INTRODUCTION

The human gammaherpesviruses (GHVs), Epstein-Barr virus (EBV, human herpesvirus 4) and Kaposi sarcoma herpesvirus (KSHV, human herpesvirus 8), are the etiologic agents of numerous lymphomas and carcinomas that are a significant clinical burden to immune-compromised individuals, including people living with HIV. Even in immune-competent individuals, infection with EBV may manifest as infectious mononucleosis and increase the risk for the development of multiple sclerosis, an autoimmune disorder involving inflammation and neurodegeneration in the central nervous system (1). B cells are a long-term reservoir for GHV, and these viruses usurp host processes such as proliferation and differentiation to facilitate chronic infection (2–5). The identification of host factors that support latency and facilitate the emergence of GHV-driven malignancies is paramount as there are currently no treatments that directly target the latent phase of infection.

A hallmark of GHV infection and GHV cancers is the rapid and persistent activation of signal transducer and activator of transcription 3 (STAT3) (6). STAT3 is a master regulator of multiple cellular processes such as proliferation, apoptosis, and metastasis (7, 8). Constitutive STAT3 activation is reported in multiple human cancers (9, 10). Cytokines are potent activators of STAT3 in both cancer and immune cells. For instance, IL-6 induces the expression of STAT3-target genes responsible for proliferation and survival supporting tumorigenesis, while IL-10 reduces immune cell function and inflammation in some contexts (11, 12). The human GHVs use diverse strategies to promote STAT3 activation (6). EBV transmembrane protein LMP1 activates NF-κB through recruitment of cytoplasmic signaling adaptors leading to IL-6-driven STAT3 activation and cell survival (13, 14). EBV LMP2A activates STAT3 through multiple host factors to promote proliferation and survival (15, 16). The viral homologs of host cytokines, EBV vIL-10 and KSHV vIL-6, and the KSHV vGPCR also activate STAT3 (17–21).

Due to their narrow host range, the study of EBV and KSHV is largely restricted to cell culture and humanized mouse models. For that reason, murid herpesvirus 4, more commonly known as murine gammaherpesvirus 68 (MHV68), is used as a model pathogen. MHV68 is colinear with KSHV, encoding 64 direct homologs, establishes long-term latency in memory B cells, and induces lymphoproliferation in immunosuppressed mice (5). The infection of mice with MHV68 is a genetically tractable system to study virus-host interactions in specific cell types during the acute or chronic phase of infection in a natural host. Viral and host factors such as NF-κB signaling pathways support the establishment and latency in B cell compartments (5, 22–27).

The interplay of viral and host factors aids in the establishment and expansion of GHV latency, taking particular advantage of B cell processes occurring during the germinal center (GC) reaction. The GC is the site within secondary lymphoid tissues where B cells undergo maturation and differentiation processes including somatic hypermutation and class switch recombination, leading to the production of high-affinity and long-lived memory B cell and plasma cell subsets (28, 29). GHVs both engage and circumvent the GC B cell selection process to promote access to the memory B cell long-term latency reservoir for EBV and likely for KSHV (30–33); events that transpire in the GC may contribute to B cell lymphomas with post-germinal center signatures (34–36). At the peak of latency establishment ~16 days post-infection (dpi), MHV68 is predominantly found in B cells bearing GC markers (22). T follicular helper cell production of IL-21 is required to support MHV68 latency establishment in GC B cells (24), while Blimp-1 is required to access the post-GC plasma cell compartment that is a source of virus reactivation (37). The MHV68 viral M2 protein promotes host IL-10 production through the nuclear factor of activated T cells (NFAT) pathway, promoting proliferation and differentiation, driving B cells to a plasmablast-like phenotype in vivo (38–40). MHV68 RTA protein encoded by ORF50 acts synergistically with STAT3 to increase transcriptional activity in response to IL-6 (41). Given the critical role of STAT3-activating cytokines IL-10 and IL-21 in MHV68 infection (24, 38) and the evolutionary investment by the GHVs to subvert STAT3 signaling, we sought to further dissect the role of STAT3 in GHV latency establishment in vivo.

We previously used a mouse model in which STAT3 is ablated specifically in the CD19+ B cell compartment to discover that STAT3 is a crucial host determinant of MHV68 latency establishment in B cells in vivo (42). In the present study, we more closely examined virus latency in GC subsets and virus-specific adaptive immune responses in two independent strains of CD19^cre/+Stat3^f/f mice to eliminate possible strain variation. We identified disordered GC architecture in B cell-specific STAT3 knockout (KO) mice, along with reduced virus-specific antibody production, concomitant with a heightened CD8+ T cell response. This aberrant immune response in the absence of STAT3 signaling in B cells led us to use a mixed bone marrow (BM) chimera approach wherein mice are reconstituted with hematopoietic cells from wild-type (WT) and B cell-specific STAT3 KO mice. Infection of mixed bone marrow chimeric mice revealed that B cells lacking STAT3 could not compete with their wild-type counterparts to support GHV latency. To gain mechanistic insight into the transcriptional consequences of STAT3 loss, we sorted STAT3 WT and KO GC B cells, with or without infection, and quantified gene expression profiles with RNA sequencing. We identified numerous host gene pathways altered by STAT3 that intersect processes of B cell biology and host response to infection.

RESULTS

Loss of STAT3 in B cells disrupts gammaherpesvirus latency and leads to abnormal GC structure

Mice with loxP-flanked exons of Stat3 (Stat3^f/f) that are crossed with mice expressing Cre recombinase under the control of the endogenous CD19 promoter exhibit loss of STAT3 only in CD19+ B cells (43). Our lab previously reported that the conditional knockout of STAT3 in B cells led to a severe defect in the establishment of MHV68 latency in the spleens of mice after intranasal or intraperitoneal (IP) infection (42). In this study, we compared MHV68 latency in two strains of B cell-specific STAT3 knockout mice that differ by the location of loxP sites that flank exons of the Stat3 gene (Fig. 1A) (44, 45). Consistent with our previous report for the CD19^cre/+Stat3^f/f-1 mice, the CD19+ B cell population of the CD19^cre/+Stat3^f/f-2 mice lacked detectable levels of STAT3 protein by immunoblot (Fig. 1A). For brevity, Stat3^f/f mice will be referred to as WT mice, and their littermate CD19^cre/+Stat3^f/f mice will be referred to as B cell-STAT3 KO mice. STAT3 tyrosine 705 (Y705) phosphorylation is the classical indicator of STAT3 activation, and this activation has been demonstrated in response to human GHV infection in cell culture with endothelial, dendritic, and B cell models (46–49). We used intracellular flow cytometry staining of splenocytes from infected mice to reveal a higher level of STAT3-Y705 phosphorylation in B cells from the spleens of infected WT mice compared to the infected littermate B cell-STAT3 KO mice (Fig. 1B).

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FIG 1 STAT3 is necessary for the efficient establishment of latency in B cells of infected mice. (A) Schematic of loxP-flanked exons of the Stat3 locus in two strains of CD19cre/+Stat3f/f mice. Immunoblot confirmation of STAT3 loss in CD19+ B cells of CD19cre/+Stat3f/f-2 mice, but not CD19- non-B cells, as previously described for CD19cre/+Stat3f/f-1 mice (42). (B–F) Stat3f/f and CD19cre/+Stat3f/f mice were infected with 1,000 PFU MHV68-H2bYFP by intraperitoneal inoculation and evaluated at 16 days post-infection. (B) Intracellular staining of STAT3-Y705 phosphorylation in B220+ B cells of naive or infected mice evaluated as frequency of pSTAT3+ B220+ cells (left panel) and mean fluorescence intensity (MFI, right panel). (C) Weights of spleens from naive or infected mice. (D) Flow cytometry gating strategy (left panel) of infected (YFP+) B cells (CD19+CD3−) and enumeration of frequencies in each strain of mice (right panel). For B–D, each symbol represents an individual mouse; bars represent mean ± SD. Data shown represent two to three independent experiments performed with three to seven mice per infected group and one to two mice for naive groups. (E) Single-cell suspensions of spleen cells were serially diluted, and the frequencies of cells harboring an MHV68 genome were determined using a limiting dilution PCR analysis. (F) Reactivation frequencies were determined by ex vivo plating of serially diluted cells on an indicator monolayer. Cytopathic effect (CPE) was scored 3 weeks post-plating. For the limiting dilution analyses (E, F), curve fit lines were determined by non-linear regression analysis; frequency values were determined by Poisson analysis, indicated by the dashed line. Symbols represent the mean ± SEM. Statistical significance was evaluated by two-tailed unpaired t test (B, C, D) or paired t test of the calculated frequencies (E, F). *P < 0.05; **P < 0.01; ***P < 0.001; ****P < 0.0001.

