key: cord-0803899-pa1mlf3b
authors: Nordström, Inger; Eriksson, Kristina
title: HHV-6B Induces IFN-Lambda1 Responses in Cord Plasmacytoid Dendritic Cells through TLR9
date: 2012-06-06
journal: PLoS One
DOI: 10.1371/journal.pone.0038683
sha: ec7e7937ff0f3f8561b73eb8a4d34de49e35e3ff
doc_id: 803899
cord_uid: pa1mlf3b

Human herpesvirus type 6B (HHV-6B) is a strong inducer of IFN-alpha and has the capacity to promote Th1 responses and block Th2 responses in vitro. In this study we addressed whether inactivated HHV-6B can also induce IFN lambda responses and to what extent interferons alpha and lambda affect Th1/Th2 polarization. We show that inactivated HHV-6B induced IFN-lambda1 (IL-29) but not IFN-lambda2 (IL-28A) responses in plasmacytoid DC and that this induction was mediated through TLR9. We have previously shown that HHV-6B promotes Th1 responses and blocks Th2 responses in both humans and mice. We now show that neutralization of IFN-alpha but not IFN-lambda1 blocked the HHV-6B-induced enhancement of Th1 responses in MLR, but did not affect the HHV-6-induced dampening of Th2 responses. Similarly, blockage of TLR9 counteracted HHV-6Bs effects on the Th1/Th2 balance. In addition, IFN-alpha but not IFN-lambda1 promoted IFN-gamma production and blocked IL-5 and IL-13 production in purified CD4+ T-cells. The lack of effect of IFN-lambda1 correlated with the absence of the IFN-lambda receptor IL-28Ralfa chain on the cell surface of both resting and activated CD4+ T-cells. We conclude that inactivated HHV-6B is a strong inducer of IFN-lambda1 in plasmacytoid DC and that this induction is TLR9-dependent. However, human CD4+ T-cells do not express the IFN-lambda receptor and are refractory to IFN-lambda1 treatment. The HHV-6B-induced alterations in the Th1/Th2 balance are instead mediated mainly through TLR9 and IFN-alpha.

The recently discovered type III IFNs share many of the antiviral properties of type I IFNs. The family consists of three members, IFN-lambda1 (IL-29), IFN-lambda2 (IL-28A), and IFN-lambda3 (IL-28B) and are commonly referred to as the IFNlambda family [1, 2] . All three IFN-lambdas utilize a common distinct receptor, the IFN-lambdaR, which is composed of the IL-10R2 chain and the unique IL-28Ralpha chain [2, 3] . The IFN-lambdaR is expressed at high densities on epithelial cells [3] but IL-28Ralpha transcripts might also be found in other cells including blood lymphocytes [2] . Binding of IFN-lambda to its receptor induces a signaling response similar to that obtained by type I IFNs [1] , even though the intensity of the IFN-lambda response is generally weaker [1, 4] . The anti-viral effects obtained by IFN-lambda protects against some but not all viral infections, and preferentially those that occur at mucosal surfaces [5, 6] .

Type I IFNs are pleiotropic and have, in addition to their antiviral properties, also T-cell immune-modulatory functions, e.g. in driving Th1 responses. IFN-alpha not only promotes IFN-gamma production by CD4+ and CD8+ T-cells [7, 8] but can also re-direct an already established Th2 response into a more Th1-like response [9] . IFN-lambda share some of the immune-modulatory functions of IFN-alpha. Signaling through the IFN-lambdaR induces the phosphorylation of both STAT 1 and STAT 4 [1, 4] , i.e. transcription factors involved in the development of IFN-gamma/Th1 responses [7, 10] . The main T-cell immune-modulatory function of IFN-lambda1 that has been reported is in dampening Th2 responses, in particular IL-13 [11] [12] [13] . It is however not conclusively proven that IFN-lambda has direct effects on CD4+ T-cell polarization rather than operating through accessory cells such as dendritic cells and monocytes [14] .

Human herpesvirus type 6B (HHV-6B) is the aetiological cause of exanthema subitum, a benign disease in young children characterized by high fever for 3-5 days. The virus is a strong inducer of type I IFN responses [15] and exposure to this virus alters the Th1/Th2 balance both in vitro and in vivo [15, 16] . Whether HHV-6B is also capable of inducing IFN-lambda responses is not known, and neither is the underlying mechanism for the Th1-promoting and Th2-dampening effects on CD4+ T-cell responses.

