key: cord-0774129-3aketsdo authors: Tschen, Shuen‐Ing; Stohlman, Stephen A.; Ramakrishna, Chandran; Hinton, David R.; Atkinson, Roscoe D.; Bergmann, Cornelia C. title: CNS viral infection diverts homing of antibody‐secreting cells from lymphoid organs to the CNS date: 2006-01-25 journal: Eur J Immunol DOI: 10.1002/eji.200535123 sha: 5bd9a8cbba75c8ee241ee3870d02dbe437b6f60f doc_id: 774129 cord_uid: 3aketsdo Neurotropic coronavirus infection of mice results in acute encephalomyelitis followed by viral persistence. Whereas cellular immunity controls acute infection, humoral immunity regulates central nervous system (CNS) persistence. Maintenance of serum Ab was correlated with tissue distribution of virus‐specific Ab‐secreting cells (ASC). Although virus‐specific ASC declined in cervical lymph node and spleen after infectious virus clearance, virus‐specific serum Ab was sustained at steady levels, with a delay in neutralizing Ab. Virus‐specific ASC within the CNS peaked rapidly 1 wk after control of infectious virus and were retained throughout chronic infection, consistent with intrathecal Ab synthesis. Surprisingly, frequencies of ASC in the BM remained low and only increased gradually. Nevertheless, virus‐specific ASC induced by peripheral infection localized to both spleen and BM. The data suggest that CNS infection provides strong stimuli to recruit ASC into the inflamed tissue through sustained up‐regulation of the CXCR3 ligands CXCL9 and CXCL10. Irrespective of Ag deprivation, CNS retention of ASC coincided with elevated BAFF expression and ongoing differentiation of class II(+ )to class II(–)CD138(+)CD19(+ )plasmablasts. These results confirm the CNS as a major ASC‐supporting environment, even after resolution of viral infection and in the absence of chronic ongoing inflammation. The preeminent goal of the immune system is to eliminate pathogens and establish immunological memory [1] . Both T cells and Ab participate in eliminating a variety of pathogens; however, sustained serum Ab is an important criteria for many vaccination strategies, as they provide the first line of defense against re-infection [2] . Upon Ag encounter in regional lymph nodes, B cells undergo clonal expansion in extrafollicular foci and within germinal centers [3, 4] . Rapidly activated B cells secrete low-affinity Ab but can undergo isotype switching and limited BCR hypermutation as they differentiate into plasmablasts [3] . In the milieu of accessory cells and cytokines, germinal center B cells undergo affinity maturation and ultimately differentiate into both Ab-secreting cells (ASC) and memory B cells. As Ag is depleted, ASC and memory B cells are detected with increasing frequency in BM [2] , where both stromal cells and other resident cells provide soluble as well as contact-dependent survival signals, including CXCL12 and BAFF [5] . Ab secretion by terminally differentiated plasma cells is independent of both Ag and T cell regulation [2, 6] . Long-lived ASC in BM and spleen maintain serum Ab, thus providing protective immunity to re-infection, sometimes for the life time of the host [2] . Upon re-infection memory B cells rapidly expand and differentiate into plasmablasts, constituting a crucial source to increase pathogenspecific Ab and replenish ASC [4, 6] . In contrast to Ag encountered in the periphery, the regulation of B cell activation by Ag sequestered within the central nervous system (CNS) is less clear. The absence of dedicated lymphatic drainage and the presence of the blood brain barrier (BBB) limits Ag transport from the CNS into secondary lymphoid tissue as well as trafficking of both cells and macromolecules into the CNS. In addition, CNS resident cells do not express MHC molecules [7] [8] [9] ; therefore, in the absence of inflammation, there is little possibility for endogenous Ag presentation, consistent with the inability to initiate immune responses within the CNS [10]. Nevertheless, Ag deposition into the CNS, under conditions in which the BBB integrity remains relatively intact, results in a robust local humoral immune response [11] . In situ ASC differentiation at the site of Ag deposition is preceded by peripheral activation, as implied by the early detection of Ag-specific ASC in cervical lymph nodes (CLN) and spleen and the necessity of CLN for intrathecal Ab production [11] . These data suggest that an Ag depot within the CNS is recognized as non-self and that functions associated with peripheral B cell differentiation are sustained within the CNS. A variety of CNS inflammatory diseases support trafficking and preferential retention of ASC within the CNS. During virusinduced encephalitis, B