Germinal Center Initiation, Variable Gene Region Hypermutation, and Mutant B Cell Selection without Detectable Immune Complexes on Follicular Dendritic Cells

doi:10.1084/jem.192.7.931

Published online 2 October 2000.

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© The Rockefeller University Press, 0022-1007/2000/10/931/ $5.00
The Journal of Experimental Medicine, Volume 192, Number 7, October 2, 2000 931-942

Original Article

Germinal Center Initiation, Variable Gene Region Hypermutation, and Mutant B Cell Selection without Detectable Immune Complexes on Follicular Dendritic Cells

Lynn G. Hannum^a, Ann M. Haberman^a, Shannon M. Anderson^a, and Mark J. Shlomchik^b

^a Section of Immunobiology, Yale University School of Medicine, New Haven, Connecticut 06510
^b Department of Laboratory Medicine, Yale University School of Medicine, New Haven, Connecticut 06510
Department of Laboratory Medicine, Yale University School of Medicine, P.O. Box 208035, 330 Cedar St., New Haven, CT 06520-8035.203-688-2748203-688-2089

Abstract

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Serum antibody (Ab) can play several roles during B cell immuneresponses. Among these is to promote the deposition of immunecomplexes (ICs) on follicular dendritic cells (FDCs). ICs onFDCs are generally thought to be critical for normal germinalcenter (GC) formation and the development and selection of memoryB cells. However, it has been very difficult to test these ideas.To determine directly whether FDC-bound complexes do indeedfunction in these roles, we have developed a transgenic (Tg)mouse in which all B lymphocytes produce only the membrane-boundform of immunoglobulin M. Immune Tg mice have 10,000-fold lessspecific Ab than wild-type mice and lack detectable ICs on FDCs.Nonetheless, primary immune responses and the GC reaction inthese mice are robust, suggesting that ICs on FDCs do not playcritical roles in immune response initiation and GC formation.Moreover, as indicated by the presence and pattern of somaticmutations, memory cell formation and selection appear normalin these IC-deficient GCs.

Key Words: B lymphocyte • transgenic mouse • surface immunoglobulin • lambda light chain • immunological memory

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Immune responses in the spleen begin with proliferating B andT cells at the interface of the T and B cell zones 1 2. Withina few days, early Ab-forming cells (AFCs) are seen, which providethe first sources of serum Ab. The B cells that participatein the early extrafollicular reaction are generally of low affinity3. By day 6 after immunization, the first signs of the germinalcenter (GC) reaction are evident. Over the next 10 d, the GCreaction peaks, culminating in the selection of higher affinitymutants and the differentiation of both memory cells and plasmacells.

Follicular dendritic cells (FDCs) are thought to play a keyrole in the formation of GCs, as well as in selection, differentiation,and maintenance of memory B cells. FDCs are dendritiform, nonphagocyticcells found in the follicles of secondary lymphoid organs 4.A striking characteristic of FDCs is their ability to retainnative immune complexes (ICs) on their surface for long periodsof time 5. The half-life of radiolabeled Ags on FDCs is months,if not years 6. Complement receptors (CRs) provide the mainmechanism for ICs trapping on FDCs. C3 fragments bound to ICsbind CR1 (CD35) and CR2 (CD21), which are highly expressed onFDCs 7 8. Depletion of C3 by cobra venom factor inhibits Ag localizationto FDCs 9, as does treatment with anti-C3 10 or anti-CR1/2 11.ICs also bind Fc receptors on FDCs, particularly during theGC response 11. Hence, except for certain Ags that might fixsufficient complement autonomously, both mechanisms for Ag retentionby FDCs require that Ag be complexed with Ab.

Several important functions have been postulated for the ICsthat deposit on FDCs. It has been hypothesized that the initiallocalization of ICs on FDCs nucleates the GC response and providesthe Ag to which GC B cells respond 6 12. This idea provides anexplanation for the delayed appearance of GCs, since severaldays would be needed to provide the Ab required to allow ICsto form and deposit. Not all earlier data agree with this roleof IC deposition on FDCs. Kroese et al. reported that rats whichare reconstituted with mature lymphocytes after irradiationcan make early GC responses to SRBC immunization even thoughtheir FDCs are transiently impaired in IC trapping at the timeGCs are first observed 13. ICs on FDCs have also been suggestedto provide the stimulus that rescues centrocytes from apoptosis14, thus leading to the formation of memory B cells. The initiationof somatic mutation, which normally occurs in the GC, may alsodepend on encounter with Ag on the FDCs. Competition with previouslyformed Ab for Ag sequestered in ICs on FDCs is thought to driveaffinity maturation of B cells 15. Thus, ICs are thought todrive the initiation and normal progression of GC and memorycell development.

Although these proposed roles for ICs retained on FDCs fit withvarious correlative data, they have been difficult to evaluateexperimentally. Mice that lack TNFR family receptors or ligandslack FDCs and also generally lack GCs. The study of immune responsesin these animals has been used to draw conclusions about theroles of FDCs 16 17. Although there are clearly some memory formationdefects in these mice, the interpretation of these data is complicated.It is difficult to attribute the mechanism of immune responsedefects because these mice have markedly disorganized lymphoidarchitecture, as well as carry mutations in key cytokine orchemokine pathways 18 19 20 that may have direct effects on lymphocyteresponses. Moreover, studies in these mutant strains do notdistinguish between the role of FDC-bound ICs and other essentialfunctions of the FDCs since neither are present.