We previously reported that the loss of STAT3 in B cells did not affect acute replication of MHV68 in the lungs of mice after intranasal infection but led to such a profound defect in latency establishment in the spleen that infected B cells were barely at the limit of detection (42). Here, we aimed to investigate the phenotype of infected B cells in the absence of STAT3, requiring us to use the more permissive IP route of infection to enable sufficient infected cells for analysis. At 16 dpi, the peak of the early phase of splenic latency, infected mice exhibit an enlargement of the spleen that follows colonization of that tissue with MHV68 (5). Spleens from both strains of B cell-STAT3 KO mice were significantly reduced in mass upon infection compared to the fourfold increase in mass observed upon infection of WT animals (Fig. 1C). The MHV68-H2bYFP recombinant virus utilizes a CMV immediate early promoter, driving constitutive expression of a histone 2b-YFP fusion protein and enabling direct analysis of infected cells (22). Consistent with the defect in splenomegaly, the frequency of B cells that expressed the YFP viral reporter gene determined by flow cytometry was reduced by three- and twofold in the spleens of the strain 1 and strain 2 B cell-STAT3 KO mice, respectively, when compared to their WT littermates (Fig. 1D). This defect in latency was confirmed by a limiting dilution nested PCR assay to quantify the frequency of B cells harboring the viral genome. A 6.6-fold defect in the frequency of infected splenocytes that harbor the MHV68 genome was observed for CD19^cre/+Stat3^f/f-2 mice (1 positive event per 1,688 cells, 1/1,688) compared to Stat3^f/f-2 WT mice (1/256) (Fig. 1E). Furthermore, in a limiting dilution reactivation assay, a 10- and 20-fold defect in spontaneous reactivation was observed upon explant of splenocytes from strain 1 and strain 2 of B cell-STAT3 KO mice compared to their WT counterparts, respectively (Fig. 1F). This reactivation defect largely mirrors the differences in latency at 16 dpi. A time course analysis of YFP+ B cells spanning 10–15 dpi was performed in strain 2 B cell-STAT3 KO mice. The absence of STAT3 led to a trend in decreased splenomegaly and a significant reduction in B cell infection as early as 12 dpi compared to WT counterparts (Fig. S1). These results confirm the importance of STAT3 in B cells for the efficient establishment of MHV68 latency in two strains of CD19^cre/+Stat3^f/f mice.

The GC reaction represents an anatomical structure within secondary lymphoid organs in which activated B cells undergo clonal selection and affinity maturation. Additionally, most MHV68-infected cells express GC B cell markers at the peak of latency (22). Thus, we further examined GC B cell infection and latency in B cell-STAT3 KO animals. Compared to WT littermates, B cell-STAT3 KO exhibited increased frequencies of GC B cells (defined here as GL7+CD95^hi of CD19+ cells) at 16 dpi (Fig. 2A). Although there was a reduction in the frequency of YFP+ B cells in B cell-STAT3 KO mice (Fig. 1D), we observed no significant difference in the frequency of YFP+ cells that displayed a GC phenotype (Fig. 2B). GC B cells can be roughly subdivided into rapidly proliferating centroblasts (CXCR4+CD86−) that are found in the dark zone and mature, non-dividing centrocytes (CXCR4− CD86+) in the light zone. By flow cytometry, infected WT mice had a 2:1 ratio of respective centroblast:centrocyte populations (Fig. 2C). However, in the absence of B cell-STAT3, we observed decreased frequencies of centroblasts in both GC B cells and YFP+ GC B cell populations that resulted in a ratio closer to 1:1 (Fig. 2C).

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FIG 2 STAT3 loss in B cells leads to an aberrant germinal center response upon infection. Stat3f/f (WT) and CD19cre/+Stat3f/f (B cell-STAT3 KO) mice were infected with 1,000 PFU MHV68-H2bYFP by intraperitoneal inoculation and evaluated at 16 dpi. (A) Flow cytometry gating strategy (left panel) and quantitation (right panel) of the frequencies of GC B cells (GL7+ CD95+ of CD19+ CD3−). (B) Flow cytometry gating strategy (left panel) and quantitation (right panel) of the frequencies of infected YFP+ cells bearing GC markers. (C) Flow cytometry gating strategy (upper panel) of dark zone centroblasts (CXCR4+ CD86−) and light zone centrocytes (CXCR4− CD86+) as a frequency of GC B cells from naive or infected mice, and infected YFP+ B cells from infected mice. Quantitation of the frequencies of centroblasts of GC B cells from naive or infected mice, and infected YFP+ B cells (lower panel). (D) Confocal microscopy of frozen spleen sections from naive mice (left panels) or infected mice (right panels) with STAT3 (Stat3f/f-2, top panels) or without B cell STAT3 (CD19cre/+Stat3 /f-2 mice, bottom panels) at 16 dpi to identify stromal cells (ERTR7, red), follicular dendritic cells (FDCs, blue), B220+ B cells (magenta), GC B cells (GL7, white), and MHV68-H2bYFP infection (green). Scale bars = microns. (E) Flow cytometry gating strategy (left panel) and quantitation (right panel) of the frequencies of plasma cells (CD138hiB220lo gated on CD3−). (F) Flow cytometry gating strategy (left panel) and quantitation (right panel) of the frequencies of infected YFP+ cells with plasma cell markers. Data shown represent the mean ± SD of two to three independent experiments performed with four to seven mice per infected group and one to two mice for naive groups. Each symbol represents an individual mouse. Square symbols represent CD19cre/+Stat3f/f-1 mice, while circle symbols represent CD19cre/+Stat3f/f-2 mice. Statistical significance was evaluated by two-tailed unpaired t test. ***, P < 0.001; ****, P < 0.0001.

To further explore the increase in GC B cells of infected mice lacking B cell-STAT3, we examined GC architecture in the spleens by immunofluorescence (Fig. 2D). MHV68 infection of WT mice has previously been shown to result in the formation of visible, compact GCs within the splenic follicles (22). Interestingly, the B cell follicles appeared smaller and more diffuse in B cell-STAT3 KO mice than in WT spleens, even in uninfected animals. Upon infection, GC B cells did not remain in characteristic compact foci in B cell-STAT3 KO mice, instead appearing dispersed throughout the follicle and overlapping extensively with the follicular dendritic cell (FDC) network. In both WT and B cell-STAT3 KO mice, most of the YFP+ cells also expressed the GC marker GL7. These data indicate that STAT3-KO in B cells alone led to a significantly altered splenic architecture.

B cells typically exit the GC as class-switched, long-lived memory B cells or antibody-secreting plasma cells. STAT3 coordinates the upregulation of Prdm1, encoding Blimp-1, a master regulator of B cell differentiation into plasma cells in response to IL-21 (50, 51). Plasma cells are a source of MHV68 reactivation in the spleen (52). Therefore, we examined plasma cell frequency and infection in the B cell-STAT3 KO mice (Fig. 2E). The frequency of B220^loCD138+ plasma cells between WT and B cell-STAT3 KO mice was similar (Fig. 2E), but we observed a marked reduction (>50%) in YFP+ B cells with a plasma cell phenotype in the B cell-STAT3 KO mice (Fig. 2F). Together, the increase in GC cells, the altered GC structure, and decrease in YFP+ plasma cells clearly indicate that broad GC defects occur in the absence of B cell-STAT3. Collectively, this deeper analysis of two strains of B cell-STAT3 KO mice confirmed the requirement for STAT3 to promote B cell latency and revealed shifts in B cell subsets of the GC at 16 dpi. Because we observed similar latency and immune responses in both strains of mutant STAT3 mice, we proceeded with CD19^cre/+Stat3^f/f-strain 2 mice for the remainder of the study.

Absence of STAT3 leads to dysregulated B and T cell responses at 42 dpi

Due to observed immune perturbations in B cell-STAT3 KO mice at the early phase of chronic infection, we analyzed the B and T cell responses at a later 42 day timepoint. Mice produce virus-specific antibodies in response to MHV68 infection through a CD4+ T cell-dependent process (53, 54). The serum IgG levels were comparable between WT and B cell-STAT3 KO mice (Fig. 3A), but there was a significant decrease in virus-specific IgG in the serum of B cell-STAT3 KO mice (Fig. 3B). Accompanying this decrease, serum from B cell-STAT3 KO mice had a significantly reduced neutralization capacity by plaque reduction assay (Fig. 3C).

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FIG 3 Reduced antibody response and heightened T cell response to MHV68 infection in B cell-STAT3 knockout mice. Stat3f/f (WT) and CD19cre/+Stat3f/f-2 (B cell-STAT3 KO) mice were infected with 1,000 PFU MHV68-H2bYFP by intraperitoneal inoculation and evaluated at 42 dpi. (A–B) Total serum IgG (A) or virus-specific IgG (B) from naive or MHV68-infected Stat3f/f and CD19cre/+ Stat3f/f mice measured by ELISA. (C) Virus neutralization in serum as determined by a plaque reduction assay. The PRNT50 value is the dilution of serum to reach 50% neutralization of plaques. Symbols represent samples pooled from three independent experiments as biological replicates, each performed in technical triplicate. (D) Flow cytometry gating strategy for phenotyping short-lived effector CD8+ T cells (SLECs). (E) KLRG1+CD127− (SLEC) of CD8+ TCRβ+ T cells by percentage of splenocytes (left panel) and total numbers per spleen (right panel). (F) Flow cytometry gating strategy for p79 tetramer+CD44+ (virus-specific) SLECs. (G) Total p79 tetramer+ CD44+ (virus-specific) of CD8+ TCRβ+ per spleen. (H) Analysis of virus-specific SLECs by percentage of spleen (left panel) and total numbers per spleen (right panel). Data shown represent the mean ± SD (A, B, E, G, and H) of two to three independent experiments performed with four to seven mice per infected group and one to two mice for naive groups. For A, B, E, G, and H, each symbol represents an individual mouse. Statistical significance was evaluated by two-tailed unpaired t test (A–C, E, G, H). **, P < 0.01; ****, P < 0.0001.