cells as well as virus-specific ASC and ASC of unknown specificities are found in the inflamed CNS [12-16]. Indirect evidence for intrathecal Ab synthesis includes oligoclonal Ab bands with restricted specificities in the cerebral spinal fluid (CSF) of patients with subacute sclerosing panencephalitis (SSPE) and multiple sclerosis (MS) [14, 17, 18] . Increased CSF to serum Ab ratios detected following a variety of experimental CNS viral infections and measles virus-induced encephalitis in humans further support local Ab production [15, 19, 20] . Similarly, during acute MS the BBB is compromised, potentially allowing ASC recruitment [21, 22] . Only a small portion of the oligoclonal bands in MS CSF are specific for a defined Ag [18, 23, 24] , while the oligoclonal Ab bands in the CSF of SSPE patients are specific for measles virus [19, 20] . These data suggest that B cells are recruited into the CNS during acute peripheral infections with neurological involvement as well as during loss of BBB integrity associated with autoimmunity. They also imply that the CNS provides a milieu capable of differentiating and maintaining ASC. Although chemokines and survival factors that influence preferential localization of ASC to the BM have recently been defined [5, 6, 15] , relatively little is known about mechanisms sustaining ASC within the CNS. Prolonged maintenance of anti-viral intrathecal Ab synthesis is a common trait following control of many acute viral CNS infections [15, 16, 25, 26] . Infection of the murine CNS with the neurotropic JHM strain of mouse hepatitis virus (JHMV) results in an acute CNS inflammatory response containing all cell types associated with anti-viral immunity, including B cells [12, 27] . Despite rapid recruitment of B cells into the CNS following JHMV infection, serum Ab is detected only after the majority of infectious virus has been eliminated [16] . The concept that humoral immunity is redundant during acute infection is supported by unimpaired initial clearance of infectious virus from the CNS of mice lacking the ability to secrete Ab [28, 29] and the absence of anti-viral ASC in the CNS of WT mice until after virus clearance [16] . However, a local Ab response within the CNS is required to control viral persistence [29] . Virus-specific ASC were measured to gain an understanding of organ-specific distribution following an inflammatory response confined to the CNS. Similar to virus-specific T cells [30] , ASC were detected within the spleen and CLN prior to the CNS [16] . Stable levels of anti-viral serum Ab suggest ASC in the BM as a primary source throughout persistence. However, virus-specific ASC were preferentially retained within the CNS and were barely detectable in BM throughout persistent infection of the CNS by JHMV, in contrast to preferential accumulation in BM observed for heterologous peripheral infections [2, [31] [32] [33] . High levels of virus-induced CXCL9 and CXCL10 mRNA within the CNS implicate CXCR3 ligands as mediators of ASC recruitment. Furthermore, BAFF mRNA up-regulation preceded ASC accumulation and remained detectable throughout ASC persistence. These data suggest that virus-induced CNS inflammation creates an environment that sustains local ASC, preenpting accumulation in the BM as a homeostatic maintenance site. until day 45 p.i. and then remained stable until day 90 p.i. (Fig. 1B) . The kinetics as well as retention of both neutralizing and isotype-specific Ab in serum were similar in infected BALB/c (H-2 d ) and C57BL/6 (H-2 b ) mice (data not shown), demonstrating the absence of a strain-dependent difference in the mouse haplotypes most commonly used to examine mouse hepatitis virus pathogenesis. Neutralizing as well as IgG and IgM serum Ab are thus sustained at constant levels following control of virus replication in the CNS. Following resolution of acute systemic and tissuespecific infections not involving the CNS, spleen and BM are the major sites harboring the ASC that maintain serum Ab levels [4, 6] . Sustained detection of serum JHMV-specific IgM and IgG after clearance of infectious virus from the CNS thus suggested continued Ig secretion by virus-specific ASC in BM or spleen. To examine potential contribution(s) of lymphoid organderived ASC in maintaining serum Ab levels following CNS infection, JHMV-specific ASC frequencies were examined longitudinally in spleen and BM. As ASC frequencies decline rapidly in CLN after day 15 p.i. [16] , maintenance in this compartment was not pursued. ASC frequencies in spleen were already low at day 21 p.i., with similar frequencies of virus-specific IgM and IgG ASC ( Fig. 2A) , consistent with