the WaNPRC [67]. One week after the SRV-2B infection (week 33), SRV-2B cDNA was detected in PBMC (691 SRV-2B genomes/10⁶ PBMC) (Fig 5C). Anti-SRV-2 IgG antibodies (2,737 MFI) were detected one week later (week 34) and increased to 16,386 MFI by week 36. Anti-SRV-2 antibody levels continued to increase reaching a maximum of 19,118 MFI at week 54. With the exception of minimal signals at weeks 46 and 48, SRV-2B cDNA was below the level of detection in PBMC (Fig 5C). The RV1 and RV2 qPCR assays remained negative during this time frame (Fig 5A). The anti-RV1 antibody levels continued to increase from week 28 reaching a maximum of 5,331 MFI by week 34 and dropped to 4,194 MFI by week 44 (Fig 5A). The LCV DNA levels in saliva and PBMC remained consistently high during this timeframe, while the anti-LCV antibody levels reached a maximum of 1,642 MFI at week 38 and decreased to 1,122 MFI by week 44. Two weeks after the SRV-2B infection (week 34), the anti-SIV antibody levels had dropped to 300 MFI and a low level of SIV DNA was detected (70 SIV genomes/10⁶ PBMC). Subsequently, the anti-SIV antibody levels increased to 973 MFI (week 58) and SIV DNA was no longer detected.

Secondary saliva infections of M04203

In attempts to further augment the herpesvirus infections in M04203, additional saliva “A” from 01019 was inoculated i.v. at week 44 and into the cheek pouch at week 52 (Fig 3B). While the anti-RV1 virion antibody level remained high after these treatments, reaching a maximum of 5,771 MFI (week 60), no RV1 or RV2 DNA was detected in PBMC or saliva (Fig 5A). The LCV DNA and antibody levels remained consistently high. The anti-SIV antibody levels continued to rise and no SIV DNA was detected in PBMC.

Co-infection of M04203 with SIVMne

Previous studies have shown that SIV infection has potent immunosuppressive effects on macaques resulting in the development of simian AIDS-associated malignancies, which is characterized by high levels of rhadinovirus and/or lymphocryptovirus in the tumor lesions [51, 60]. Since SIV DNA was no longer detected in PBMC at week 62, M04203 was injected i.v. with high-titer purified SIVMne on week 64 to try to induce a lentivirus-associated immunosuppression. High levels of SIV DNA were detected after the SIV inoculation reaching a maximum (1,887 SIV genomes/10⁶ PBMC) four weeks after inoculation (week 68) (Fig 5D). The level of SIV declined to 63 SIV genomes/10⁶ PBMC by week 82. The RFHVMf DNA levels in saliva and PBMC remained undetectable after the SIVMne infection and no obvious changes in LCV status were noted, as LCV DNA and anti-LCV antibody levels remained high.

Quantitation of blood lymphocytes in M04203

The M04203 blood lymphocytes were immunophenotyped and quantitated in the longitudinal samples. An increase in the various T-cell subsets was observed 2 weeks after the initial saliva inoculation (Fig 6A). Four weeks after the appearance of high levels of RFHVMf, MfaLCV and SIV at week 16, a dramatic reduction in the level of the T-cell and B-cell subsets was observed, which rebounded by week 26. A second increase in the circulating T-cell subsets was detected 2 weeks after the experimental SRV-2B infection. This increase was followed by a dramatic reduction in the T-cell and B-cell subsets 7 weeks after the SRV-2B infection (week 40). The T-cell and B-cell populations again rebounded quickly showing some variation through week 82 (Fig 6A), which did not show any correlation with saliva inoculations or SIVMne infection. Throughout the experimental time frame, the level of CD4⁺CD8⁻ T-cells remained high (Fig 6), showing no evidence of lentivirus induced immunosuppression, contrasting to the situation observed in K04199 (Fig 4D).