An additional informative approach has been the study of micethat lack CR1/2, in which the FDC's ability to capture Ag isreduced. These mice make very weak Ab responses to T cell–dependentAgs, as well as reduced GC responses 21 22. However, at leasta substantial part of the deficiency was due to disruption ofCR1/2 expression on B cells, and not primarily due to FDCs lackingthe ability to capture ICs via CR1/2 21 23. In any case, Ag maydeposit on FDCs via Fc receptors even in the absence of theCR1/2 receptor 11.

To better define the roles of ICs on FDCs, it would be advantageousto study B cell immune responses in the absence of secretedAb and hence in the absence of IC deposition on FDCs. To accomplishthis, we have developed a transgenic (Tg) mouse in which B cellsare functional but cannot secrete Ab. The membrane Ig (mIg)Tg consists of a rearranged VDJ joined to an IgM H chain fromwhich the secreted exon and polyadenylation site had been excised24. We chose to use Vh186.2 so that pairing of the Tg H chainwith endogenous ${lambda}$ light chain would result in a small, readilydetectable population of cells specific for the hapten (4-hydroxy-3-nitrophenyl)acetyl (NP). As mIg Tg mice have markedly reducedAb and undetectable IC deposition on FDCs, we have used themto investigate the role of Abs in the development and maintenanceof primary and secondary immune responses.

Materials and Methods

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

mIg Construct and Tg Mouse Production.
The mIg H chain construct was as described 24. In brief, a rearrangedVDJ segment containing Vh186.2 was ligated to an IgM^a constantregion from which the secreted exon and polyadenylation sitehad been excised, resulting in production of only membrane-boundIg. The construct was tested by transfection into CH1, a ${lambda}$ /IgM^b-expressingcell line 25. CH1-mIg transfectants expressed surface IgM^a anti-NP,yet did not secrete any detectable IgM^a into culture supernatant(data not shown). A control strain, the membrane plus secretedIg ([m+s]Ig) Tg, was produced using a similar construct withan intact secreted exon.

Tg-positive founders were identified by Southern blot. mIg Tgmice were first backcrossed with CB.17 mice (IgM^b congenicsof BALB/c). Levels of Tg-derived surface IgM^a expression onB cells from the founder lines were compared with the (m+s)Igcontrol strain by FACS^®; two that matched the (m+s)Ig Tgmice closely were chosen for study. To eliminate endogenousH chain production, the mIg Tg x CB.17 mice were backcrossedonto the JH knockout strain (JHD/CB.17). The resulting strain,referred to as mIg Tg, has >99% CB.17 background genes. mIgTg mice are housed under specific pathogen-free conditions andreceive Sulfatrim in drinking water 4 d/wk.

Ags and Immunizations.
Chicken gamma globulin (CGG; Sigma-Aldrich) and human serumalbumin (HSA; Amour Pharmaceutical) were haptenated with NP-hydroxysuccinimideester (Cambridge Research Biochemicals/Genosys). 7–12-wk-oldmice were immunized intraperitoneally with 50 µg alum-precipitatedNP₂₄CGG or NP₁₅HSA. For secondary immunizations, 50 µgsoluble Ag was administered in PBS.

ELISA.
Anti-NP was measured as ${lambda}$ ⁺ Ig that binds to (4-hydroxy-3-nitro-2-iodo-phenyl)acetyl(NIP)-BSA–coated plates. In the context of the Vh186.2Tg, this should account for virtually all anti-NP, and includesall Ig H chain isotypes. Immulon 2 plates (Dynex Technologies)were coated overnight with NIP₂₆-BSA. Plates were blocked with1% BSA, followed by incubation with serial dilutions of serumat 37°C for 1 h. After washing and incubation with polyclonalanti- ${lambda}$ –alkaline phosphatase (Southern Biotechnology Associates,Inc.) plates were developed with p-nitrophenyl phosphate (Sigma-Aldrich).For anti-IgM ELISA, plates were coated overnight with b7-6 (anti-IgM)and blocked with 1% BSA; anti-IgM–alkaline phosphatase(Southern Biotechnology Associates, Inc.) was used as the secondaryAb.

Flow Cytometry.
FACS^® was performed as described 26. PE (Molecular Probes)haptenated with NIP-hydroxysuccinimide ester (NIP-PE; CambridgeResearch Biochemicals/Genosys) was used to identify NP-specificB cells, as Vh186.2/ ${lambda}$ recognizes NIP with high affinity. In additionto NIP-PE, splenocytes were stained with anti- ${lambda}$ –fluorescein(Southern Biotechnology Associates, Inc.), and GL-1–biotin(anti–B7-2) followed by streptavidin–Spectral red(Southern Biotechnology Associates, Inc.).

Histology.
5 µm frozen spleen sections were thaw mounted onto poly-L-lysine(Sigma-Aldrich)–coated slides, fixed in cold acetone for10 min, and stored at –80°C. Tissue was blocked with1% BSA (Gemini Bioproducts) in PBS/0.1% Tween 20, or with 1%ovalbumin (ICN Biomedicals) containing 10% rat serum (GeminiBioproducts) when staining with mouse anti-HSA. Sections werestained with peanut agglutinin–horseradish peroxidase(PNA-HRP; EY Labs), anti- ${lambda}$ –alkaline phosphatase (SouthernBiotechnology Associates, Inc.), anti-CD35–biotin (BDPharMingen), anti-CGG–biotin (Accurate), or anti-HSA–biotin.Anti-HSA was affinity purified from serum of HSA-immune BALB/cmice; serum was complement inactivated at 56°C for 30 min,diluted 1:1 with PBS containing 0.05% sodium azide, and runover a column of HSA-coupled Affi-Gel 15 (Bio-Rad Laboratories).Eluted anti-HSA was then conjugated to biotin-XX (MolecularProbes).