We previously reported that the latency defect in B cell-STAT3 KO mice was maintained even during the maintenance phase of infection at 42 dpi (42), and we confirmed this for CD19^cre/+Stat3^f/f-2 mice (Fig. S1). T cells and effector cytokines such as interferon (IFN)-γ control viral load during chronic infection with MHV68 (55). Activated, antigen-stimulated CD8+ T cells proliferate and differentiate into short-lived effector T cells or memory precursor effector T cells in response to infection. The B cell-STAT3 KO mice had an increase in short-lived effector T cells by both percentage and total numbers when compared to their WT littermates 42 dpi (Fig. 3D through E). We quantified the number of CD44^hiCD8+ T cells binding to MHC class I tetramers presenting the immunodominant epitope p79 derived from MHV68 ORF61 (Fig. 3F). The spleens of B cell-STAT3 KO mice had twice the number of p79-specific CD8+ T cells (Fig. 3G), and a greater proportion of these virus-specific T cells were short-lived effector T cells compared to WT mice (Fig. 3H). These unexpected aberrations in both the humoral and cell-mediated immune response confounded further mechanistic studies of B cell-STAT3 as a latency determinant and led us to develop an alternative mouse model to identify the B cell-intrinsic roles for STAT3.

Infection of a mixed bone marrow chimeric mouse model reveals B cell-intrinsic role for STAT3 in GHV latency establishment

Application of mixed BM chimeras to MHV68 infection has yielded important insight into the effects of B cell host determinants on infection (24, 26, 56). To better define the B cell-intrinsic role of STAT3, we generated mixed BM chimeras to analyze MHV68 latency in the context of the same adaptive immune response within each animal. To do this, CD45.2+ BM from Stat3^f/ftdTomato^stopf/f mice (WT STAT3 B cells) and from CD19^cre/+Stat3^f/ftdTomato^stopf/f mice (STAT3 KO B cells) was mixed 1:1 and transferred into CD45.1+ recipients that had been irradiated for myeloablation (Fig. 4A). The tdTomato^stopf/f reporter results in tdTomato red fluorescent protein production after Cre recombinase expression. In the CD19^cre/+Stat3^f/ftdTomato^stopf/f mice, tdTomato expression marks B cell with STAT3 deletion, allowing for discrimination of STAT3 WT B cells and KO B cells. Sorted tdTomato+ B cells were analyzed by immunoblot to confirm the loss of STAT3 protein specifically in the CD19+ tdTomato+ B cell population from CD19^cre/+Stat3^f/ftdTomato^stopf/f mice but not Stat3^f/ftdTomato^stopf/f WT B cells that lack Cre recombinase expression (Fig. S2A). TdTomato expression from CD19+ B cells (Stat3^f/ftdTomato^stopf/f) and CD19 haploinsufficiency (CD19^cre/+) did not impact MHV68 latency (Fig. S2B through D), and the CD19^cre/+Stat3^f/ftdTomato^stopf/f reproduced the latency defect (Fig. S2E and F) observed for the CD19^cre/+Stat3^f/f models (Fig. 1).

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FIG 4 Mixed bone marrow chimera models reveal intrinsic requirement for STAT3 in B cells for efficient establishment of latency with MHV68. (A) Schematic depiction of the generation and infection of mixed BM chimera set 1 generated by reconstitution of CD45.1+ C57/BL6-recipient mice with bone marrow from CD45.2+ Stat3f/ftdTomatostopf/f (WT) and CD19cre/+Stat3f/ftdTomatostopf/f mice (B cell-STAT3 KO). (B-C) Mixed BM chimeric set 1 mice were infected with 1,000 PFU MHV68-H2bYFP by intraperitoneal (i.p.) inoculation and evaluated at 16 dpi. (B) Single-cell suspensions of sorted tdTomato− (WT) and tdTomato+ (STAT3 KO) B cells were serially diluted, and the frequencies of cells harboring MHV68 genomes were determined using limiting dilution PCR. (C) Reactivation frequencies were determined by ex vivo plating of serially diluted sorted tdTomato− (WT) and tdTomato+ (STAT3 KO) B cells on an indicator monolayer. Cytopathic effect (CPE) was scored 3 weeks post-plating. For the limiting dilution analyses (B, C), curve fit lines were determined by non-linear regression analysis; frequency values were determined by Poisson analysis, indicated by the dashed line. Symbols represent the mean ± SEM of three independent experiments performed with six mice per infected group. (D) Schematic depiction of the generation and infection of mixed BM chimera set 2 mice generated by reconstitution of CD45.1+ C57/BL6-recipient mice reconstituted with bone marrow from CD19cre/+ and CD19cre/+Stat3f/ftdTomatostopf/f mice. (E–G) Mixed BM chimera set 2 mice were infected with 1,000 PFU MHV68-H2bYFP by i.p. inoculation and evaluated at 16 dpi. (E) Flow cytometry gating strategy for infected (YFP+) STAT3 WT (tdTomato−) and STAT3 KO (tdTomato+) B cells (B220+ CD3−) followed by quantitation of the frequency of infected B cells from mixed BM chimeras. (F) Confocal microscopy of frozen spleen sections of spleens from chimeric mice harvested on day 16 post-infection. For immunofluorescence imaging, tdTomato+ STAT3 KO B cells are red; MHV68-YFP+ cells are green; FDCs are blue; and B220+ B cells are magenta. Top panels, lower magnification images; bottom panels, higher magnification images of top panels. Far left panels, all colors; middle left omits B220 for easier visualization of tdTomato+ B cells; middle right panel, gated on the tdTomato cells infected with MHV68; far right panel is same as middle right panel but masks MHV68 signal (green) for easier visualization of tdTomato+ B cells. Scale bars = microns. (G) Quantitation of STAT3 WT and STAT3 KO germinal center B cells of total B cells (left panel) or of YFP+ B cells (right panel) by flow cytometry. Data for E and G represent the aggregated data from three independent experiments performed with six to seven mice per infected group. Each group of paired symbols represents the WT and KO B cell populations from one chimeric animal. Statistical significance was evaluated by paired t test. *, P < 0.05; ****, P < 0.0001.

At 16 dpi, CD45.2+ splenocytes from the mixed BM chimeras were sorted to isolate tdTomato+ (STAT3 KO) and tdTomato− (STAT3 WT) B cells. Based on a limiting dilution, nested PCR for MHV68, KO B cells had a fivefold decrease in the frequency of genome-positive cells (average of 1/219) compared to their WT counterparts (average of 1/44) (Fig. 4B). The limiting dilution explant reactivation assay confirmed this decrease in latency establishment, but the frequency of spontaneous reactivation was not reduced further (Fig. 4C). These findings reinforce our initial findings (Fig. 1) and more rigorously demonstrate a B cell-intrinsic requirement for STAT3 in B cells for the efficient establishment of MHV68 latency.

To control for the haploinsufficiency of CD19 on the surface of CD19^cre/+ B cells, a second mixed BM chimera model was generated using donor CD19^cre/+Stat3^+/+ BM in combination with BM from CD19^cre/+Stat3^f/ftdTomato^stopf/f mice (Fig. 4D). Flow cytometric analysis of the chimeras revealed an eightfold reduction in the frequency of MHV68-infected, YFP+ STAT3 KO B cells compared to their paired WT B cell counterparts (0.06% versus 0.51%) in the same animal at 16 dpi (Fig. 4E). Confocal microscopy of frozen tissue sections of infected spleen sections from mixed BM chimeras identified STAT3 WT (tdTomato−) and KO (tdTomato+, red) B220+ B cells interspersed throughout the tissue (Fig. 4F). The ratio of STAT3 WT:KO B cells was consistent with the mean 39:61 ratio of reconstitution for the respective WT:KO B cells determined by flow cytometry. TdTomato+ KO B cells were rarely detected in the YFP+ population, in contrast to frequent detection of YFP+ tdTomato- WT B cells. This is consistent with the failure of KO B cells to support latency in the splenic follicle based on limiting dilution PCR (Fig. 4B) and flow cytometric analysis of splenic single-cell suspensions (Fig. 4E). In contrast to the GC phenotype observed upon infection of mice that lacked STAT3 in all CD19+ cells (Fig. 2A), there was no difference in the frequency of GC B cells between the STAT3 WT and KO populations in the mixed BM chimera model (Fig. 4F and G; Fig. S2G and H). These findings substantiate STAT3 as a B cell-intrinsic latency determinant for GHV latency establishment in an in vivo model of infection wherein STAT3 WT and KO B cell populations reside in the same animal.

The STAT3-dependent transcriptional landscape of GC B cell genes

STAT3 directly regulates host genes conducive to proliferation and plasma cell differentiation in response to cytokines in the GC microenvironment, but the STAT3-dependent transcriptional landscape of GHV-infected GC B cells in the host has not been defined. Capitalizing on the ability to use flow cytometry to differentiate uninfected from YFP+ infected GC B cells, with and without STAT3 (tdTomato+), we sorted and collected specific subsets for RNA-sequencing. The CD45.2+ donor cells were gated on tdTomato to sort the STAT3 KO from WT B220+ B cells, followed by non-GC (GL7− CD95−) and GC (GL7+ CD95+) B cells (Fig. 5A). Last, the GC cells were sorted based on YFP to separate uninfected YFP− from infected YFP+ GC cells. In a principal component (PC) analysis, the non-GC and GC samples demonstrated the most difference along PC1, followed by separation of YFP− and YFP+ samples (Fig. 5B). The infected YFP+ WT GC segregated from the YFP+ STAT3 KO GC samples in PC2. Hierarchical clustering of the top 350 variable genes across all samples revealed binodal clustering of genes based on their regulation in non-GC versus GC B cells (Fig. 5C).