Long-term monitoring of M04203 and dexamethasone treatment

Blood and saliva samples of M04203 were continually collected for 209 weeks (~ 4 years) after the initial saliva inoculation, at which time the experiment was terminated and the animal was culled. Prior to termination, M04203 was treated with dexamethasone 2 mg/kg/day for 7 days (weeks 164–165) and then with 1 mg/kg/day every three days (week 165 to week 179) after which the treatment tapered 10% per week until the dose was 0.1 mg/kg/day by week 201 (see Fig 3). Dexamethasone is a glucocorticoid agonist that has multiple anti-inflammatory and immunosuppressive functions [75]. The CD4/CD8 ratio of M04203 remained relatively constant (~ 0.8) until the initiation of dexamethasone treatment at week 164, at which point the ratio dropped precipitously reaching a level of 0.08 by week 176 (Fig 7D). The CD4/CD8 ratio varied between 0.1 and 0.2 during the treatment period and rose slightly by week 209 (0.35). Until week 164, the total neutrophil and monocyte counts remained constant while the lymphocyte counts decreased slowly to 50% of the initial values (Fig 7C). Dexamethasone treatment induced high levels of circulating neutrophils, which returned to baseline after treatment, while a concomitant and significant drop in lymphocyte counts was observed (Fig 7C). The lymphocyte numbers rebounded during the later stage of the tapered drug treatment and the monocytes showed a transient increase.

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Fig 7. Complete Longitudinal Analysis of the Experimental Infection of M04203.

The juvenile macaque M04203 was experimentally inoculated with saliva from the donor macaques as indicated in the legend to Figure 5. Blood and saliva samples were collected weekly and/or biweekly until the experiment was terminated 209 weeks after the initial saliva inoculation and M04203 was culled. At week 164, the animal received a course of dexamethasone treatment as indicated in the text and Figure 3. A) The RV1 genome levels were determined using the RV1 qPCR assay and the RV1 antibody levels were determined using the RV1 Luminex assay. B) the LCV genome levels were determined using the LCV qPCR assay and the LCV antibody levels were determined using the LCV Luminex assay. C) The absolute count of neutrophils, monocytes and lymphocytes was determined. D) the CD4/CD8 ratio was determined from the lymphocyte count.

The effects of dexamethasone on the blood cell populations had no obvious effect on the RFHVMf infection, as no RV1 DNA was detected in saliva or PBMC during the remainder of the experiment (Fig 7A). The high levels of anti-RV1 virion antibodies detected during the first 80 weeks after the initial saliva inoculation slowly decreased achieving a relatively stable level of ~2,000 MFI during the next 100 weeks (Fig 7A). The RV1 antibody levels dropped to 800 MFI during the dexamethasone treatment period and restabilized at ~1,500 MFI after treatment. From weeks 80 to 180, the levels of LCV in saliva and PBMC and the levels of anti-LCV virion antibodies remained high (Fig 7B). Dexamethasone treatment decreased the anti-LCV antibody levels, which rebounded similar to that seen with the anti-RV1 antibodies. An initial drop in the level of LCV DNA in saliva was observed after the dexamethasone treatment (1.7 × 10⁵ to 1.1 × 10³ LCV genomes/ml saliva). The LCV DNA level rebounded to 2 x 10⁶ LCV genomes/ml saliva during the tapering stages of the dexamethasone treatment but dropped to 600 at week 209. At this time, the level of LCV DNA in PBMC was equivalent to the level before dexamethasone treatment (~10⁴ LCV genomes/10⁶ PBMC).

At necropsy the tissues and organs of M04203 were grossly unremarkable, with no evidence of disease processes. Analysis by qPCR revealed no evidence of RV1 or RV2 DNA in saliva, PBMC, ileocecal junction, liver, mesenteric lymph nodes, salivary gland, spleen or tonsil (Table 2). In contrast, LCV DNA was detected in both saliva (657 LCV genomes/ml saliva) and PBMC (11,049 LCV genomes/10⁶ PBMC) at the time of necropsy and low levels of LCV were detected in the tonsil, mesenteric lymph node, salivary gland, and spleen (Table 2).