In Vitro Deposition of ICs.
Goat anti-CGG (Southern Biotechnology Associates, Inc.) andCGG protein were mixed together at a weight ratio of 2:1 withfresh 10% mouse serum in PBS on ice for 30 min to form ICs atthe dilutions indicated. ICs were incubated at 37°C for1 h on acetone-fixed sections of spleen from an mIg Tg mousethat had received 50 µg NP-CGG in alum 12 d earlier. Thedeposited complexes were detected with a biotinylated donkeyF(ab')₂ anti-CGG Ab (Accurate) and developed with streptavidin–alkalinephosphatase reagent. The in vivo–localized Ag was developedat the same time in both the mIg Tg mouse (same mouse as usedfor the in vitro localization) and the day 9 immune (m+s)IgTg mouse for negative and positive controls, respectively, usingthe same detection Ab and substrate.

Sequencing.
${lambda}$ ⁺ day 16 GCs were microdissected from stained spleen sections.Cell clusters were digested overnight at 37°C in 20 µl25% PBS containing 10 µg proteinase K. V ${lambda}$ 1 sequences wereamplified by nested PCR using Pfu (Stratagene): external primers5'-GCACCTCAAGTCTTGGAGAG-3' and 5'-ACTCTCTCTCCTGGCTCTCA-3', andinternal primers 5'-CTACACTGCAGTGGGTATGCAACAATGCG-3' and 5'-GTTCTCTAGACCTAGGACAGTCAGTTTGG-3'.Amplified DNA was isolated by phenol/chloroform/isoamyl alcohol(25:24:1) extraction followed by gel purification, digestionof gel blocks with GELase (Epicentre), and ethanol precipitation.V ${lambda}$ 1 DNA was ligated via T4 DNA ligase (New England Biolabs, Inc.)to pBluescript II KS (Stratagene) cut with PstI and XbaI (NewEngland Biolabs, Inc.). Ligation products were transformed intoDH5 ${alpha}$ . V ${lambda}$ 1 DNA was further amplified by placing colonies directlyinto PCR reactions containing the following primers: 5'-AATTAACCCTCACTAAAGGG-3'and 5'-GTAATACGACTCACTATAGGGC-3'. DNA was purified from thePCR reaction mixture with GFX DNA and Gel Band Purificationkit (Amersham Pharmacia Biotech), mixed with sequencing primer5'-TCGAGGTCGACGGTATC-3', and sequenced by the Keck BiotechnologyResource Laboratory at Yale University School of Medicine usingApplied Biosystems 377 DNA sequencers.

Statistics.
The unpaired t test was performed using StatView v4.5 (AbacusSoftware). P < 0.05 was considered significant.

Results

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

The mIg Tg Reconstitutes NP Binding by ${lambda}$ ¹ B Cells but without Detectable Anti-NP Ab.
The mIg Tg has been backcrossed onto the JH knockout strain(JHD/JHD), and thus only the Tg-encoded H chain V region isexpressed. As predicted, expression of Vh186.2 in all B cellsyields 2–4% of splenocytes in an unimmunized mIg Tg mousethat are NP specific and ${lambda}$ ⁺ by FACS^® analysis (Fig. 1). Thecontrol (m+s)Ig Tg strain, made from an otherwise identicalconstruct that retains the intact secreted exon, has a similarNP-specific population. To confirm that mIg Tg B cells werenot capable of secreting IgM upon stimulation in vitro, mIgTg splenocytes were cultured for 5 d with 50 µg/ml LPS(Fig. 2). As expected, mIg Tg splenocytes did not produce anydetectable IgM. Splenocytes from mIg Tg mice with intact endogenousIg Jh alleles did produce IgM, presumably emanating from a smallnumber of B cells that expressed endogenous H chains.

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Figure 1 The mIgM Tg rescues B cell development and confers specificity for NIP on ${lambda}$ ⁺ B cells when expressed on the JHD background. FACS^® profiles of splenocytes from CB.17 (left) or mIg Tg mice (JHD background) are shown. The top row demonstrates sole expression of IgM^a in the mIg Tg mice. The bottom row demonstrates that ${lambda}$ ⁺ B cells in the mIg Tg mice bind to NIP (as NIP-PE) in proportion to the amount of surface ${lambda}$ . There are practically no detectable ${lambda}$ ⁺ NP-binding cells in the CB.17 mice (bottom left).

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Figure 2 Lack of secretion of IgM from mIg Tg mice after stimulation by LPS in vitro. Splenocytes from mIg Tg mice (i.e., on the JHD background) and the original mIg x CB.17 mice (which expressed some endogenous H chain) were cultured with 50 µg/ml LPS for 5 d to determine their capacity to secrete IgM in vitro. Supernatants from multiple wells were pooled and total IgM was quantitated by ELISA.

No NP-specific Ig could be detected in sera from naive mIg Tgmice, even with an assay sensitivity of 20 ng/ml; indeed, mIgTg sera were indistinguishable from JHD/JHD control sera (datanot shown). Anti-NP concentrations in unimmunized (m+s)Ig Tgand CB.17 mice were in the range of 1 µg/ml.

mIg Tg Mice Mount Primary Responses.
Having eliminated preexisting Ab, we asked whether mIg Tg micewould develop a normal primary response, since ICs might beimportant in the initial stimulation of B cells 27 28. To determineif primary responses in mice with similar B cell repertoireswould be diminished by lack of Ab, mIg Tg and (m+s)Ig Tg micewere immunized with NP-HSA, NP-CGG, or CGG alone, and splenocyteswere analyzed by FACS^® between days 0 and 28 (Fig. 3). Ag-specificB cells bound NIP-PE and expressed ${lambda}$ light chain (Fig. 1). InNP-immunized mIg Tg and (m+s)Ig Tg mice, Ag-specific B cellscomprised an increasingly large percentage of the splenocytes(Fig. 3 A), peaking between days 12 and 16. Similar effectswere seen on the total number of NP-specific cells (data notshown). There is a similar proportional increase of NP-specificcells in both strains. By day 28, the percentage of NP-specificcells in both Tg strains had dropped, although not yet backto baseline levels. NP-specific B cells in carrier-immunizedcontrols remained near baseline levels.