the decline after day 10 p.i. [16] . Splenic IgG ASC further declined gradually with time p.i. but remained detectable. In contrast, the complete disappearance of IgM ASC by day 45 p.i. suggests distinct trafficking, differentiation and/or survival of IgM versus IgG ASC ( Fig. 2A) . IgG-secreting ASC in BM were barely detectable at day 21 p.i., whereas IgM ASC were not detected until day 45 p.i. (Fig. 2B) . The frequency of ASC in BM increased very slowly with time, implying ongoing recruitment and/or continued differentiation of memory B cells or plasmablasts. However, even at day 90 p.i., only a minimal frequency of ASC was detected in BM. These data suggest that only a small population of virus-specific ASC in peripheral organs contribute to sustained serum anti-viral Ab levels. Previous data revealed that virus-specific ASC frequencies peak within the CNS by day 21 p.i. and persist to at least day 30 p.i. at much higher levels than in secondary lymphoid organs [16] . The prolonged presence of ASC within the CNS following clearance of infectious virus contrasts with the rapid ASC decline in spleens and lungs following resolution of LCMV and Sendai virus infections [2, 31] . To determine the fate of ASC during persistence, virus-specific ASC frequencies within the CNS were monitored longitudinally. Both IgG and IgM virus-specific ASC in the CNS declined steadily after the peak at day 21 p.i. (Fig. 3 ). IgG ASC in the CNS declined to approximately 50% by day 60 p.i., and a further 50% loss occurred between days 60 and 90 after infection. The peak frequency of virus-specific IgM ASC was significantly reduced compared to IgG ASC and dropped by *50% between days 21 and 45 after infection. However, in contrast to IgG ASC, the frequency of virusspecific IgM ASC remained relatively constant between days 45 and 90 p.i. (Fig. 3) . Overall, the frequency of virus-specific ASC in the CNS at day 90 p.i. exceeded frequencies in peripheral organs (Fig. 2) . To characterize the distribution of ASC within the CNS, CD138 was used as a marker for pre-plasma and terminally differentiated plasma cells, with the caveat that this approach does not specifically identify virusspecific ASC. CD138 + cells were present in both gray and white matter, with a significant number in areas of demyelination in both spinal cord (Fig. 4A ) and brain (data not shown) at day 35 after infection. The respective areas were confirmed as demyelinated by staining adjacent serial sections with luxol fast blue (data not shown). At day 90 p.i., viral Ag had been cleared from the CNS, and demyelination was significantly ameliorated (data not shown); however, CD138 + cells were still present in the CNS (Fig. 4B , C). Substantial numbers of both IgG and IgM ASC were also detected at day 90 after infection. At 90 days p.i., CD138 + , IgG + and IgM + cells were widely distributed in both gray and white matter within the brain parenchyma and in perivascular areas within the spinal cords ( Fig. 4D -F). These data contrast with an ultrastructural examination of the CNS of mice approximately 1 year p.i. with a distinct variant of JHMV, which suggested preferential retention of plasma cells in the meninges [34] . Retention of ASC within the CNS parenchyma, associated with intrathecal Ab production, is consistent with an increased CSF to serum ratio of anti-viral Ab observed following JHMV infection in both mice and rats [35] [36] [37] . Organ-specific ASC distribution ASC frequency analysis reflects enrichment of distinct populations but does not recapitulate total numbers per organ. Data derived from experiments depicted in Fig. 2 and 3 were converted to ASC per tissue to account for overall higher numbers of lymphocytes in spleen and BM compared to the CNS. Vastly higher numbers of ASC were detected within the CNS compared to BM and spleen at day 21 p.i., irrespective of isotype (Fig. 5A, B) , suggesting preferential trafficking of pre-plasma cells into the CNS and/or more rapid local differentiation [11] . On a total tissue basis, IgG ASC numbers progressively declined within the CNS, remained relatively constant in spleen and slowly increased in BM, eventually reaching numbers equivalent to spleen at days 40-60 p.i. (Fig. 5A) . Slightly different dynamics were observed between days 60 and 90 p.i., when numbers continued to decline in spleen and CNS but increased in BM (Fig. 5A, B) . The continued decline of CNS IgG ASC by day 90 p.i. eventually resulted in an equal distribution of total IgG ASC in CNS and BM (Fig. 5A ). Although IgM ASC were not detected in BM at day 21 p.i. (Fig. 5B) , they ultimately increased, reaching numbers similar to the