In this study we investigated whether inactivated HHV-6B could induce the production of IFN-lambda by cord plasmacytoid dendritic cells (pDC), and to what extent this production contributed to the documented shift in the Th1/Th2 balance. We show that inactivated HHV-6B induces the production of IFN-lambda1 by cord pDC in a TLR9-dependent fashion. IFNlambda however had no direct effect on human cord T-cell polarization, which correlates with the lack of expression of the IL-28Ralpha on human CD4+ T-cells. We conclude that IFN-lambda1 has no direct effects on the Th1/Th2 differentiation of human CD4+ T-cells.

We have previously shown that inactivated HHV-6B induces a strong IFN-alpha response in cord pDC, which we confirm in Fig. 1A . In addition, we show that inactivated HHV-6B also induces high levels of IFN-lambda1 from pDC (Fig. 1B) , but no or little IFN-lambda2 (Fig. 1C) . The lack of induction of IFN-lambda2 was not dependent on the kinetics, at these low levels remained constant over 72 h (Fig. 1D ). It should be noted that the sensitivity of the ELISAs varied from 10 pg/ml for IFN-alpha, 60 pg/ml for IFN-lambda1 and 100 pg/ml for IFN-lambda2. This means that we have not been able to detect potential low IFN-lambda2 responses. The HHV-6B-induced production of both IFN-alpha and IFN-lambda1 was dependent on TLR9 as it was completely abolished in the presence of a TLR9-specific inhibitor, G-ODN (Fig. 1A-B ).

Neutralization of IFN-alpha but not IFN-lambda1 blocks the HHV-6B-induced promotion of Th1 responses in cord mixed lymphocyte reactions without affecting the HHV-6-induced dampening of Th2 responses

We have previously shown that HHV-6B exposure promotes Th1 development and blocks Th2 development both in vitro and in vivo in humans and in mice [15, 16] . To assess whether IFN-alpha or IFN-lambda1 is implicated in the HHV-6B-induced Th1/Th2 shift in vitro, we performed MLR of cord pDC and CD4+ T-cells in the presence or absence of HHV-6B and either a specific inhibitor of TLR9 (G-ODN) or neutralizing antibodies to IFN-alpha or IFN-lambda1. In titration experiments, we found that at 10 ug/ ml, both these antibodies neutralized 5000 pg/ml of recombinant IFN-alpha and IFN-lambda1, respectively (not shown). As shown before [15] , the CD4+ T-cell production of IFN-gamma was increased while the production of IL-5 and IL-13 was decreased in MLR cultures exposed to HHV-6B ( Fig. 2A-C) . Neutralizing antibodies to IFN-alpha blocked the HHV-6B-induced IFNgamma responses while neutralizing antibodies to IFN-lambda1 did not have this effect ( Fig. 2A) . Addition of G-ODN, a specific blocker of TLR9 signaling, blocked the HHV-6B-induced increase in IFN-gamma production and also the HHV-6-induced dampening of IL-13 responses in these cultures (Fig. 3) . Neutralization of IFN-alpha or IFN-lambda1 did however not impact on the HHV-6B-induced dampening of IL-5 and IL-13 responses ( Fig. 2B -C).

To assess whether IFN-lambda1 shares the CD4+ T-cell immune-modulatory functions of IFN-alpha, we added recombinant human IFN-alpha and IFN-lambda1 to cultures of anti-CD3stimulated cord CD4+ T-cells and measured their production of IFN-gamma, IL-5 and IL-13. To ascertain that the recombinant cytokines used were biologically functional we first assessed their ability to induce MxA transcription in purified pDC and found that four hour incubation with IFN-alpha or IFN-lambda1 enhanced the MxA transcription 50-fold and 10-fold, respectively. Since anti-CD3 activation alone did not give rise to any measurable IL-13 responses (not shown), we added soluble anti-CD28 to these cultures. As expected, IFN-alpha had profound effects on the cytokine production profiles and promoted both IFN-gamma and IL-10 responses and blocked IL-5 and IL-13 Figure 1 . HHV-6B induces the production of IFN-alpha, IFN-lambda1 but not IFN-lambda2 in pDC in a TLR9-dependent fashion. Purified cord pDC were exposed to inactivated HHV-6B in the presence or absence of G-ODN, a TLR9-specific inhibitor. The levels of responses by the T-cells (Fig. 4) . IFN-lambda1 on the other hand did not affect the production of any of these cytokines (Fig. 4) .