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Figure 3 Time course analysis of primary response to NP immunization. mIg and (m+s)Ig Tg splenocytes were analyzed by FACS^® at various time points after immunization with NP-HSA, NP-CGG, or CGG alone. (A) Mean percentages of NP-specific splenocytes; (B) the mean percentage of NP-specific splenocytes that are B7-2^high. Error bars indicate SEM. Numbers of mice: d0, n = 4; d28, n = 3; d5–16, NP-HSA, n = 3; CGG mIg Tg, n = 4–5; NP-CGG mIg Tg, n = 5–6; CGG (m+s)Ig Tg, n = 3; NP-CGG (m+s)Ig Tg, n = 4–7. Data are combined from three experiments.

To provide evidence of Ag-specific activation of mIg Tg B cells,we determined the percentage of NP-specific splenocytes expressinghigh levels of B7-2 after immunization with NP or carrier (Fig. 3B). The percentage of B7-2^high NP-specific cells peaks at day12 in both mIg Tg and (m+s)Ig Tg mice, whereas levels in carrier-immunizedmice remain low. These results indicate that mIg Tg B cellsbecome activated upon immunization, with kinetics similar tothose of (m+s)Ig Tg controls.

Ab Levels in mIg Tg Serum Are Markedly Reduced.
In spite of robust proliferative responses that resulted in15–20% of total splenocytes carrying the NP specificity,serum Ab responses to immunization in mIg Tg mice were severelyblunted and required an ultrasensitive assay for detection.At day 12 after immunization with NP-HSA, there was a mean of90 ng/ml anti-NP in mIg Tg sera; five of six mice had $≤$ 60 ng/ml(Fig. 4). This quantity of NP Ab is 100-fold less than in immunized(m+s)Ig Tg mice and 10,000-fold less than in immunized CB.17mice, despite the much higher precursor frequency of NP-specificB cells in mIg Tg mice than in CB.17 mice.

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Figure 4 Ab secretion is markedly reduced in mIg Tg mice. NP Ab levels from mIg Tg, (m+s)Ig Tg, and CB.17 mice bled on day 12 after receiving 50 µg NP-HSA. Error bars indicate SEM. Note that mIg Tg mice produce $~$ 10,000-fold less NP Ab compared with wild-type CB.17 mice.

It was surprising to find any serum Ab in mIg Tg mice sinceendogenous JH loci in these mice are inactivated. Shedding ofmIgM is unlikely to account for this, given our inability todetect any secreted IgM in vitro after LPS stimulation. Someof the Ab is IgG (data not shown), and thus we believe thatthese minute quantities of Ab arise via rare interchromosomalisotype switch events between the Tg locus and the endogenousIgH loci 29. Regardless of the mechanism by which this Ab emerges,the quantity of anti-NP at day 12 after immunization in mIgTg mice is three orders of magnitude less than the amount ofimmunizing Ag, whereas in CB.17 mice, Ab is far in excess ofAg. This indicates that if any ICs form in the mIg Tg model,the amount must be radically reduced. In particular, the likelihoodthat two Ab molecules would bind Ag in close proximity, as requiredfor C' activation, is remote given the extreme Ag excess.

mIg Tg Mice Produce NP-specific GCs.
The second question addressed in these studies was whether GCswould form in the absence of IC deposition. This question wasraised by the suggestion that early and/or preexisting Ab wasrequired in order to promote the shift to the GC reaction 12.If so, GC formation in mIg Tg mice—with no preexistinganti-NP and a 4-log reduction in Ab at a time when the GC responsepeaks—should be impaired. To investigate this, spleensections from mIg Tg, (m+s)Ig Tg, and CB.17 mice, removed onday 12 after immunization, were double-stained with PNA andanti- ${lambda}$ to identify ${lambda}$ ⁺ (NP-specific) GCs. mIg Tg mice producedNP-specific GCs upon immunization with either NP-CGG or NP-HSA;carrier-immunized mIg Tg mice produced only ${lambda}$ ^– (presumablycarrier-specific) GCs (Fig. 5 and Fig. 6). The number of NP-specificGCs present in the mIg Tg spleens was equal to or greater thanthat in the (m+s)Ig Tg or CB.17 spleens (Fig. 6), indicatingthat the mIg Tg GC response is not diminished by lack of Abor ICs. Indeed, as is evident from the substantially greatersize of the GCs in both types of Tg mice compared with thosein CB.17 mice (Fig. 6), the Tg mice make extremely vigorousGCs. Moreover, the kinetics of the GC response is similar inthe two types of Tg mice (data not shown). The normal GC responsein mIg Tg mice is not solely attributable to the enriched anti-NPrepertoire, as carrier Ags also induce GCs despite the presumablybelow normal precursor frequencies for the carrier epitopes(Fig. 5 B, Fig. 6, and data not shown).