CNS by day 90 p.i. (Fig. 5B) . As terminally differentiated ASC are sessile [4, 5] , these dynamics presumably reflect progressive loss of survival factors within the CNS but continued differentiation of ASC within the BM, rather than redistribution from the CNS to the BM. However, the vastly greater virusspecific ASC frequencies and numbers per organ imply enhanced recruitment/survival factors within the CNS compared to peripheral lymphoid compartments following the resolution of encephalitis (Fig. 2, 4, 5) . Consistent with enhanced recruitment/survival within the CNS, increased virus-specific IgG plaque diameter with time p.i. suggests ASC maturation [38] . In contrast, the diameter of virus-specific plaques derived from BM remained relatively constant throughout infection (data not shown). To further explore differentiation of ASC within the CNS, infiltrating cells were analyzed phenotypically for expression of plasmablast markers. ASC are typically characterized by down-regulation of the B cell lineage markers B220 and CD19 but expression of CD138 [4] . Plasma cells furthermore lose class II expression through transcriptional repression of the class II transcriptional activator CIITA [4] . Flow cytometric analysis of CD45 hi brain infiltrates indicated a prominent increase of CD138 + cells between days 14 and 21 p.i. (Fig. 6A) , consistent with detection of virus-specific ASC by ELISPOT. CD138 + cells were B220but retained CD19 expression (data not shown). Although their percentage was low, CD138 + cells increased in frequency by day 70 p.i. (Fig. 6A) . Furthermore, whereas the majority of CD138 + cells expressed class II early during persistence, class IIcells dominated later. CD138 + class IIcells were even more abundant in spinal cords, the predominant site of persistence and demyelination [39] , by day 70 p.i. (Fig. 6B) . Surprisingly, CD138 + cells retained CD19 expression, suggesting incomplete differentiation. Nevertheless, decreasing class II surface expression on CD138 + pre-plasma cells supports ongoing differentiation for at least a 2-month period. These data suggest that plasmablasts are recruited into the CNS at early stages of differentiation from secondary lymphoid organs. Migration of plasmablasts into inflamed tissues frequently correlates with CXCL10 expression [40] [41] [42] . Transient responsiveness to the CXCR3 ligands CXCL9, 10 and 11 has also been shown to mediate plasmablast migration in vitro [40] . JHMV infection induces CNS expression of both CXCL9 and CXCL10 within 3 days p.i. [43] , potentially supporting recruitment of ASC. During CNS autoimmune disease, ASC accumulation is associated with expression of CXCL13, a ligand involved in B cell migration toward follicular DC, and expression of BAFF, a B cell and ASC survival factor [42, 44, 45] . Expression of mRNA for the chemokines CXCL9, CXCL10 and CXCL13 as well as BAFF was thus analyzed during acute replication and the persistent phase (Table 1 ). CXCL9 and CXCL10 mRNA were most prominent between days 8 and 14 p.i. and decreased substantially following clearance of infectious virus, confirming previous results [43] . The lack of CXCL13 mRNA expression implies the absence of follicular DC involvement and local lymphoid follicle formation [44] . BAFF mRNA levels peaked delayed compared to the CXCR3 ligands but preceded peak ASC accumulation (Table 1) . Although BAFF mRNA decreased slowly after day 21 p.i., levels were still elevated 5-fold over naive levels 75 days after infection. Thus, maximum BAFF mRNA levels preceded peak accumulation of virusspecific ASC and declined with similar kinetics as ASC during viral persistence. These data suggest that CXCL9 and CXCL10 function as recruitment cytokines and that BAFF constitutes a potential survival factor for ASC within the brain. To analyze whether the preferential localization of ASC within the CNS compared to BM is unique to virusinduced encephalitis, virus-specific ASC distribution was analyzed following a relatively benign self-limiting peripheral JHMV infection. Frequencies as well as total numbers of virus-specific IgG and IgM ASC were combined to facilitate comparison of CNS-restricted (Fig. 7A ) and transient peripheral (Fig. 7B ) viral infection. In contrast to the low frequencies of total virus-specific ASC in spleen and BM following CNS infection, peripheral infection resulted in substantially increased frequencies in the spleen as well as BM (Fig. 7B) . No ASC were detected in the CNS following peripheral infection, suggesting that in contrast to activated T cells [46] , activated B cells do not traffic into the CNS. Differences in ASC distribution were even