IFN-lambda1, IFN-lambda2 and IFN-lambda3 act by binding to the IFN-lambdaR. We examined the expression of the IFN-lambdaR-specific IL-28Ralpha chain on pDC (Fig. 5A ), resting CD4+ cells (Fig. 5B ) and on CD4+ cells that had been activated for 24 h with anti-CD3 (Fig. 5C ) or cultured for 24 h in the presence of IFN-alpha (Fig. 5D ). We found that neither resting nor activated CD4+ T-cells expressed any detectable levels of IL-28Ralpha whereas low levels could be detected on pDC.

In this study we show that inactivated HHV-6B is a potent inducer of IFN-lambda1 but not IFN-lambda2 in pDC through a TLR9-dependent signaling pathway. In addition we show that IFN-lambda1 does not share the ability if IFN-alpha to directly alter the function of T-cells. Firstly, T-cells do not express IL-28Ralpha, i.e. the IFN-lambdaR. Secondly, addition of recombinant IFN-lambda to activated CD4+ T-cells does not change their Th1/Th2 cytokine profile. Thirdly, neutralization of IFN-lamb-da1 does not affect virus-induced alterations in the Th1/Th2 balance.

Inactivated HHV-6B was a strong inducer of IFN-lambda1 but not IFN-lambda2 in cord pDC. Even though IFN-lambda1 genes are considered to be early response genes whereas IFN-lambda2 is expressed with delayed kinetics [14] , there were no apparent IFN-lambda2 responses even at 72 h post activation. IFN-lambda2 depends on the inducible IRF7 pathway whereas IFN-lambda1 is also regulated by the constitutively expressed IRF3 [17] . Since IRF7 is constitutively expressed in pDC [18] , our data clearly show that pDC produce higher amounts of IFN-lambda1 compared to IFN-lambda2 in response to HHV-6B exposure. We have previously shown that inactivated HHV-6B can induce high levels of IFN-alpha by cord pDC [15] and the data from this study show that both the IFN-alpha and the IFN-lambda1 responses induced by HHV-6B are mediated through TLR9. This is in accordance with many other herpesviruses such as varicella zoster virus, HSV and EBV, which all induce type I IFN responses in pDC through the TLR9 pathway [19] [20] [21] .

We confirm previous studies showing that IFN-alpha has the capacity to alter the overall Th1/Th2 balance. That IFN-alpha has T-cell immune-modulatory functions is well established [7] [8] [9] and reflects the almost universal expression of the IFN-alpha/beta receptor on nucleated cells. However, when we neutralized IFNalpha in HHV-6B-exposed mixed lymphocyte reactions we only managed to influence the Th1 responses. Thus, addition of neutralizing antibodies to IFN-alpha blocked the virus-induced enhancement in IFN-gamma production without affecting the virus-induced reduction in Th2 cytokines. In contrast, addition of recombinant IFN-alpha to activated cord CD4+ T-cells affected both the Th1 and the Th2 responses. In this setting, IFN-alpha enhanced the production of IFN-gamma and reduced the production of IL-5 and IL-13. This implies that IFN-alpha indeed has the capacity to influence both Th1 and Th2 responses. The lack-of-effect of anti-IFN-alpha in enhancing the Th2 responses in the HHV-6B-exposed cord MLR could imply that other factors than IFN-alpha also has a Th2-dampening effect. In relation to this, we recently showed that enveloped viruses (in this case coronavirus, CMV, HSV-1, influenza virus and morbillivirus), but not naked virus, blocked IL-13 responses in vitro, and that this inhibition occurred independently of IFN-alpha responses [22] . This would argue for an IFN-alpha-independent modulation of IL-13 responses by virus such as HHV-6B.