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FIG 5 RNA-sequencing of B cells from infected mixed BM chimeric mice reveals transcriptional differences intrinsic to STAT3-ablated B cells. (A) Schematic depiction of flow cytometry sorting strategy for B cell populations from mixed BM chimeric mice. YFP+ infected and YFP− uninfected GL7+ CD95+ germinal center cells were sorted and collected from tdTomato− and tdTomato+ populations 16 dpi. Non-GC (GL7− CD95−) cells were also collected for tdTomato− and tdTomato+ populations. (B) Principal component analysis to analyze the clustering of RNAseq samples from the indicated flow sorted populations, mixed BM chimeric set 2. (C) Hierarchical clustering of the top 350 differentially expressed genes (DEGs) across all samples, mixed BM chimeric set 2. (D–E) For each, volcano plots with significance cutoffs displaying log2 fold change versus –log10 adj P value. Heatmaps display genes with adjusted P value ≤0.05 and at least twofold change between indicated comparisons. Gene set enrichment analysis (GSEA) panels display HALLMARK gene sets with adjusted P value ≤0.05, |NES| ≥2. Size of dot represents fraction of genes from the gene set that are leading edge genes in the specified comparison. (D) Bioinformatic analysis comparing GC and non-GC B cells, mixed BM chimeric set 2. Heatmap (right panel) of differentially regulated GC-specific genes curated from Broad Institute GSEA gene sets. (E) Bioinformatic analysis comparing uninfected STAT3 KO GC B cells to uninfected STAT3 WT GC B cells, mixed BM chimera set 2. Heatmaps (right panels) of DEGs in replicate RNAseq data sets from mixed BM chimera sets 1 and 2; genes listed detail hallmark IFNα response and STAT3-regulated genes.

A comparison of WT GC to WT non-GC B cells in a volcano plot that highlighted genes with a minimum twofold change and adjusted P value <0.05 identified the upregulation of GC-signature genes Aicda, Mki67, Cd80, and Fas, with downregulation of Foxp1 and Cd38 (57, 58). In a gene set enrichment analysis (GSEA), hallmark gene sets associated with proliferation, such as E2F targets, G2M checkpoint, MYC targets, and MTOR signaling, were positively enriched in the GC cells compared to the non-GC B cells, while interferon-α and IFNγ response pathways had a negative enrichment score (Fig. 5D).

Next, KO GC cells were compared to their WT GC counterparts. Genes encoding B cell surface proteins IL-9R (Il9r) and CD23 (Fcer2a) were highly upregulated upon loss of STAT3, while known STAT3 target genes Socs3 and Prdm1 were downregulated (Fig. 5E, upper left panel). Hallmark gene sets for G2M checkpoint, E2F targets, and MYC proliferative pathways were negatively enriched in the KO GC cells, in striking contrast to WT GC cells, and highlight the role of STAT3 as a driver of cell cycle and proliferation (Fig. 5E, lower left panel). Regarding upregulated gene sets, the IFNα and IFNγ response gene sets had the highest enrichment scores, indicating a heightened IFN profile in KO GC cells. An enhanced IFN response encompassed an increased transcript expression of IFNα and IFNγ receptors and downstream signaling molecules Stat1, Stat2, Irf9, and IFN-stimulated genes (ISGs) including Ebi3, Irf1, and Gbp10 in both mixed BM chimera data sets (Fig. 5E, right panels). In summary, the loss of the master regulator STAT3 led to significant changes in the transcriptional landscape of GC cells, marked by the downregulation of genes driving proliferation and cell cycle progression and an upregulation of genes driving a type I and type II IFN response in the mixed BM chimera model.

The impact of MHV68 infection and STAT3 on GC B cell gene expression

Viral gene expression was tightly restricted in GC B cells, with very low levels of expression across the viral genome (Table S1). Although viral gene expression was minimal in GC cells at 16 dpi, there was a greater than fourfold higher expression level of genes with functions in immune modulation (M3, mK3), viral gene transactivation (ORF57), and viral DNA replication (ORF6, ORF21, ORF59, and ORF61) compared to the mean expression level of all viral ORFs (Fig. 6A; Fig. S3). Notably, ORF6 and ORF61 are the source of immunodominant CD8 T cell epitopes in infected C57BL/6 mice (59). However, there were no significant changes in the viral gene expression profile of infected GC B cells in the absence of STAT3.

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FIG 6 Loss of STAT3 leads to a heightened interferon response in germinal center B cells. (A) Viral gene expression of infected YFP+ cells sorted from WT and KO GC B cells from the two mixed BM chimera experiments. Bars represent the mean of the median-scaled CPM TMM values for each group of samples. (B) Hierarchical clustering of differentially expressed genes (DEGs) from the comparison of infected STAT3 WT and infected STAT3 KO GC B cells in mixed BM chimera set 2, with the addition of uninfected GC B cells and separated into four distinct clusters of gene expression patterns. Output generated in Morpheus, . These were filtered to retain only genes with adj P value ≤0.05 and at least twofold change comparing infected WT and infected KO GC B cells. (C) Heatmap visualization of select gene expression across uninfected and infected GC samples in mixed BM chimera set 2. Il10 and STAT3 target genes Socs3 and Prdm1 are included for reference. The remaining genes are DEGs from (B) or leading-edge genes common to both mixed BM chimera data sets. Leading edge genes from the hallmark IFNα response, IFNγ response, and mTOR signaling gene sets as revealed from pre-ranked GSEA of the infected KO GC versus infected WT GC B cell are noted, along with genes with roles in B cell biology and broader cellular processes. (D–E) Bioinformatic analysis comparing infected WT germinal center to uninfected WT GC B cells (D) and infected KO GC to infected WT GC B cells (E). Upper volcano plots display log2 fold change versus –log10P value for mixed BM chimera set 2. Hist1h2bg reflects the H2b-YFP fusion gene delivered by the recombinant MHV68-H2bYFP reporter virus. Lower GSEA panels display hallmark gene sets with adj P value ≤0.05, |NES| ≥1.5 that were common to both mixed BM chimera data sets. Size of dot represents fraction of genes from the gene set that are leading edge genes in the specified comparison.

MHV68 infection of WT GC cells led to a multitude of host transcriptional changes. Hierarchical clustering of DEGs comparing infected KO and WT GC cells revealed four distinct clusters of genes that demarcate the combined impact of infection and the status of STAT3 (Fig. 6B; Table S2). Genes in cluster I were upregulated by the presence of the virus in WT GC but to a lesser degree in infected STAT3 KO cells; genes of this cluster encode Il10 and regulatory proteins, such as Pik3cb and Ret, in addition to mTOR pathway molecules Asns, Cdkn1a, Cth, and Trib3 (Fig. 6B and C). Gene expression in clusters II and III was positively or negatively regulated by STAT3, respectively. Genes in cluster II include STAT3-regulated genes Prdm1, S1pr1, and Socs3, while genes in cluster III include the regulatory factor Smad1 and the nucleotide biosynthetic molecule Upp1 (Fig. 6B and C). Cluster IV genes such as Fcer2a, Il9r, Aire, Vav3, Icos, and numerous interferon response genes were downregulated by the virus in WT infection, but this virus-driven decrease was blocked in the absence of STAT3 (Fig. 6B and C).

We and others previously reported a bias in the B cell immunoglobulin (Ig) repertoire in the context of MHV68 infection; infected B cells exhibited immunoglobulin heavy chain V gene usage that was non-overlapping with uninfected cells and displayed bias in lambda light chain (34, 60). Here, comparison of infected with uninfected WT GC cells revealed the downregulation of multiple Ig heavy chain and light chain V genes (Fig. 6D, upper panel). The predominant IgH V genes were distinct in the infected GC compared to their uninfected WT counterparts from both sets of BM chimera models (Fig. S4A and B). Additionally, we confirmed that infected cells utilize lambda light chain more frequently (Fig. S4C and D).

Broadly, the comparison of infected to uninfected WT GC B cells by volcano plot revealed more host genes were downregulated (756 genes) than upregulated (426 genes) (Fig. 6D, upper panel). Loss of STAT3 in B cells altered the infected GC profile, leading to upregulation of 362 genes and downregulation of 315 genes ((Fig. 6E, upper panel). GSEA identified positive enrichment for MYC targets, oxidative phosphorylation, and MTOR signaling upon MHV68 infection of WT GC B cells, highlighting the increased expression of genes involved in cell cycle progression and metabolism (Fig. 6D, lower panel), similar to reports for primary B cells newly infected with EBV (61). In contrast, MYC and MTOR gene sets were negatively enriched when comparing infected KO and infected WT GC cells, suggesting that signatures of proliferation in the infected B cells are dependent on STAT3 (Fig. 6E, lower panel). Consistent with the known impacts of MHV68 in blocking host IFN responses (62–67), there was a negative enrichment for genes involved in response to IFNα and IFNγ in the infected WT GC B cells (Fig. 6D). This includes the downregulation of signaling molecules Stat2 and downstream ISGs Gbps 2b, 6, 8, and 10, Oasl2, Tap1, Usp18, and Trim21 (Fig. 6C; Fig. S5). STAT3 negatively regulates the type I IFN response by induction of the suppressor of cytokine signaling factor 3, Socs3, that suppresses STAT1 and STAT2, in addition to repression of Irf9 transcription and by direct binding of STAT1 partners (68–70). Socs3 was downregulated in the absence of STAT3 in sorted GC B cells (Fig. 6C and E), as validated by qRT-PCR in B cells from infected mice (Fig. S6). Consistent with decreased expression of Socs3, GSEA revealed an enrichment in genes associated with IFNα and IFNγ responses in infected KO compared to infected WT GC cells in mixed BM chimera samples (Fig. 6E; Fig. S5). Taken together, MHV68 infection reprograms GC B cells in vivo to upregulate networks that promote proliferation while impairing genes associated with IFN responses. This virus-induced signature is reversed in the absence of STAT3.