more dramatic at the level of total number per tissue. Contrasting with the CNS infection (Fig. 7C) , the vast majority of virus-specific ASC localized to the spleen following peripheral infection (Fig. 7D) . Although total numbers of virus-specific ASC in BM of peripherally infected mice were lower than in spleen (Fig. 7D) , ASC numbers in BM still exceeded those in the CNS of infected mice (Fig. 7B) , suggesting no inherent defect in trafficking to BM. The overall paucity of peripheral ASC following CNS infection is consistent with limited viral Ag in lymphoid tissues and rapid recruitment into the CNS. Furthermore, enhanced virus-specific ASC elicited by peripheral viral infection presumably reflect higher viral Ag load. Nevertheless, the preferential retention of ASC in spleen following a peripheral infection contrasts with the distribution of ASC following immunization with inert Ag and either systemic or respiratory viral infections [2, 31, 47 ]. Humoral immune responses are essential for resolution of many acute viral infections, especially those caused by cytopathic viruses [48] . Furthermore, persisting serum Ab induced by previous infection or vaccination provides a strong defense against re-infection [2] . Long-lived BM ASC are thought to provide a major source of persisting serum Ab following a variety of acute systemic viral infections [2, 31, 49] . However, it has long been evident that the CNS also provides a preferred ASC survival niche [13, 15, 17] . Studies of experimental CNS infections in animal models, systemic viral infections in humans resulting in encephalitis as well as CNS autoimmune disease, especially MS, all imply intrathecal Ab production [13, 15, 17-20, 44, 50] . However, B cell recruitment and CNS survival signals following virus-induced inflammation are largely unexplored. The present data demonstrate that a neurotropic coronavirus infection limited to the CNS results in preferential recruitment and long-term ASC retention, despite clearance of infectious virus. Although the site of ASC differentiation is not resolved, kinetic parameters suggest initial activation in the periphery. Virus-specific ASC are detected in the lymphoid tissues prior to the CNS [16], similar to findings for T cells [30] . Consistent with their derivation from secondary lymphoid organ germinal centers, virus-specific ASC in the CNS emerge subsequent to germinal center reactions, which peak *12 days p.i. [4, 6] , and are sustained after viral Ag and inflammation have subsided. Assessment of plasmablast recruitment via their CD138 + phenotype revealed kinetics similar to those demonstrated by ELISPOT. Retained expression of CD19 and class II indicates migration at an early differentiation state. The subsequent relative increase in CD138 + cells and gradual loss of class II expression during the persistent state suggest ongoing local differentiation within the CNS and/or preferential survival of a more differentiated phenotype [21] . The former notion is supported by a substantially increased proportion of class II -CD138 + cells in spinal cords compared to brains at day 70 p.i. as well as increased spot size of ASC derived from brains at late compared to early times p.i. (data not shown). A role of CNS-localized persisting viral Ag in driving ASC differentiation and retention remains elusive. Intrathecal Ab secretion is associated with a variety of CNS infectious and autoimmune diseases and involves responses to self Ag as well as persisting microbial Ag [14, [51] [52] [53] . Although a small frequency of oligoclonal Ab in the CSF of MS patients are specific for Ag associated with viral infections acquired as young adults, the majority have as-yet-undefined specificities [18] . These data suggest that ASC can be retained within the human CNS for prolonged periods in the apparent absence of microbial Ag. However, a confounding issue is the role of self Ag in potentially propagating novel ASC subpopulations during chronic inflammation [23, 44] . During JHMV infection, virus-specific T cells decline rapidly as viral replication is controlled and Ag diminishes; nevertheless, T cell retention is prolonged in the continued presence of viral Ag/RNA [39] . In contrast, virus-specific ASC only reach peak levels after viral Ag is reduced to barely detectable levels and infectious virus is below detection limits. Their frequencies and total numbers subsequently also decline, albeit at a much reduced rate compared to T cells. These data imply distinct and largely Ag-independent ASC survival signals. Up-regulation of BAFF mRNA prior to peak ASC accumulation and a gradual concomitant decrease in BAFF mRNA