IFN-lambda1 is reported to be especially efficient in dampening Th2 responses, in particular IL-13 [11] [12] [13] . In our hands, IFN-lambda1 had no such effect. When we added recombinant IFN-lambda1 to activated cord CD4+ T-cells, we could not document any effect on either Th1 (IFN-gamma) or Th2 (IL-5 and IL-13) responses. In addition, neutralization of IFN-lambda1 in HHV- Data are expressed as medians and the 25% and 75% percentile (the boxes) with the minimum and maximum responses for n = 5. * = p,0.05 using ANOVA with Bonferroni's multiple comparison test. doi:10.1371/journal.pone.0038683.g004 6B-exposed cord mixed lymphocyte reactions did not affect the levels of either Th1 or Th2 cytokines, including IL-13. We therefore decided to check for the expression of the IFN-lambda receptor on CD4+ T-cells. Resting CD4+ T-cells did not show any expression of the IL-28Ralpha chain, nor did CD4+ T-cells that had been activated with anti-CD3 or exposed to IFN-alpha. Previous studies have identified IL-28Ralpha transcripts in human T-cells [13, 23] but our data clearly show that there is no IL-28Ralpha protein expression on the cell surface on neither resting nor activated CD4+ cells. We thus conclude that IFN-lambda1 does not have direct effects on CD4+ T-cells due to the lack-of-expression of the cognate cytokine receptor. This is in line with a recent report by Arasteh et al [24] showing that IFN-lambda2 has no effect on CD25 expression or proliferation of cord CD4+ T-cells. There is however one report showing a direct effect of IFN-lambda1 on purified human CD4+ T-cells [13] . In this study it was shown that IFN-lambda not only suppressed GATA-3induced Th2 responses but also indirectly enhanced IFN-gamma responses [13] . However, the authors used negative selection for the CD4+ purification. Given that the purified cells used were not completely pure (.95%) indicates that there might have been some accessory cells left among the CD4+ T-cells [13] . If so, the effect of IFN-lambda1 could well be mediated indirectly via some other cell subset.

Monocyte-derived macrophages not monocytes or monocytederived DC express the functional IFN-lambdaR [25] . The transcript for the IL-28Ralpha has also been found in pDC [26] and we now show that pDC express low levels of IL28Ralpha on the cell surface. This indicates to us that IFN-lambda acts preferentially on certain subsets of antigen-presenting cells and that the observed effects of IFN-lambda on CD4+ T-cell differentiation [11] [12] [13] are indirect. The most plausible mode of action of IFN-lambda is through its interaction with myeloid cells [27] . This assumption is substantiated by in vitro studies showing that IFN-lambda blocks IL-13 responses and promotes IFNgamma responses through its effects on dendritic cells [11, 12] . Furthermore, IFN-lambda promotes Th1 responses and blocks Th2 and Th17 responses in vivo in mice through its modulation of the IL-12 production by lung myeloid dendritic cells [28] . The Th2 dampening and Th1 promoting effects could be adoptively transferred by IL-28A-treated CD11c + cells [28] .

We have recently shown that infection with HHV-6B before 18 months-of-age is associated with a significantly reduced incidence of allergic sensitization (OR: 0.08, 95% CI: 0.009-0.68) [15] suggesting that HHV-6B infection might protect children from allergy. Experimentally, we strengthened this hypothesis by showing that HHV-6B exposure blocks Th2 responses and allergy development in a mouse model of allergic disease [16] . In vitro we showed that HHV-6B can promote Th1 responses (IFN-gamma) and reduce Th2 responses (IL-5 and IL-13) [15] . The results from the present study indicate that these effects are mediated in part through IFN-alpha. We initially hypothesized that IFN-lambda is implicated in dampening the Th2 responses [11] [12] [13] , but this was not the case in our in vitro system. However, IFN-lambda might well play a role in reducing Th2 responses in vivo, as shown by Koltsida et al [28] .

In summary, we show that inactivated HHV-6B induces IFN-lambda1 responses in pDC through TLR9. The secreted IFN-lambda1 does however not affect CD4+ T-cells directly as human CD4+ T-cells do not express the IFN-lambdaR and are refractory to IFN-lambda1 treatment.

Virus HHV-6B strain Z29 (available from the HHV-6 foundation repository, www.hhv-6foundation.org/research/repository/ repository-reagents-available) was kindly donated by Dr Helena Dahl, SMI, Stockholm. The virus was grown in MOLT-3 cells (available at ATCC: CRL 1552) in Iscoves complete medium (Iscoves medium with 10% FBS (Biological Industries, Kibbutz Beit Haemek, Israel), 3 ug ml 21 L-glutamine (Gibco, UK), 0.1 mg ml 21 gentamycin sulphate (Essex Lä kemedel AB, Stockholm, Sweden)) containing 5 ug/ml cortisone (Solucortef, UpJohn). After 2-3 weeks, the suspensions were centrifuged at 1500 rpm. The virus-containing supernatants were then centrifuged for 1 h at 100,0006g. The viruses were resuspended in Iscoves complete medium. Viral content was determined by quantitative PCR. The virus was inactivated at 2500 rad prior to use.

Fresh cord blood pDC were isolated from cord blood mononuclear cells using the pDC isolation kit from Miltenyi Biotec (Auburn, CA). PDC were dispersed in 24 well plates (10 6 cells/ well) in the presence or absence of virus (70 genome copies/pDC) in 1 ml Iscoves complete medium. In some experiments, a TLR9 antagonist (G-ODN, 15 uM, InVitrogen) [29] was added. Supernatants were collected after 24 h, 48 h and 72 h and frozen at 270uC until assayed for cytokine content.