Reduction of CD23 expression on infected B cells is influenced by STAT3

A comparison of infected KO GC with infected WT GC cells uncovered significant changes in genes with functional links to biological processes of B cells in the absence of STAT3, including regulatory proteins (Socs3, Pik3b, Vav3, and Cdkn2a), transcription factors (Prdm1 and Aire), and cell surface proteins that mediate responses to the microenvironment to influence B cell differentiation (S1pr1, Il9r, and Fcer2a). (Fig. 6C and E, upper panel). Fcer2a encodes the low-affinity IgE receptor commonly known as CD23, a surface marker that has been reported to promote B cell activation and to function as a negative regulator of IgE responses (71–73). In agreement with RNAseq, Fcer2a transcript levels were markedly upregulated in KO B cells compared to WT B cells that were isolated from naive and MHV68-infected mice (Fig. S6C and D). Further validation was revealed by flow cytometric analysis of CD19+ B cell subsets. The frequency of CD23^hi B cells was significantly reduced in WT-infected mice but only slightly diminished in B cell-STAT3 KO mice (Fig. 7A, right panel). The WT B cells directly infected with MHV68 (YFP+) had a threefold lower CD23^hi expression compared to STAT3 KO cells (Fig. 7A). Next, we examined whether MHV68 infection of primary B cells ex vivo impacts CD23 surface expression via STAT3. Primary B cells from WT and B cell-STAT3 KO mice were infected and analyzed at 3 dpi. MHV68 infection led to an increase in STAT3-Y705 phosphorylation in the YFP+ subset, indicating that direct infection activates STAT3 (Fig. S7A). Infection also led to a twofold decrease in the frequency of WT B cells with CD23^hi expression (Fig. 7B) and a fourfold decrease in Fcer2a transcript levels (Fig. S6E), but no significant change was observed between uninfected and infected B cells lacking STAT3. Taken together, the repression of CD23 transcript and surface expression on murine B cells upon MHV68 infection are mediated in part by STAT3.

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FIG 7 IL-21-stimulated reduction of CD23 surface expression is dependent on STAT3. (A) Left panel, histogram depiction of surface CD23 expression on B cells from naïve mice compared to B cells or YFP+ B cells from infected WT (Stat3f/f) or B cell STAT3 KO (CD19cre/+Stat3f/f) mice at 16 dpi based on flow cytometric analysis. Middle and right panels are the quantitation of the frequency of CD23hi B cells from the indicated populations. Symbols represent individual mice ± SD from one (YFP+ B cells) to six (B cells from naïve and infected mice) independent experiments performed with three to seven mice per infected group and one to two mice per naive groups. (B) Frequency of Stat3f/f and CD19cre/+Stat3f/f B cells with CD23hi expression upon mock or MHV68 infection, 3 dpi. (C) Left panel, histogram depiction of CD23hi B cells from anti-CD40 MHV68-infected cultures treated concurrently without or with IL-21 for 3 days, as indicated. Right panel, gated histogram data summarized in bar graphs. (D) Histogram depiction of CD23 surface expression on EBV+ GM12878 lymphoblastoid B cell lines (LCLs) that express Cas9 in addition to control sgRNA or sgRNA targeting STAT3. Cells were mock stimulated or stimulated with IL-21 (100 ng/mL) for 6 days. Statistical significance was evaluated by one-way ANOVA followed by Sidak’s multiple comparisons or an unpaired one-tailed t test for the YFP+ cell analysis; ***, P < 0.001; ****, P < 0.0001 ; ns, P > 0.05.

IL-21 signaling in B cells is necessary for the efficient establishment of latency with MHV68 (24). IL-21 is a well-known activator of STAT3 (Fig. S7B) that promotes B cell activation and germinal center processes leading to plasma cell differentiation (74–76). Consistent with previous reports (71, 77), activation of CD40 signaling led to the upregulation of CD23 from 37% to 94% of WT (Stat3^f/f) B cells, while IL-21 in combination with α-CD40 significantly reduced CD23^hi expression to 60% on WT B cells (Fig. S7C). This IL-21-stimulated downregulation was largely reversed in STAT3 KO B cells (CD19^cre/+ Stat3^f/f). In the context of MHV68 infection, IL-21 in combination with α-CD40 led to a twofold reduction in CD23^hi WT B cells that was partially restored in the absence of STAT3 (Fig. 7C). The analysis of this STAT3-dependent IL-21 downregulation of CD23 was extended to an EBV+ lymphoblastoid B cell line (LCL), which highly expresses CD23 (78). Surface CD23 levels were greatly diminished on LCL GM12878 upon a 6-day treatment with IL-21. However, CRISPR-mediated knockout of STAT3 rendered two independent LCL cultures non-responsive to IL-21-induced loss of surface CD23 (Fig. 7D). These findings reveal a role for STAT3 in regulating the CD23 surface molecule on B cells in response to IL-21 in the context of GHV infection.

DISCUSSION

Here, we aimed to identify transcriptional and functional roles for STAT3 in B cells newly infected with a gammaherpesvirus in vivo. First, we verified a significant defect in latency establishment in two strains of B cell-STAT3 knockout mice. This decrease in virus latency was accompanied by an increase in GC B cells and a reduction of infected plasma cells. Our analyses identified altered GC architecture in B cell-STAT3 KO mice, along with reduced virus-specific antibody production, and a heightened CD8 T cell response. This perturbed immune response led us to develop a mixed BM chimera model wherein STAT3 KO B cells and WT B cells were both present as potential reservoirs of latency in the same host microenvironment. B cells lacking STAT3 were not able to compete with their wild-type counterparts to support GHV latency at 16 dpi. To dissect the transcriptional consequences of STAT3 loss, RNA sequencing was performed on sorted STAT3 WT and KO GC B cells, with and without MHV68 infection. Our analysis revealed that STAT3 targets pathways associated with proliferation and interferon responses in GC B cells infected with MHV68.

We previously reported a requirement of STAT3 to support the efficient establishment of latency in a B cell-STAT3 KO mice model (42). Briefly, infection of B cell-STAT3 KO mice led to a reduction in splenic latency and an increase in GC B cells 16 dpi. Here, we expand upon these results in a second strain of STAT3 KO mice and report new findings of alterations in the virus-specific immune response that call attention to the role for STAT3 in GC development after virus infection. Immunization of STAT3-KO mice with ovalbumin led to a notable decrease in GC B cells, short-lived GC structures, and a decrease in plasma cells (79). MHV68 infection resulted in an increase in total GC B cells in B cell-STAT3 KO mice, but immunofluorescence of infected spleen sections revealed smaller follicles with less organized GCs in B cell-STAT3 KO mice (Fig. 2D). MHV68 infection of mice leads to an increase in highly proliferative centroblasts compared to centrocytes within the infected GC population, as well as the total GC population (22, 24). In the absence of STAT3, we observed a reduced frequency of centroblasts in naive mice, as well as those infected with MHV68, with the ratio further skewed toward centrocytes in the infected GC population (Fig. 2C). The aberrant GC architecture and the reduction in centroblasts at 16 dpi along with the reduction in virus-specific antibodies suggest that GC cycling between dark and light zones may be disrupted in GCs of mice lacking STAT3 in B cells. Recently, STAT3^fl/flCD23^Cre mice were reported to have defects in GC organization due to aberrant light zone to dark zone recycling upon antigen immunization or influenza virus infection (80). In an analysis of the STAT3-regulated GC transcriptome, pathways involving Myc, E2F, and mTORC1 signaling were strongly enriched (80), demonstrating common biologic roles for B cell STAT3 identified from our analysis of MHV68-infected CD19^cre/+Stat3^f/f mouse models.

In the GC reaction, B cells differentiate and exit the GC as class-switched, long-lived memory B cells or antibody-secreting plasma cells. STAT3 coordinates the upregulation of Prdm1, encoding Blimp-1, which is a master regulator of B cell differentiation to plasma cells in response to IL-21 (50, 51). These plasma cells are a source of MHV68 reactivation in the spleen (52), and long-lived plasma cells are a long-term latency reservoir in the bone marrow, which led us to examine plasma cells in the B cell-STAT3 KO mice. There was no difference in plasma cell frequency at 16 dpi, although there was a decrease in infected (YFP+) plasma cells in B cell-STAT3 KO mice. This phenotype was also reported for MHV68 infection of IL-21R KO mice, where IL-21 signaling is necessary for latency establishment (24). Regarding chronic infection at 42 dpi, there was a significant reduction in virus-specific IgG (Fig. 3B) and virus-neutralizing activity in serum (Fig. 3C) from B cell-STAT3 KO mice. We note that the defect in B cell infection was observed even earlier at 12 dpi, but the limited number of infected cells precluded an in-depth analysis of this population.

The latency-associated M2 protein of MHV68 is critical for viral latency establishment in mice (81, 82). M2 induces high levels of IL-10 secretion in B cells and drives B cells to differentiate into plasmablasts in vivo (38–40). IL-10 is an anti-inflammatory cytokine that suppresses natural killer and T cell effector responses (83). An increase in virus-specific, short-lived effector CD8+ T cells (SLECs) was noted in the B cell-STAT3 KO mice at 42 dpi (Fig. 3H). The heightened virus-specific CD8+ T cell response may be a byproduct of the latency defect in B cell-STAT3 KO mice, driven by a reduction in MHV68 M2-driven production of the immunosuppressive cytokine IL-10. This finding is consistent with reports of increased virus-specific effector T cells in mice infected with a recombinant MHV68 virus that does not express the viral M2 protein (38).

Mixed BM chimeras have been employed to bypass immune defects caused by global deletion of signaling molecules CD40 and IL-21R or NF-κB p50 (24, 26, 56). Here, BM from STAT3 B cell-competent and -ablated mice was mixed to create an in vivo model wherein STAT3 WT and KO B cells are simultaneously evaluated for their ability to support latency, in the context of the same microenvironment and immune response to infection. This model reveals that the loss of STAT3 leads to a marked reduction in MHV68+ B cells (Fig. 4B and E), confirming that STAT3 is required to promote B cell latency by GHV in the GC. This rigorous analysis supports STAT3 as a B cell-intrinsic host factor essential for latency establishment in primary B cells.