levels and ASC after day 21 p.i. support BAFF as a likely candidate molecule required for ASC survival in the CNS [42, 44, 45] . Furthermore, the inability to detect CXCL13 weakens the concept of a potential role for local follicle formation in supporting de novo ASC generation, in contrast to involvement of this mechanism during chronic autoimmune disease [44] . In addition, ASC of multiple isotypes are retained within the CNS for prolonged periods following CNS JHMV infection [16] . Retention of IgM ASC in the CNS, persisting serum IgM and gradual accumulation in BM suggest a potential role for IgM in control of JHMV persistence, similar to other viral infections [48] . Irrespective of unique isotype patterns induced by distinct CNS infections, all isotypes can be sustained within the CNS [13] . Retention thus appears dependent upon the host's response to the virus itself and not a generalized response to CNS inflammation. Transient ASC detection within spleen is a common denominator in infections confined to the CNS as well as systemic, respiratory and intestinal infections [2, 13, 15, 31] . However, in contrast to systemic infections, in which a decline in splenic ASC numbers is counterbalanced by an increase in BM ASC, few ASC ever appear in the BM following JHMV infection. Preferential CNS retention, concomitant with poor BM accumulation, appears unique compared to localized infections of lung or intestinal tract [31, 33] and may reflect the primary role of intrathecal Ab in controlling viral persistence [13, 15, 16] . A prominent intrathecal Ab response to JHMV infection is supported by increased CFS to serum ratios of virus-specific antibodies in rats and mice [36] . In extreme cases, some animals only exhibited viral Ab in CSF and not in the corresponding serum [36] . Extremely limited ASC localization to BM suggests that ASC are diverted from a default trafficking pathway into the BM characteristic of peripheral infections [2] . Our data suggest that strong induction of both CXCL9 and CXCL10 within the CNS during acute infection mediates recruitment of CXCR3-expressing plasmablasts. Continued expression of these chemokines as virus is cleared may sustain ongoing recruitment as ASC continue to emerge from lymphoid organs. The elevated level of BAFF mRNA within the CNS supports induction of factors necessary for prolonged ASC survival [54] . Furthermore, in contrast to ASC apoptosis within inflammatory lesions following virus clearance from peripheral tissues, few apoptotic cells are detected in the CNS [55] , and ASC are retained in apparent preference to BM. Together these data support the concept that the CNS provides a milieu for sustained ASC viability and Ab secretion. The results are consistent with intrathecal Ab synthesis in a variety of human pathological conditions as well as rodent models [11, 13, 15, [18] [19] [20] . Importantly, the paucity of ASC in BM suggests that differentiating ASC are diverted and migrate toward virus-induced chemokines within the CNS. CXCL9 and CXCL10, early chemokines induced by JHMV [43] , are maintained during peak ASC recruitment and support a role for CXCR3 ligands in ASC recruitment. CXCL12 and BAFF, which are constitutively expressed at high levels in BM, may be candidates facilitating ASC retention in the CNS [6] . The recent discovery of BAFF up-regulation in CNS plaques associated with MS and in mice with experimental autoimmune encephalomyelitis [44, 45] provides a mechanism for the promotion of ASC survival during CNS autoimmune disease. Similarly, following CNS infection, BAFF was up-regulated concurrently with viral clearance, and mRNA expression was maintained within the CNS throughout persistence. These data suggest that maintenance of ASC during chronic viral infections associated with limited ongoing inflammation may involve components similar to chronic inflammatory diseases, albeit with limited contribution of viral Ag. Male 6-wk-old C57BL/6 and BALB/c mice, sero-negative for mouse hepatitis virus, were obtained from the National Cancer Institute (Frederick, MD). Mice were maintained in a specific pathogen-free environment and infected within 1 wk of arrival. CNS infection was induced by intracerebral inoculation of the neutralizing mAb-selected 2.2v-1 variant of JHMV [56] . Mice were injected in the left hemisphere with 30 lL containing 250 PFU JHMV diluted in endotoxin-free Dulbecco's PBS. For peripheral infections mice were injected i.p. with 1 Â 10 6 PFU JHMV as previously described [55] . All procedures were performed in compliance with Keck School of Medicine Institutional Animal Care and Use Committee approved protocols. Serum