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Figure 5 mIg Tg mice produce GCs. Spleens from mIg Tg, (m+s)Ig Tg, and CB.17 mice were removed on day 12 after immunization with NP-CGG or CGG. Spleen sections were stained with PNA-HRP (red) to detect GCs and anti- ${lambda}$ light chain (blue) to detect ${lambda}$ -expressing B cells. Immunization with NP-CGG produces ${lambda}$ ⁺ NP-specific GCs: (A) mIg Tg, (C) (m+s)Ig Tg, (D) CB.17. Immunization with CGG produces only ${lambda}$ ^– GCs (B; mIg Tg). Note the much larger size of the GCs from mIg Tg and (m+s)Ig Tg mice (A–C) compared with wild-type mice (D).

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Figure 6 mIg Tg mice make a normal number of GCs in response to immunization. The mean number of NP-specific GCs per random 40x view of spleen sections; error bars indicate SEM. Means represent counts from three to eight mice per treatment group. Bar heights show total number of GCs. The number of ${lambda}$ ⁺ GCs is indicated by the hatched bars and the number of ${lambda}$ ^– GCs by the gray bars. unim, unimmunized.

Lack of Detectable Ag Localization in mIg Tg Mice.
To confirm that the marked reduction in specific Ab levels inmIg Tg mice prevented normal localization of Ag to the FDCs,adjacent spleen sections were stained with a polyclonal antiserumspecific for the protein Ag carrier or with monoclonal anti-CD35,along with PNA. This strategy identifies Ag deposited on FDCsin GCs. A rigorous test of Ab-mediated localization of Ag issecondary immunization, in which case any leakiness in the systemshould be revealed. 5 wk after receiving 50 µg NP-CGG,mIg and (m+s)Ig Tg mice were given 50 µg NP-CGG intravenouslyin PBS. Spleens were removed at day 3 after reimmunization,and serial spleen sections were stained. There was no detectablelocalization of Ag in mIg Tg spleens, whereas numerous FDC networksin (m+s)Ig Tg spleens stained darkly with anti-CGG (Fig. 7A–D).Similar results were achieved when mIg and (m+s)Ig Tg mice werereimmunized with NP-HSA 12 wk after primary immunization andspleen sections were stained with anti-HSA (Fig. 7E–H).Note from the serial sections stained with anti-CR1/2 to revealFDCs that the pattern of Ag deposition matched the distributionof FDCs. We also investigated primary responses: as expectedfrom the secondary response data, at day 12 after NP immunization,no Ag was detectable in mIg Tg mice, whereas Ag was clearlyvisible in many (m+s)Ig Tg GCs (Fig. 8 and data not shown).

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Figure 7 Lack of Ag localization in mIg Tg mice. Spleens were removed on day 3 or 5 after secondary immunization with NP-CGG (A–D) or NP-HSA (E–H), respectively, from either mIg Tg (A, B, E, and F) or (m+s)Ig Tg (C, D, G, and H) mice. Serial spleen sections were stained with PNA-HRP to show GCs (red), plus anti-CGG (A and C) or anti-HSA (E and G) to detect localized Ag (blue), and anti-CD35 (B, D, F, and H) to visualize FDCs (blue). FDCs are present in mIg Tg mice; however, no Ag localization was detected in any mIg Tg GCs. Original magnification: x40 (A–F) and x100 (G and H).

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Figure 8 Estimation of the sensitivity of IC detection on FDCs in vivo. ICs that had been naturally deposited in vivo or artificially in vitro were detected using the same reagents at the same time, as described in detail in Materials and Methods. Since mIg Tg mice are negative in the in vivo deposition assay (B and see Fig. 7), we undertook this experiment to estimate the dynamic range of the assay and to establish the minimum amount of reduction needed in the mIg Tg in order to have a negative result. Thus, a dilution series was constructed for the in vitro ICs, which were then assayed on serial sections of mIg Tg spleen. All staining and development were performed simultaneously and stopped at the same time. A shows typical in vivo localization in (m+s)Ig Tg mice. B shows the lack of such in a mIg Tg mouse. D–F show various dilutions of the IC titrations: (C) 20 µg/ml; (D) 2.5 µg/ml; (E) 0.15 µg/ml; and (F) 0.05 µg/ml. The intensity of staining in C was comparable to the in vivo positive in A. At 400-fold less ICs (F), staining is barely detectable in nearly all GCs (F; and other similar GCs not shown), indicating an endpoint for the titration. Thus, there is an $~$ 400-fold dynamic range of the assay, and lack of staining roughly corresponds to a 400-fold or greater reduction in deposited ICs.

The sensitivity of detection was investigated using an in vitroIC-localization assay to construct a standard curve for comparisonwith simultaneous staining of in vivo samples (see Materialsand Methods). In vitro–prepared ICs using CGG and a polyclonalanti-CGG were incubated in the presence of fresh mouse serumwith spleen sections from day 12 immune mIg Tg mice. Since essentiallyall GCs in mIg Tg mice are ${lambda}$ ⁺ and thus NP specific (see Fig. 6),there should be few if any B cells in GCs of these immune micethat could bind the carrier Ag CGG. Binding to FDCs was detectedusing labeled anti-CGG, as performed for in vivo Ag localizationstudies in Fig. 7. The quantities of ICs were then titratedand an endpoint dilution was established (Fig. 8). The patternof this distribution resembles that of FDCs, as determined bystaining with anti-CR1/2 on adjacent sections (data not shown).Moreover, no such localization was seen in the absence of asource of fresh C' (data not shown), again strongly indicatingthat deposition on FDCs, rather than binding to B cells, isbeing observed. The dilution that gave similar intensity ofstaining to the in vivo localization that was detected simultaneouslyon sections from (m+s)IgM Tg mice was identified. By comparingthis to the endpoint, a minimum estimate of the sensitivitywas obtained. We estimate this to be 400-fold less than theintensity routinely seen in the (m+s)IgM Tg mice, thus attributingan order of magnitude to the meaning of lack of detectable ICsin the mIg mice.