This is the first report of an unbiased transcriptional profile of MHV68-infected GC B cells. We capitalized on our ability to distinguish STAT3 KO B cells from WT counterparts based on Cre-inducible tdTomato expression in STAT3 KO B cells and the YFP reporter gene from MHV68-H2bYFP. Fluorescence-activated cell sorter (FACS) sorting for non-GC and GC subsets, with and without STAT3, with and without infection, followed by RNAseq enabled us to define the multitude of changes to the transcriptional landscape of GC B cells driven by the virus and those changes that are dependent on STAT3 (Fig. 5C). GSEA of GC B cells revealed a virus-driven enrichment for MYC targets and metabolic processes of oxidative phosphorylation and mTOR, while IFNα and γ responses are diminished. MYC plays a major role in GC processes, regulating GC B cell entry and cycling between dark and light zones (84). Absence of MYC leads to reduced numbers of affinity-matured B cells within the GC. The impairment of MYC leads to the collapse of established GCs (85). Comparing STAT3 KO and WT GC B cells, there was a negative enrichment for MYC target genes by GSEA, consistent with the role for STAT3 in MYC-driven proliferation (86, 87).

MHV68 encodes numerous proteins to bypass the IFN response and promote replication and latency. MHV68 ORF11 and ORF36 interfere with IRF3 binding, blocking the transcription of IFNβ (63, 66). In addition, MHV68 ORF54 induces degradation of IFNAR1 to block IFN signaling (64), while the latency protein M2 impairs downstream IFN signaling by inducing the downregulation of STAT1 and STAT2 (62). We observed low transcript levels of these ORFs in YFP+ GC cells at 16 dpi (Fig. 6A). A consistent finding in the comparison of STAT3 WT and KO GC B cells was the positive enrichment for IFN response pathways in uninfected and infected STAT3 KO B cells. IFN responses restrict MHV68 latency through the induction of interferon-stimulated genes, which typically promote an antiviral state (5, 88–91). Host factors that restrict MHV68 infection include those that promote IFN production like IRF3 and IRF7, and those that respond to IFN to directly induce ISG transcription like IRF1, STAT1, and STAT2 (62, 65, 92–95). Mice lacking STAT1, IFN-αβ receptor, or combination IFN-αβ and IFN-γ receptors succumb to infection with MHV68 (96), stressing the importance of the IFN response in combating the virus. In the absence of STAT3, there was an upregulation of ISGs such as Oasl2 and the family of guanylate-binding proteins (GBPs). Many of these ISGs have known antiviral function; the human homolog of murine Gbp2b is human GBP1, and it was recently reported to block KSHV capsid transport by disrupting cytoskeletal actin networks (97). However, ISGs such as Usp18 and Trim21 that negatively regulate the IFN response were also upregulated (98, 99). A subset of patients with autosomal dominant hyper-IgE syndrome caused by loss-of-function mutations in STAT3 have been observed to develop a lupus-like syndrome involving heightened type I IFN responses (100). Further studies are required to clarify the net impact of these dysregulated ISGs on early events in gammaherpesvirus infection in de novo-infected primary B cells. STAT3 has been reported to negatively regulate the type I and II IFN responses by upregulating Socs3, repressing the transcription of IRF9, STATs 1, and 2, and competing for binding with STAT1 to reduce ISGF3 transcriptional complex formation (68–70). While we observed consistent downregulation of Socs3 in the absence of STAT3 in GC B cells of infected mice, the mechanism by which STAT3 suppresses IFN responses in MHV68-infected B cells, via either direct or indirect regulation, requires additional investigation.

The loss of STAT3 in GC B cells led to the downregulation of known STAT3 target genes, Prdm1, S1pr1, and Socs3, but also revealed the dysregulation of Il9r that encodes the receptor for IL-9 and Fcer2a that encodes CD23, the low-affinity IgE receptor. We observed that IL-21 suppresses CD23 expression in primary B cells at least in part through STAT3, consistent with transcript upregulation previously reported in an RNAseq data set of a diffuse large B cell lymphoma cell line treated with an shRNA targeting STAT3 (68). CD23 was downregulated in total splenic B cells upon MHV68 infection in mice and upon ex vivo infection of primary B cell cultures, even more so in the directly infected cells (Fig. 7A). CD40-ligation leads to the induction of CD23 on the surface of activated B cells (71). We observed that IL-21 reversed CD40 induction of CD23 in a STAT3-regulated manner, leading us to postulate that STAT3 is repressing CD23 expression through IL-21 signaling. Hyper-IgE syndrome patients have autosomal dominant loss-of-function mutations in STAT3, in whom naive and memory B cells are noted to have heightened CD23 surface levels (101). Future studies are needed to define the STAT3-dependent mechanism of CD23 downregulation in response to infection or IL-21. While the functional consequence of CD23 loss for B cells infected with MHV68 is unclear, caution is warranted when using CD23 to demarcate follicular B cells in the context of MHV68 infection.

EBNA2, a key latency-associated transactivator and transforming factor of EBV, and RTA, the master lytic transactivator of KSHV, each upregulate the CD23 promoter through interactions with host RBP-Jkappa (102–104). CD23 expression is an indicator of B cell activation and surface CD23 complexes with surface CD21 and IgE (71, 73). Soluble CD23 (sCD23) is released upon metalloproteinase cleavage and mediates activation and differentiation of lymphocytes (72). sCD23 regulates IgE synthesis in human B cells, likely by binding CD21 and membrane IgE (105). Membrane and sCD23 are induced by RTA and EBNA2 (102, 106), and transfer of conditioned media containing sCD23 leads to activation of lymphocyte cultures (102). EBV+ LCLs express LMP1, a potent activator of STAT3, and EBNA2, a known activator of STAT3 and inducer of CD23 (107, 108). IL-21 treatment promotes the proliferation of EBV+ diffuse large B cell lymphomas, inducing LMP1, STAT3 activation, and MYC expression (109). Our finding that IL-21 treatment led to CD23 downregulation in EBV+ LCLs that retain STAT3 but not in those silenced for STAT3 expression suggests that CD23 induction by EBNA2 is lost in the absence of IL-21-induced STAT3 activation. Taken together, these findings suggest that a dynamic shift in STAT3 signaling occurs upon engagement of GHV-infected B cells with the GC cytokine IL-21. One outcome is the reduction in the levels of CD23, a B cell activation factor that has two mechanisms of action. Determining the consequences of these changes, and whether CD23 functions directly via receptor-mediated signaling on the infected B cell or indirectly via sCD23 shed into the GC microenvironment, will require careful delineation.

Our study highlights STAT3 signaling as a critical host pathway commandeered by GHVs to promote latency. We report that the requirement for STAT3 in MHV68 latency establishment is intrinsic to the infected B cell. STAT3 is activated upon MHV68 infection, and those infected B cells have gene signatures that partially overlap with signatures of virus-driven reprogramming reported for EBV and KSHV (110, 111). Understanding the virus-host interplay during long-term latency and how the GHVs utilize host factors and pathways to develop cancers is paramount. KSHV miRNAs block STAT3, and inhibition of STAT3 increases reactivation from latency (112). While there is a long-term latency defect in B cell-STAT3 KO mice 42 dpi, the role of STAT3 in the maintenance of MHV68 has not been investigated. A recent study reveals a role for the STAT3-activating cytokine IL-16 in inhibiting MHV68 reactivation through the STAT3-p21 axis (113). Though the use of JAK and direct STAT3 inhibitors show promise in clinical trials, deeper understanding of the role of STAT3 in viral persistence is required, as some GHV cancers may lose their dependency on STAT3 (114). This study provides a comprehensive examination into understanding signaling downstream of STAT3 in GHV infection in vivo by transcriptional profiling of the major B cell latency reservoir. Future studies to delineate factors downstream of STAT3 in the context of GHV latency will reveal new avenues of treatment important for the prevention and treatment of GHV-driven malignancies.

MATERIALS AND METHODS

Animal models

Strain 1 designates Stat3^f/f mice with exons 12–14 flanked by loxP elements (44), and Strain 2 designates Stat3^f/f mice with exons 18–20 flanked by loxP elements [B6.129S1-Stat3^tm1Xyfu/J] (The Jackson Laboratory, Bar Harbor, ME) (45). CD19^cre/cre mice [B6.129P2(C)-Cd19 ^tm1(cre)Cgn/J] (Jackson) were crossed with Strain 1 and Strain 2 mice to generate Stat3^f/fCD19^cre/+-1 and -2 mice, respectively. Stat3^f/f and Stat3^f/fCD19^cre/+ mice used in pathogenesis experiments were littermates derived from crossing Stat3^f/f mice with Stat3^f/f mice heterozygous for CD19^cre; sexes were randomly assigned to experimental groups.