Cord CD4+ T-cells were isolated from pDC-depleted CBMC using the Dynal CD4 + Isolation Kit according to manufacturer's instructions (Invitrogen AB, Stockholm, Sweden) yielding .95% pure CD4+ T-cells. The cells were cultured in 96 well flat-bottom Nunc tissue culture plates (10 5 cells/well) pre-coated with 3 ug/ml anti-human CD3 (3 ug/ml, OKT-3, Ortho-McNeil Pharmaceutical, Raritan, NJ) in Iscoves complete medium in the presence or absence of anti-human CD28 (1 ug/ml, BD), recombinant human IFN-alpha (10 ug/ml; PBL interferon source) or IFN-lambda1 (10 ug/ml; Peprotech). Supernatants were collected after 48h and analyzed for cytokine content (see below).

Cord CD4+ T-cells (10 5 ) were cultured with allogeneic cord pDC (2610 4 ) in 96 well flat-bottom Nunc tissue culture plates in Iscoves complete medium together with irradiated HHV-6 (70 genome copies/pDC), in the presence or absence of G-ODN (15 uM) or neutralizing antibodies to human IFN-alpha (10 ug/ ml; PBL interferon source) or IFN-lambda1 (10 ug/ml; R&D, catnr: MAB15981). Supernatants were collected after 48 h and analyzed for cytokine content (see below).

IFN-alpha content was assessed using an ELISA kit from PBL Biomedical Laboratories. IFN-lambda1, IFN-lambda2, and IL-13 levels were determined using specific Duoset ELISAs (R&D). IFNgamma and IL-5 contents were determined using the Human Th1/Th2 Cytokine Cytometric Bead Array Kit (BD Biosciences Pharmingen, San Diego, CA) using a FacsCanto2 flow cytometer and the data were analysed using the FCAP array Software (BD Biosciences Pharmingen).

Cord cells were analyzed directly upon isolation or after 24 h incubation with IFN-alpha (5 ug/ml) or solid-phase anti-CD3 (3 ug/ml). For the staining, 10 6 cells were treated for 20 min with Fc-block (BD Pharmingen) and then incubated with anti-IL28R-PE (R&D, catalogue number FAB5260P) or a PE-labelled isotype control (mouse IgG) together with anti-CD4-Pacific blue (BioLegend) for 30 min. Stained cells were analyzed in an iCyt Eclipse (Sony) and the data generated were processed with FlowJo version 7.6.5.

Total RNA was isolated from pDC that had been cultured for 6 h with recombinant IFN-alpha or IFN-lambda1, using the RNeasy kit from Qiagen according to manufacturer's instructions. Total RNA was used for cDNA synthesis using 0.5 mg/ml random hexamer and 0.01 mM dNTP in a total volume of 12 ml. This was followed by heating to 65uC for 5 minutes, a quick chill on ice and brief centrifugation. 20-40 U/ml RNase inhibitor, 0.2 mM DTT, 1x First-Strand buffer and 200 U/ml SuperscriptRT was then added and incubated at 37uC for 50 minutes, followed by termination of the reaction at 70uC, 15 min. MxA mRNA expression levels was determined using a TaqManH Gene Expression Assay (Applied Biosystems). Primers and probes for MxA and the housekeeping gene GAPDH were purchased from Applied Biosystems, cat no. Hs00895608_m1 and Hs99999905_m1, respectively. Each qPCR was carried out in a total volume of 20 ml containing 10 ng cDNA, 0.9 mM of each primer and 0.25 mM probe under the following conditions: 50uC for 2 min, 95uC for 10 min, 95uC for 15 s, 60uC for 1 min in 40 cycles. Data was analyzed using the 7500 system software for the 7500 real time PCR system and is presented as the ratio of MxA amplificied transcripts to GAPDH amplified transcripts.

Student's t-test and ANOVA with Bonferronis multiple comparison test were performed using GraphPad Prism version 5 for Window (GraphPad Software, San Diego, USA).

These studies were approved by The Ethics Committee at the Faculty of Medicine, University of Gothenburg, Sweden. All mothers were given oral and written information, and gave oral consent to participate in the study. Written consent was not required by the Ethics Committee for this study as no personal information or identity was recorded, and the cord blood was collected from the umbilical cord after the birth of the child (law 2003: 460, paragraphs 4 and 13).

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