mIg Tg GC B Cells Undergo Somatic Mutation of the V ${lambda}$ Region.
Somatic mutation of Ig genes is a hallmark of memory B cells30. Selection of mutations, presumably based on higher affinity,occurs concurrent with memory B cell development 31. In TNFRfamily knockout mice, memory B cell development was abnormal.To determine whether lack of ICs on FDCs affected memory B celldevelopment by altering mutation or selection in the mIg Tgmice, we microdissected NP-specific GCs from spleen sectionsof mIg Tg and (m+s)Ig Tg mice at day 16 after immunization andsequenced the endogenous V ${lambda}$ 1 genes.

Clearly, mutation is occurring in mIg Tg mice, with the averageV ${lambda}$ having 1.4 mutations in $~$ 300 basepairs sequenced. This frequencyis comparable to the number of Vh chain mutations in ${lambda}$ ⁺ GCs ofnormal mice 32. In both mIg Tg and (m+s)Ig Tg mice, the numbersof replacement mutations in ${lambda}$ CDRs are significantly higher thanwould be predicted at random, suggesting that selection of mutantsby Ag also takes place in mIg Tg GCs (Table ). We compiled alist of partial sequences showing all the V ${lambda}$ codons that containedreplacement mutations in any of the sequences from mIg Tg and(m+s)Ig Tg mice, plus those reported in NP-CGG–immunizedC57BL/6 mice (33; Fig. 9). Several mutations seen in mIg TgCDRs are also seen in (m+s)Ig Tg and normal mice. These recurrentamino acid replacements are found almost exclusively in theCDRs, again suggesting that Ag-driven selection is occurringand that it is qualitatively comparable to that in Ab-secretingmice.

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Table 1 Number of Replacement (R) and Silent (S) Mutations in V ${lambda}$ 1 Sequences from GC B Cells

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Figure 9 V ${lambda}$ 1 sequences from mIg Tg mice contain replacement (R) mutations common to (m+s)Ig Tg and nontransgenic mice. GC cells from mIg Tg and (m+s)Ig Tg mice were microdissected on day 16 after immunization with NP-CGG or NP-HSA, and V ${lambda}$ 1 sequenced. All mIg Tg and (m+s)Ig Tg V ${lambda}$ 1 codons containing replacement mutations in any of the sequences are listed, in addition to those reported in C57BL/6 mice after NP-CGG immunization by Taketani et al. (reference 50). The number of sequences represented is shown in parentheses; see Table for additional details. Shaded columns indicate codons at which mIg Tg sequences share mutations with (m+s)Ig Tg and/or published non-Tg sequences.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

These studies test several long-held ideas about the role ofpreexisting Ab and ICs in the normal development of B cell immuneresponses. By providing a scenario in which B cells exist inthe near absence of Ab, the mIg Tg mouse model allows us todistinguish between processes in which ICs actually participateand those that simply coincide with the presence of Ag on FDCs.The ability to make these distinctions without resorting togene deletions that result in pleiomorphic defects suggestsa reevaluation of some of the current concepts for the roleof FDC-bound ICs in primary B cell responses.

A 4-log reduction in specific Ab was achieved in the mIg Tgmice. Consistent with this reduction, there was no detectabledeposition (>400-fold reduction) of Ag on FDCs in vivo inmIg Tg mice. The lack of IC deposition confirmed the widelyheld concept that such deposits are Ab dependent, with the ICsbinding FcRs and CR1/2 11 on FDCs. Since Ag is deposited onFDCs as ICs, it seems likely that for most Ags the process isdependent on the classical pathway, an idea confirmed by ourfindings that observable deposition required the presence ofAb both in vivo and in vitro. In addition, immune responsesare grossly normal in Factor B–deficient mice 34, unlikethe situation for C4-deficient mice 35.

The proposed model we are testing is that the visible immunedeposits on FDCs are the limiting factor for GC development,division, maturation, and memory B cell selection. Any processfor which FDC-retained Ag is essential should display inhibitionat least proportional to the lowered Ab level. Were they notthe limiting factor, the functions attributed to these depositsin controlling the onset and size of the GC and in providinglimiting amounts of Ag to promote affinity selection would notbe possible. We have eliminated the main if not the only mechanismof IC deposition. According to the prevailing hypothesis, thisshould have resulted in a detectable decrease in some or allof these functions.

ICs were not required for a normal proliferative or GC response,since GC reactions of normal size, frequency, and kinetics wereobserved in mIg Tg mice. This is not simply an effect of highanti-NP precursor frequency, as carrier Ags alone also elicita good GC response. Thus, our data are consistent with the interpretationsof Kroese et al., who inferred that IC localization may notbe necessary for the early GC response by studying irradiatedrats, which transiently demonstrate poor IC trapping by FDCsyet initiate GC responses a few days before detectable IC localizationreturns after irradiation 13. Here we further show that IC depositionis not required for normal kinetics and size of the GC reaction,or for later events such as mutation and selection.