TdTomato^stopf/f mice [B6.Cg-Gt(ROSA)26Sor^{tm14(CAG-tdTomato)Hze}/J] (Jackson) were crossed with Stat3^f/f CD19^cre/+ mice for multiple generations to generate CD19^cre/+Stat3^f/ftdTomato^stopf/f mice. First, a male CD19^cre/+Stat3^f/f mouse was crossed with a female tdTomato^stopf/f mouse generating progeny mice that were heterozygous at the CD19, Stat3, and tdTomato loci. Next, an F1 cross was set up with a male and female mouse of the following genotypes: CD19^cre/+Stat3^f/+tdTomato^stopf/+ and CD19^+/+Stat3^f/+tdTomato^stopf/+. Progeny mice from this pairing were then set up for an F2 cross, consisting of a male and female pairing of the following genotypes: CD19^cre/+Stat3^f/+tdTomato^stopf/f and CD19^+/+Stat3^f/+tdTomato^stopf/f. Mice produced from this F2 cross maintained floxed alleles for both the Stat3 and tdTomato loci as follows: CD19^cre/+Stat3^f/ftdTomato^stopf/f and CD19^+/+Stat3^f/ftdTomato^stopf/f. To maintain the colony and produce mice for experiments, parings were set up which consisted of the following genotypes: CD19^cre/+Stat3^f/ftdTomato^stopf/f and CD19^+/+Stat3^f/ftdTomato^stopf/f. Mice were backcrossed for at least five generations before experiments were performed.

CD19^cre/+ mice were generated by crossing CD19^cre/cre mice with C57BL/6 mice. Ly5.1 (CD45.1) [B6.SJL-Ptprca Pepcb/BoyJ] (Jackson) were the recipient mice for bone marrow chimera studies. All mice were bred at the Stony Brook University Division of Laboratory Animal Research facility or the National Institutes of Health Division of Veterinary Resources, unless stated otherwise. Mice were housed in a specific pathogen-free environment, and all mouse experiments were performed in accordance with guidelines under protocols approved by the Institutional Animal Care and Use Committee of Stony Brook University and the NCI Animal Care and Use Committee.

Generation of mixed bone marrow chimeric mice

Recipient Ly5.1 (CD45.1) [B6.SJL-Ptprca Pepcb/BoyJ] (Jackson) at 6 weeks of age were gamma irradiated with 900 rads, in split dose. Next, mice were injected retro-orbitally with two million bone marrow cells isolated from donor CD19^cre/+Stat3^f/ftdTomato^stopf/f (KO) and Stat3^f/ftdTomato^stopf/f (WT) mice at a 50% WT:50% KO bone marrow ratio for the first set of chimeras or with five million bone marrow cells isolated from donor CD19^cre/+Stat3^f/ftdTomato^stopf/f (KO) and CD19^cre/+ (WT) mice at a 30% WT:70% KO bone marrow ratio for the second set of chimeras. All female mice were used; there is no discernible difference between male and female mice with respect to establishment of MHV68 latent infection. Mice were treated with acidified water 2 weeks prior to and after irradiation. Verification of chimerism was performed 6 weeks post transfer through collection of blood by submandibular bleed, followed by flow cytometry. The mean reconstitution ratio was 66% WT:34% KO cells for the first set of chimeras and 39% WT:61% KO for the second set of chimeras.

Cells and viruses

Recombinant MHV68 expressing H2bYFP fusion protein (rMHV68-H2bYFP) was used for the infection (115). Mice (8–12 weeks old) were infected by intraperitoneal injection with 1,000 PFU in 0.5 mL under isoflurane anesthesia. Mouse spleens were homogenized, treated to remove red blood cells, and passed through a 100-µm-pore-size nylon filter. For ex vivo experiments, flow sorting, and RNA-sequencing, splenocytes were subject to negative selection to enrich for B cells (Pan B Cell Isolation Kit; Stemcell, Vancouver, BC, Canada). Cells were counted using Vi-CELL BLU Cell Viability Analyzer (Beckman Coulter, Pasadena, CA). Blood was collected posthumously by cardiac puncture. Serum was collected after a centrifugation at 20,000 × g for 20 min at room temperature.

For STAT3 knockout in the EBV+ LCLs, single-guide RNA (sgRNA)-directed CRISPR-Cas9 gene knockout was performed as previously described (116). In brief, two independent STAT3 targeting sgRNAs (GAGACCGAGGTGTATCACCA and AACATGGAAGAATCCAACAA) from Brunello library (117) were cloned into pLentiGuide-puro (a gift from Feng Zhang, Addgene # 52963). Lentiviruses were produced by transfection of 293T cells and used to transduce Cas9+ GM12878 LCLs as previously described (116, 118). In parallel, GM12878 were transduced with control lentivirus expressing an sgRNA targeting GFP (pXPR-011, a gift from John Doench). Transduced LCLs were selected by puromycin (3 ug/mL, Invitrogen) for 3 days.

Cell stimulation and ex vivo virus infection

For cytokine stimulations ex vivo, primary murine splenocytes were harvested from spleens of Stat3^f/f and Stat3^f/fCD19^cre mice. Single-cell suspensions were subjected to negative selection to enrich for B cells (Pan B Cell Isolation Kit; Stemcell, Vancouver, BC, Canada). Primary B cells were plated in a 96-well plate at a concentration of 4–5 × 10⁵ cells/mL, in 200 µL of primary B cell media (RPMI 1640 supplemented with 20% FBS, HEPES, non-essential amino acids, sodium pyruvate, penicillin/streptomycin, L-glutamine, β-mercaptoethanol). rMHV68-H2bYFP was added at an MOI of 20 in the presence of polybrene, followed by centrifugation at 1,500 × g for 1 h at RT, and resuspended in 250 µL primary B cell media supplemented with 5 µg/mL LPS (Sigma) overnight. Cells were treated with 10 µg/mL anti-CD40 (BioLegend) or 25 ng/mL murine IL-21 (PeproTech), alone or in combinations, as indicated. For ex vivo infection, primary B cells were plated at a cell density of 1 × 10⁶ cells/mL, in 200 µL of primary B cell media in each well of a 24-well plate.

At day 6 post puromycin selection, Cas9+ GM12878 cells were seeded at a density of 5 × 10⁵ cells/mL in RPMI with 10% fetal bovine serum (FBS; Gibco) in 12 well plates. LCLs were mock stimulated with PBS or with IL-21 (BioLegend, 100 ng/mL in PBS). LCLs were re-seeded in fresh culture medium supplemented with IL-21 every 2 days and assayed by FACS at the end of 6 days.

Limiting dilution analysis of latency and reactivation

To determine the frequency of cells harboring the viral genome as an indicator of latency, single-cell suspensions were analyzed by single-copy-nested PCR as previously described (119). To determine the frequency of cells harboring latent virus capable of reactivation upon explant, single-cell suspensions were plated in 12 serial twofold dilutions on a monolayer of MEF cells prepared from C57BL/6 mice and scored for CPE 3 weeks after plating. Parallel samples were mechanically disrupted using a Mini-BeadBeater prior to plating on the monolayer of MEFs to release preformed virus and score for preformed infectious virus (119).

Immunoblotting

Total protein lysate was harvested in lysis buffer [150 mM sodium chloride, 1.0% IGEPAL CA-630, 0.5% sodium deoxycholate, 0.1% sodium dodecyl sulfate, 50 mM Tris (pH 8.0)] supplemented with a protease inhibitor cocktail (Sigma, St. Louis, MO). Proteins were separated on 4%–20% SDS-PAGE gels and transferred to a polyvinylidene fluoride membrane. Antibodies against STAT3 (clone K-15; Santa Cruz Biotechnology, Dallas, TX) and α-tubulin (clone B-5-1-2; Sigma) were detected using secondary anti-mouse (Rockland, Limerick, PA) or secondary anti-rabbit (Invitrogen, Grand Island, NY) antibodies by immunoblot analysis with an Odyssey Imager (Li-COR Biosciences, Lincoln, NE).

Flow cytometry

For the analysis of murine B cells and T cells, 2 × 10⁶ splenocytes were resuspended in 50 µL of FACS buffer (PBS with 2% FBS) and blocked with TruStain fcX (clone 93; BioLegend, San Diego, CA). The cells were washed and stained to identify B cell subsets with fluorophore-conjugated antibodies against CD45.2 (clone 104), CD19 (clone 6D5), B220 (clone RA3-682), CD138 (clone 281-2), CD95 (clone 15A7), CD21 (clone 7E9), CD23 (clone B3B4), CXCR4 (clone L276F12), CD86 (clone GL-1), and CD3 (clone 17A2) or biotinylated antibody against GL7 (clone GL-7) that was detected using secondary streptavidin-conjugated allophycocyanin-cyanin7. T cell subsets were identified with antibodies against CD4 (clone GK1.5), CD8 (clone 53-6.7), CD44 (clone IM7), CD127 (clone A7R34), KLRG1 (clone 2F1/KLRG1), TCRβ (clone H57-597). H-2K(b)-p79 MHC-peptide complex was provided as biotinylated monomers by the NIH tetramer core facility and reconstituted with streptavidin-conjugated allophycocyanin. For STAT3-Y705 phosphorylation detection, cells were blocked with TruStain fcX before staining for surface markers. Following fixation and permeabilization with Fixation/Permeabilization Kit (BD Biosciences, San Jose, CA), cells were permeabilized a second time in ice cold 100% methanol for 20 min. Cells were then stained with PE anti-STAT3 Phospho (Tyr705) antibody (Biolegend). For sorting, splenocytes were first enriched for B cells by depletion of non-B cells with magnetic microbeads (Pan B Cell Isolation Kit; Stemcell, Vancouver, BC, Canada) and then sorted using antibodies described above on a FACSAria III sorter (BD Biosciences) or MoFlo sorter (Beckman Coulter, Indianapolis, IN) into cold FACS buffer. All antibodies were purchased from BioLegend, Invitrogen, or BD Biosciences. The data were collected using a CytoFLEX flow cytometer (Beckman Coulter) and analyzed using FlowJo v10.8.1 (Treestar Inc., Ashland, OR). Dead cells were excluded based on Alexa Fluor 700 NHS Ester uptake. Doublets were excluded through forward scatter-height by forward scatter-area parameters.