Cells

Raji cells (P8) were obtained from M. Thouless (UW) and cultured in RPMI at 37 ^oC.

Animals

All macaques (M. nemestrina and M. fascicularis) were housed at the Washington National Primate Research Center (WaNPRC) from 2005–2009 in accordance with standards of the American Association for Accreditation of Laboratory Animal Care and the experimental protocol3146-03 was approved by the University of Washington Institutional Animal Care and Use Committee. The animals were restricted to protected contact due to veterinary and research staff concerns regarding potential injury and spread of infection. They were fed a nutritionally balanced diet of monkey biscuits twice per day, participated in the WaNPRC Environmental Enhancement Plan, and were provided enrichment items on a daily basis. The research adhered to the American Society of Primatologists Principles for the Ethical Treatment of Nonhuman Primates. All animals were housed indoors on a 12-hr light cycle. The subjects were housed in two-tiered stainless steel cages, complying with Animal Welfare Act USDA standards for NHPs based on animal weight. The animals were observed daily by trained animal care staff, and underwent ketamine-sedated physical examination including CBC/serum chemistry monthly.

Blood and saliva samples were obtained under anesthesia using Ketamine. Experimental endpoints were in accordance with the University of Washington IACUC-approved AIDS Monitoring Protocol, which is a scoring system based on body weight changes, CD4 counts, hematocrit and clinical concerns identified by the veterinary staff. Euthanasia was performed using an overdose of pentobarbital, while under ketamine anesthesia in accordance with AVMA guidelines, and all efforts were made to minimize suffering.

Plasma samples were obtained during the biannual health screening of macaques at the WaNPRC and tested with the RV1 and RV2-specific Luminex assays for evidence of RV1 and/or RV2 rhadinovirus infections, which are endemic in the colony [65]. Two juvenile M. nemestrina M04203 (1.0 years) and K04199 (0.5 years) were determined to be naïve for both macaque RV1 and RV2 rhadinovirus infections by Luminex-based serological and qPCR molecular assays. Twenty adult macaques in concurrent SIV/SHIV vaccine and therapeutic research protocols were identified as possible RFHV+ donors with high titers of anti-RV1 antibodies. Three adult long-term non-progressors in these studies, M. fascicularis 01019 and 98039 and M. nemestrina A02241, were identified as RFHV+ donor animals as they exhibited high levels of RV1 rhadinovirus DNA in saliva by qPCR.

Saliva collection

During routine blood draws after ketamine sedation, saliva samples were collected by keeping the macaques in a face-down position allowing the saliva to drip into a petri dish. To obtain saliva for the experimental transmission studies, donor macaques were given 5 mg of pilocarpine 30 minutes before administration of ketamine to induce salivation. The animals were carefully monitored to prevent choking. Saliva was collected and cells were removed from saliva of 98039 and 01019 by centrifugation at 800 × g for 10 min. The supernatant was diluted 1:1 with sterile PBS and filtered through a 0.45 μ. Whatman syringe filter, which is designed for viscous solutions.

Inoculation of naïve macaques

The saliva preparation from 01019 (3.25 ml) was injected i.v. into M04203 and saliva from 98039 (3.75 ml) was injected i.v. into K04199. Unfiltered whole saliva from A02241 was inserted into the cheek pouches of both M04203 and K04199. Saliva and blood samples were collected weekly and/or bi-weekly from M04203 and K04199. At week 23 post infection, K04199 developed clinical signs meeting the end point criteria for AIDS protocols and was terminated. At weeks 26–29 after the initial saliva infection, M04203 was treated with a regimen of cyclosporine A (15 mgs/kg) IM daily to induce immunosuppression. M04203 was infected with SRV-2B at week 32 and with SIVMne at week 64 to further induce immunosuppression. M04203 was administered dexamethasone 2 mg/Kg daily for 7 days (week 164–165) and then 1 mg/Kg every 3 days from week 166 to week 179 then tapering doses to 0.1 mg/Kg by week 200. M04203 was euthanized at the end of the protocol, week 209. The animals were necropsied and the organs and tissues were examined microscopically.