Recently, Ehrenstein et al. 27 concluded that natural IgM acceleratesthe primary Ab response, an interpretation based on delayedIgG production in mutant mice that lacked secreted IgM but thatcontained secreted IgG. Similarly, Boes et al. 28 inferred thatIgM-containing ICs stimulate GC reactions, since the GC responsewas moderately impaired in a similar mutant model. However,the fact that the GC response in mIg Tg mice is not diminishedcompared with (m+s)Ig Tg or CB.17 mice argues against this interpretation.The muted immune responses may reflect dominant signaling throughthe inhibitory Fc ${gamma}$ RIIB 36 in mice that contain only IgG and noIgM. No such imbalance would have existed in mIg Tg mice.

Time course analysis of the relative size and activation stateof NP-specific B cell populations revealed similar kineticsfor primary responses in mIg Tg and (m+s)Ig Tg mice. Based onin vitro data, Liu et al. suggested that B cell receptor (BCR)signaling, as a consequence of binding Ag on FDCs, rescues centrocytesfrom apoptosis 14. If such interactions were truly critical,then we should have observed massive loss of centrocytes andthus much smaller GCs. Instead, we see large GCs with normalkinetics and well-developed light zones. Therefore, althoughinteraction with Ag may well be critical for the preservationof centrocytes in the GC, the source of Ag need not be ICs boundto FDCs.

The normal kinetics of the proliferative and GC responses inmIg mice also has implications for the mechanisms for turningoff primary responses. The termination of the primary responsehas been attributed both to Ab-mediated Ag clearance and toinhibitory signals mediated by Fc ${gamma}$ R coligation with the BCR,as would occur when B cells bind IgG-containing ICs 36. Sincethe kinetics of GC appearance are normal in mIg Tg mice, otherintrinsic, non–Ab-dependent mechanisms must also be importantin dampening the immune response.

Once the GC reaction is established, GC B cells undergo somaticmutation of Ig genes 37. In the normal spleen, mutation appearsrestricted to GCs 32, although the stimulus for onset of mutationremains unclear. Direct sequencing of V ${lambda}$ genes microdissectedfrom GCs shows that mutation occurs normally in mIg Tg GC Bcells, indicating that ICs on FDCs are not responsible for theinitiation of mutation, although other signals from FDCs maystill play a role. Affinity maturation is thought to involvepreferential expansion and/or survival of those GC B cells thatacquire affinity-enhancing mutations. It is thought that higher-affinitymutants are selected by their ability to compete with Ab alreadybound to Ag on FDCs. Analysis of mutations in mIg Tg mice doesnot support this concept. The number of replacement mutationsin ${lambda}$ 1 sequences is higher than would be predicted for a nonselectedpopulation. Further, comparison of patterns of replacement mutationsin mIg Tg mice with (m+s)Ig Tg and non-Tg mice reveals mutationscommon to the three strains at several sites in CDRs. Both ofthese features indicate that Ag-driven selection is occurringin mIg Tg mice.

It is important to compare our findings with those of eitherCR1/2 knockout or TNF/TNFR family knockout mice. GCs developednormally in CR1/2^–/– mice that were provided withwild-type bone marrow, in which only the FDCs lacked CR1/2 21.However, a firm conclusion about IC localization was not drawn,since IC deposition could still occur via FcRs 11. Moreover,a second group found reduced GC formation when FDCs lacked CR1/2,suggesting a role of CR1/2 on FDCs 38. Thus, previous resultsin this area were conflicting with regard to the role of IClocalization and GC initiation. The finding in mIg Tg mice thatvigorous GC formation does occur in the absence of depositionof ICs on FDCs establishes that this event is not essentialfor GC formation.

The situation is also complex in TNF/TNFR family knockouts.Affinity maturation and somatic hypermutation have been reportedin lymphotoxin (LT)- ${alpha}$ ^–/– mice, which lack FDCs, haveabnormal splenic architecture, and do not form GCs 19. However,this response is suboptimal, requires high dose Ag or multipleimmunizations, and for some Ags such as SRBCs, IgG responsesand memory formation are dramatically reduced 16 19. A similarpicture was seen in the LT-β ^–/– mice 20. TNFR1^–/–mice can form long-lived memory cells if infected with replicatingvirus, but respond poorly and lack long-lived IgG or memoryif immunized with killed virus 17. However, given the pleiotropicdefects including lymphoid architecture disruption consequentto lack of LT- ${alpha}$ or TNFR1 expression throughout the body, it isdifficult to draw specific conclusions about the physiologicrole of IC deposition on FDCs from the LT- ${alpha}$ or TNFR1 knockouts.The lack of defects in follicular architecture and other functionsof FDCs in mIg Tg mice contrasts with the situation in LT-deficientor TNFR1^–/– mice, thus implicating disruptions inthese aspects, rather than lack of FDC-bound Ag, in the immuneresponse defects. Recent work from Chaplin and colleagues highlightsthis point, demonstrating that the normal lymphoid architectureis required to allow wild-type memory B cells to function 16.mIg Tg mice have apparently normal mutation and selection; mutationand possibly some selection were also observed in the LT-deficientmice, suggesting that GCs were not required for this function.Thus GCs, but not FDC-bound ICs, are needed for optimal mutationand selection, though the GCs are not required for some degreeof mutation.

It has been suggested that B cell CR1/2 cross-linking by C3fragments fixed on ICs was essential for B cell activation 35 39 40.If this were true, the normal activation and expansion of NP-specificB cells in mIg Tg mice would be surprising. There are at leasttwo possible explanations for this paradox: complement-complexedAg is believed to augment B cell stimulation at particularlylow doses of Ag; the dose of the Ag (50 µg) used in ourcase, though comparable to that used in the above studies, maynot have been limiting. However, even at 1/4 of this dose permouse we saw normal responses (data not shown). This suggeststhat CR1/2 must by itself be present on a responding B cellfor it to participate effectively in a GC reaction, even ifits BCR is strongly cross-linked. An additional possibilityis that mIgM that is aggregated on the cell surface by BCR ligationcan fix complement 41 42, and that C3b deposition occurs locallyat the surface of the B cell. If this were the case, then theimmune responses in mIg Tg mice suggest that such a mechanismis sufficient to drive B cell activation via CR1/2 and sIg cocross-linking.