For the analysis of EBV+ LCLs, cells were washed once with FACS buffer (2% FBS in PBS) and then stained with APC conjugated anti-CD23 (5 uL per samples) for 30 min at room temperature. Stained cells were washed twice with FACS buffer and analyzed by flow cytometry on a BD FACSCalibur instrument.

Enzyme-linked immunosorbent assay

To measure total IgG levels and antibody specificity in the serum, plates were coated with either 2 µg/mL of donkey anti-mouse IgG (Affinipure; Jackson ImmunoResearch Laboratories, West Grove, PA), carbonate buffer (0.0875 M Na₂CO₃, 0.0125 M HCO₃, pH 9.2) or 0.5% paraformaldehyde-fixed viral antigen-carbonate buffer and incubated overnight at 4°C. Coated plates were washed in PBS with 0.05% Tween 20 (PBS-T) and blocked in 3% milk-PBS-T prior to incubation with serial dilutions of serum or the mouse IgG standard (Invitrogen, Jackson ImmunoResearch) in 1% milk-PBS-T for 2 h at RT. IgG was detected by the use of horseradish peroxidase-conjugated donkey anti-mouse IgG (Jackson ImmunoResearch), SureBlue TMB (SeraCare, Milford, PA), and stop solution, and absorbance at 450 nm was read on FluoStar Omega (BMT Labtech, Cary, NC).

Neutralization assay

Neutralization was tested by means of a plaque reduction neutralization test adapted from reference (54). Briefly, threefold serum dilutions, starting from an initial concentration of 1:80 in Dulbecco’s modified Eagle medium (DMEM) supplemented with 10% FBS, 100 U/mL penicillin, 100 µg/mL streptomycin, and 2 mM L-glutamine, were incubated with 150 PFU of MHV68 on ice for 1 h. The virus/serum mixture was then added to a sub-confluent BHK21 monolayer (4 × 10⁴ cells/well) plated the previous day in a 24-well plate, in triplicate. As a control, three wells received no-serum-added virus. Plates were rocked every 15 min for 1 h at 37°C. Infected cells were overlaid with 1.5% methyl cellulose solution in DMEM containing 2.5% FBS and incubated at 37°C for 3–4 days. Methylcellulose media was then aspirated, and cell monolayers were stained with a solution of crystal violet (0.1%) in formalin to facilitate identification and quantification of plaques. Percent neutralization was determined by comparison of the number of plaques in experimental wells compared to no-serum-added control wells, and each data point was the average of three wells.

Immunofluorescence

For confocal microscopy of frozen spleen sections, spleens were removed at the indicated day post-infection, fixed in periodate-lysine-paraformaldehyde fixative for 48 h, and then moved to 30% sucrose/PBS solution for 24 h. Tissues were embedded in optimal-cutting-temperature medium (Electron Microscopy Sciences) and frozen in dry-ice-cooled isopentane. 16-µm sections were cut on a Leica cryostat (Leica Microsystems, Buffalo Grove, IL). Sections were blocked with 5% goat, donkey, bovine, rat, or rabbit serum and then stained with a combination of the following Abs: ERTR7 (Abcam, Boston, MA), B220 (clone RA3-6B2, Biolegend), GL7 (clone GL-7, Thermo Fisher Scientific), and CD21/35 (clone eBio4E3, eBioscience, San Diego, CA). Sections were incubated with secondary antibodies as needed and for controls, and images were acquired on a Leica SP8 or Stellaris Confocal microscope. To increase staining intensity of MHV68, spleens were stained with anti-GFP Ab (EPR14104, Abcam) and goat anti-chicken Alexa Fluor 488 (ThermoFisher Scientific, Waltham, MA). Images were processed and analyzed using Imaris software 8.0 (Oxford Instruments). Where indicated, the spots function of Imaris was used to identify and create spots for MHV68+ cells. Spots were masked on TdTomato expression inside the spot to reveal MHV68+ tdTomato+ cells, referred to as “gated.”

RNA-sequencing

A quantity of 5 × 10⁴ cells sorted on the markers of interest by flow cytometry were spun down, resuspended in 50 µL of TRIzol, and stored at −80°C. GENEWIZ (South Plainfield, NJ) performed RNA extraction, quality control, library preparation, and Illumina sequencing.

The custom reference genome allowing quantification of both viral and host expression used in this alignment (“mm10_MHV68YFP_Krug”) consisted of the mouse reference (mm10/Apr. 2019/GRCm38) with a modified MHV68 sequence added as an additional pseudochromosome. This viral genome was prepared from the annotated herpesvirus genome (NCBI reference ) with the addition of a CMV-driven histone 2b-YFP fusion gene locus found in the recombinant MHV68-H2bYFP. The custom gene annotations used for gene expression quantification consisted of a concatenation of the mm10 GENCODE annotation version M21 [99] and annotations of the MHV68 genome. The first annotation (“mm10_MHV68YFP_Krug_Ov”) measures expression using complete viral ORF annotations, including those regions that overlap. In the second annotation (“mm10_MHV68YFP_Krug_NoOv”), overlapping regions of the viral ORFs were removed to create a minimal, non-overlapping annotation. This second annotation was used to make conservative estimates of the expression of individual viral genes reported here.

Raw sequencing files were aligned and counted using the CCR Collaborative Bioinformatics Resource in-house pipeline (). Briefly, reads were trimmed of low-quality bases, and adapter sequences were removed using Cutadapt v1.18 (http://gensoft.pasteur.fr/docs/cutadapt/1.18). Mapping of reads to the custom reference hybrid genome described below was performed using STAR v2.7.0f in two-pass mode (120, 121). Then, RSEM v1.3.0 was used to quantify gene-level expression (122), with quantile normalization and differential expression of genes analysis performed using limma-voom v3.38.3 (123). The data discussed in this publication, the custom genome reference FASTA, and both annotation GTFs have been deposited in and are accessible through GEO Series accession .

Bioinformatics analysis and visualization

Data analysis and visualization were performed in the NIH Integrated Analysis Portal (NIDAP) using R programs developed on Foundry (Palantir Technologies) for normalization, differential expression analysis, GSEA, and visualization. First, raw counts were imported and transformed to counts per million (CPM) and filtered to retain genes that had at least two samples with non-zero CPM counts in at least one group. Next, quantile normalization and batch correction across samples were used to account for factors that would prevent direct comparisons between samples. Heatmaps were created using the quantile-normalized, batch-corrected RNA-seq data. A principal component analysis demonstrating the within- and between-group variance in expression after dimensionality reduction was generated using NIDAP. Differential expression of genes analysis utilized log₂-CPM transformed raw counts, implemented with the Limma Voom R package. Volcano plots were created from DEG analysis of each comparison highlighting significant fold changes (log₂ fold change) >1 or <−1, with a significant P value (adj P value <0.05). GSEA in NIDAP used the Limma Voom calculated t-statistic ranking to test comparisons against the Broad Institute GSEA hallmark-curated gene sets. Bubble plots generated to display GSEA outputs were generated using SRPLOT (http://www.bioinformatics.com.cn/plot_basic_gopathway_enrichment_bubbleplot_081_en).

Gene signatures were developed using the Molecular Signature Database [MSigDB, (124)] with GO annotations provided by the Gene Ontology resource (125, 126). Germinal center signature was developed using intersection of the following GO data sets: GO:0002314, GO:0002467, GO:0002636, and GO:0002634, accessed on 15 December 2022. Viral infection signature was developed using intersection of the following GO data sets: Hallmark: MM3877, GO:0016032, GO:0039528, GO:0045071, GO:1903901, and GO:0002230. Hierarchical clustering heatmaps were generated using Morpheus (). Hierarchical clustering for all samples or 350 top variable genes was performed using a one minus pearson correlation metric, with complete linkage. CPM trimmed mean of M (TMM) values for viral ORFs were normalized using a scaling factor generated from median total viral counts of samples within a data set.

Statistical analyses

Data were analyzed using GraphPad Prism software (Prism 8; GraphPad Software, Inc., La Jolla, CA). Significance was evaluated by unpaired two-tailed t test, paired t test, one-way ANOVA, or paired one-tailed t test of the log-transformed frequency values of samples from matched experiments, as noted. Using Poisson distribution analysis, the frequencies of latency establishment and reactivation from latency were determined by the intersection of non-linear regression curves with the line at 63.2%.

ACKNOWLEDGMENTS

We thank the laboratories of Robert Yarchoan and Joseph M. Ziegelbauer for sharing critical equipment, as well as flow cytometry cores, animal facilities, and support staff at Stony Brook University and the National Institutes of Health. We also thank Adrianus Van Der Velden, Pawan Kumar, Flaminia Talos, and members of the Krug laboratory for helpful discussion. This work utilized the computational resources of the NIH HPC Biowulf cluster (http://hpc.nih.gov).

This research was supported in part by the Intramural Research Programs of the NIH, the National Cancer Institute (NCI) (C.H.H. and L.T.K.), and the National Institute of Allergy and Infectious Diseases (NIAID) (G.V.S. and H.D.H.). C.H.H., L.T.K., and N.C.R. were supported by NIH NCI RO1AI119079. S.M.O. was supported by a postdoctoral fellowship from Translational Research Institute (TRI) grant TL1 TR003109 through the NIH National Center for Advancing Translational Sciences. Y.L. was supported by a postdoctoral fellowship from Lymphoma Research Foundation. K.M.M. was supported by NIH NIAID R01AI12539, the Recombinant Antibody Production Core [CPRIT RP190507], and the Virginia Harris Cockrell endowment fund. B.E.G. was supported by NIH NIAID AI164709, NIH NCI CA228700, and U01CA275301. J.C.F. was supported by NIH NCI R01CA167065 and NIH NIAID R21AI139580.