SRV-2B isolation and infection

Raji cells were cultured with a frozen buffy coat sample from macaque T81273 diagnosed with KS-like retroperitoneal fibromatosis tumors, obtained from C.-C. Tsai (WaNPRC), and a single infectious clone of SRV-2 (RFS-4) was obtained. Sequence analysis revealed that this SRV-2 clone belonged to the SRV-2B strain associated with the development of retroperitoneal fibromatosis and reactivation of RFHV [74]. At week 32, M04203 was inoculated i.v. with the RFS-4 SRV-2B clone (1 × 10⁷ viral genomes).

SIVMne infection

Purified preparations of SIVMne that have been used in previous SIV vaccination studies [78, 79] were obtained from S.-L. Hu (WaNPRC). Macaque M04203 was inoculated i.v. at week 64 with SIVMne at 20 50% macaque infectious doses.

Antibody reagents

Phycoerythrin-labeled anti-human IgG (Jackson ImmunoResearch Laboratories) was used to detect IgG in macaque serum in the Luminex assays.

Viral load and blood cell quantitation

Blood cell counts and immunophenotyping were performed by the WaNPRC Central Core. PBMC and plasma were separated from blood by gradient centrifugation using Lymphoprep separation medium (Invitrogen). DNA was isolated from PBMC and saliva samples and viral loads were determined using real-time qPCR with TaqMan primers and probes. The SIV qPCR assay [68] and the RV1 [66] and RV2 [34] rhadinovirus assays have been described previously. The SRV-2B qPCR was developed using the forward primer SRV2B-a 5’ CCCGAATTACGATACCAC 3’, the reverse primer SRV2B-b 5’ GTAGCAGTAAGAAGATTAAAGG 3’ and Taqman probe 5’ 56-FAM/TTAGCTTTGCCTAAGGCCCGTG/3BHQ_1 3’ (Integrated DNA Technologies, Inc./ Coralville, IA). The PCR reaction conditions were the same as for the RV2 qPCR and OSM qPCR assays, allowing simultaneous assay runs. The PCR efficiency of the SRV-2B assay was 99.2% (data not shown).

Viral copy number per cell was determined using a qPCR assay targeting oncostatin M (OSM), a single copy cellular gene [66]. The copy number for each assay was calculated from the cycle threshold (C_t) using the Bio-Rad software. The viral load was determined as a cellular genome copy equivalent using the formula:

Viral load (genome equivalent copies) = Viral copy number/diploid OSM copy number Samples were assayed in duplicate and the means were determined.

Luminex serological assay

The high throughput multiplex RV1 and RV2 Luminex serological assays were described previously [65]. The EBV Luminex assay was similarly developed using the EBV (B95–8 strain) purified viral lysate (Advanced Biotechnologies, Inc) coupled to Luminex beads. Briefly, the Luminex bead sets coupled to RV1 (KSHV), RV2 (RRV), or EBV virion proteins were incubated with heat-inactivated serum or plasma diluted 1:50 in PBS. Bound antibody was detected using the phycoerythrin-labeled mouse anti-human IgG monoclonal antibody in the Luminex 200HT system (Luminex). The SIV and SRV-2 Luminex assays were performed by the WaNPRC core, as published previously [67].

Data Analysis

The GraphPad Prism software (San Diego, CA) was used for statistical analysis. For the Luminex data, a cut-off limit of 58 MFI (RV1 assay) and 95 MFI (RV2 assay) was derived from the mean of the non-reactive juvenile sera (RV1 = 9 sera; RV2 = 10 sera) plus 5 standard deviations, as described previously [65].