The results reported here raise two general questions. First,if Ag bound to FDCs is not required to promote the primary GCreaction, what is the source of Ag to drive the GC response?Second, what is the function of retained Ag on FDCs if GC formation,mutation, and selection and memory B cell development can occurin its absence? As for the source of Ag, we do believe theremust be a continuous source to maintain the response. Normally,this would be in the form of a proliferating pathogen that wouldsupply a fresh source until the pathogen was eliminated. Inthe case of protein Ags, it is noteworthy that optimal immunizationrequires a depot preparation as in alum or Freund's adjuvant.These depots would release a continuous supply of Ags in a waythat simulates the pathogen situation. In either case, therewould be free Ag in the animal, which we believe is the normalsource of Ag for B cells. This should not be surprising, asfree Ag is almost certainly the source that initiates the extrafollicularas well as T cell–independent responses. An additionalinteresting possibility is marginal zone (MZ) B cells, whichhave been shown to transport Ag into follicles 13 43. However,in mIg Tg mice FDCs are not evidently receptors of Ag transportedvia MZ B cells. Perhaps Ig secretion by MZ B cells is an importantaspect of their ability to transfer ICs to FDCs. On the otherhand, MZ B cells could well serve to transport Ag directly toGC B cells in mIg Tg and possibly normal mice. Given the resultsof Kroese et al. 13, this is unlikely to be important for initiationof GCs but it could be critical for the maintenance of GCs.Indeed, MacLennan and colleagues have recently shown that therecan be a GC response that is T cell independent but not sustained,suggesting that requirements for initiation and maintenanceof GCs are likely to be different 44. Finally, we cannot formallyexclude the possibility that alterations in Ag metabolism inAb-free mice could affect Ag distribution and at least partiallycompensate for the lack of ICs bound to FDCs. However, the unalteredkinetics of the GC response in mIg Tg mice suggests that Agavailability is not markedly altered. Nor did we detect an increasein B cell–bound Ag (which was not readily observed inany situation, Fig. 5 and Fig. 8) in these mice.

Regarding the functions of FDC-bound Ag, there are several possibilities.Although it is apparent from mutation analysis that some selectiondoes occur, we have not ruled out impairment in mIg Tg mice.Long-term maintenance of memory B cells remains an additionalpossible function of retained Ag. Quantitation of memory B cellswould help resolve this, as would very long-term functionalmemory experiments. FDCs could act as an IC "sink" for the GC45. By trapping any ICs present in the GC, FDCs would reducepotential Fc ${gamma}$ R-mediated downregulation of activated GC B cells.The mIg Tg mouse is neutral in this regard, as there are noICs to be removed or to mediate downregulation. An additionalpossibility is that retained Ag could play a role in the regulationof Ab production, for example by helping to promote plasma celllongevity. Recent studies have revealed a population of long-livedplasma cells in the bone marrow and spleen that continue toundergo affinity maturation after the GC reaction has waned46 47. Addition of IgG-complexed neutralized Ag after primaryimmunization increased long-term specific Ab titers, suggestinga connection between the presence of retained Ag and continuingAb production 48. Interestingly, AFC survival in TNFR^–/–mice is much more strongly impaired than memory cell survival17. These data are also consistent with the idea that, as Ablevels wane, ICs on FDCs could dissociate, releasing some boundAg and thereby stimulating plasma cells to renew Ab production.

The FDC network is a prominent and dynamic feature of the Bcell follicle and GC. The deposition and retention of ICs onFDCs are striking and no doubt important aspects of FDC function.Our results suggest that the prevailing concepts of how ICscontribute to the development, selection, and possibly maintenanceof memory B cells should be reconsidered. More detailed evaluationwill be needed to further clarify the roles of IC capture andFDCs in general. The system we describe here, along with otherssuch as the CR1/2^–/– 21 22 and FcR^–/–49, should be instrumental in this effort.

Acknowledgments

We thank Cynthia Chi and Hong Zhou for technical assistance;Garnett Kelsoe and Joe Dal Porto for instruction on GC microdissection;and Alfred Bothwell, Michael Cancro, and Martin Weigert forcritical review of the manuscript.

This work was supported by National Institutes of Health grantAI43603 (M.J. Shlomchik). A.M. Haberman was supported by a grantfrom the Donaghue Foundation, and L.G. Hannum was supportedby National Institutes of Health Training Grant AI07019 anda Richard K. Gershon Predoctoral Fellowship.

Submitted: 25 April 2000
Revised: 14 August 2000
Accepted: 15 August 2000

L.G. Hannum's present address is University of Southern Maine/Lewiston-AuburnCollege, 51 Westminster St., Lewiston, ME 04240.

Abbreviations used in this paper: AFC, Ab-forming cell; BCR,B cell receptor; CGG, chicken gamma globulin; CR, complementreceptor; FDC, follicular dendritic cell; GC, germinal center;HSA, human serum albumin; IC, immune complex; JHD, JH knockoutstrain; LT, lymphotoxin; mIg, membrane Ig; MZ, marginal zone;PNA-HRP, peanut agglutinin–horseradish peroxidase; Tg,transgenic or transgene.

References

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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