anti-JHMV Ab levels were determined by ELISA as previously described [16] . Briefly, 2-fold serum dilutions (pooled from three to five individuals per time point) were adsorbed overnight at 4 C onto 96-well plates coated with a serum-free supernatant derived from JHMV-infected DBT cells (6 Â 10 3 PFU/well) diluted in 0.1 M sodium phosphate buffer (pH 9). Bound Ab was detected with biotinylated goat antimouse IgG and IgM (Jackson ImmunoResearch Laboratories, West Grove, PA), avidin peroxidase and 1 mg/mL 2,2 0azinobis-(3-ethylbenzothiazoline-6-sulphonic acid) (ABTS; Roche Diagnostics Corp., Indianapolis, IN) in PBS containing H 2 O 2 . Optical densities were determined at 405 nm in a Microplate Autoreader (Bio-Tek Instruments, Winooski, VT) and titers calculated as reciprocals of the highest dilution that exceeded three standard deviations over the mean negative control. Neutralizing titers were determined as previously described using sera pooled from three to five individuals per time point [16] . Briefly, heat-inactivated sera (56 C for 30 min) were incubated with 200 PFU JHMV in 96-well plates for 90 min at 37 C. Following addition of DBT cells (9 Â 10 4 cells/well), cultures were incubated for 48 h at 37 C. Neutralization titers represent the highest dilution that prevented virus-induced cytopathic effects. Groups of four to six JHMV-infected mice were perfused with PBS at various times after infection. Single-cell suspensions from spleen or BM were depleted of red blood cells by Trisbased ammonium chloride treatment and resuspended in RPMI medium containing 25 mM Hepes (pH 7.2) supplemented with 10% FCS. CNS mononuclear cells were isolated as previously described [16] . Briefly, brains and spinal cords were mechanically dissociated and the homogenate adjusted to 30% Percoll (Amersham Pharmacia Biotech, Piscataway, NJ). A 70% Percoll underlay was added prior to centrifugation at 800 Â g for 25 min at 4 C. Mononuclear cells were recovered from the 30%/70% interface, diluted in serum-free RPMI medium containing 25 mM Hepes, collected by centrifugation and washed three times. For ELISPOT analysis cells were resuspended in RPMI containing 25 mM Hepes and 10% FCS. For flow cytometry, cells were blocked with 10% mouse sera and rat anti-mouse CD16/32 (2.4G2; BD PharMingen, San Diego, CA) prior to staining with labeled mAb specific for CD45 (30-F11), CD19 (1D3), B220 (RA3-6B2), CD138 (281-2) and MHC class II (2G9). All mAb were obtained from BD PharMingen. Cells were analyzed with a FACSCalibur flow cytometer (Becton Dickinson, Mountain View, CA) using Cellquest Pro software. Forward and side scatter signals were used to establish a gate excluding dead cells and tissue debris, and at least 50 000 events were analyzed. Virus-specific ASC were detected by ELISPOT as previously described [16] . Briefly, Millipore Multiscreen 96-well plates (Bedford, MA) were coated by overnight incubation at 4 C with supernatant collected from JHMV-infected DBT cells propagated under serum-free conditions (*5 Â 10 5 PFU/ well). Control wells were coated with virus-free medium. Mononuclear cells isolated from spleen, BM and CNS were added at various dilutions and incubated for 4 h at 37 C. Single-cell spots were visualized by sequential addition of biotinylated goat anti-mouse IgG or IgM (Jackson ImmunoResearch Laboratories), avidin peroxidase (Sigma, St. Louis, MO) and 3,3 0 -Diaminobenzidine substrate (Sigma). Color was developed at room temperature for 5-10 min. The wells were then washed with water, air dried and the spots counted using a dissecting microscope. ELISPOT images were taken by using Zeiss KS Elispot imaging system. Mice were perfused with PBS, and brains and spinal cords were removed and snap frozen. Distribution of IgG and IgM ASC was determined by staining acetone-fixed sections with biotinylated goat anti-mouse IgG or IgM (Jackson ImmunoResearch Laboratories). Plasma cell distribution was examined using anti-CD138 (BD PharMingen). Slides were counterstained with hematoxylin and scored in a blinded manner. RNA was extracted from half brains of individual mice (three per group) by homogenization in guanidine isothiocyanate. Samples were sheared prior to centrifugation in 5.7 M cesium chloride (100 000 Â g for 18 h) and treated with DNAase I (Roche) to avoid DNA contamination. AMV reverse transcrip-tase (Promega, Madison, WI) was used for reverse transcription. 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The authors wish to express their gratitude to Wenqiang Wei, Emmanuel Dimacali and Ernesto Barron for excellent technical assistance with the immunohistochemistry, real-time PCR and photography.