Abstract
The contribution of three-dimensional genome organization to physiological ageing is not well known. Here we show that large-scale chromatin reorganization distinguishes young and old bone marrow progenitor (pro-) B cells. These changes result in increased interactions at the compartment level and reduced interactions within topologically associated domains (TADs). The gene encoding Ebf1, a key B cell regulator, switches from compartment A to B with age. Genetically reducing Ebf1 recapitulates some features of old pro-B cells. TADs that are most reduced with age contain genes important for B cell development, including the immunoglobulin heavy chain (Igh) locus. Weaker intra-TAD interactions at Igh correlate with altered variable (V), diversity (D) and joining (J) gene recombination. Our observations implicate three-dimensional chromatin reorganization as a major driver of pro-B cell phenotypes that impair B lymphopoiesis with age.
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Main
Structural organization of the genome provides a platform for optimal gene expression1. Chromosome conformation capture techniques have revealed several levels of organization such as multi-megabase (Mb)-sized compartments2, Mb-sized topologically associated domains (TADs)3,4 and kilobase-sized chromosomal loops5. Structural changes at each level alters gene expression associated with cellular differentiation or disease6. For example, compartment changes have been noted during embryonic stem (ES) cell differentiation in vitro7,8 and at specific stages of B lymphocyte differentiation in vivo9. TADs are largely invariant across cell types; however, subdomains within TADs vary between cell types and are associated with cell-specific gene expression5,10,11,12. Additionally, chromosomal translocations that disrupt TAD structure have been proposed to contribute to altered gene expression in cancer13.
By contrast, very little is known about chromatin reorganization during organismal ageing, especially in the immune system. Most studies utilize senescent cells generated in culture as surrogates for physiological ageing14. Senescent cells show substantial changes in chromatin structure, including de-repression of heterochromatic compartment B, regional changes from compartment B to A facilitated by loss of facultative heterochromatin, and altered chromosomal looping that activates inflammatory gene expression15,16,17,18,19,20,21,22. The extent to which chromatin features of senescent cells reflects organismal ageing remains unclear, especially because these features vary depending upon the mode of senescence induction18. In this Article, we studied age-associated chromatin structure changes at a key checkpoint during B lymphocyte development in the bone marrow.
Dysregulated immune function during ageing underlies susceptibility to infectious diseases, autoimmunity and cancers23,24,25. Aged individuals also respond poorly to immunization, thereby precluding them from the most effective intervention against microbial pathogens23,26,27,28. B and T lymphocytes, which are central for responding to infection or vaccination, are reduced with age23. For B cells, this is reflected in reduced numbers of pro-B and pre-B cells, which are developmental stages soon after commitment of multipotential precursors to the B lineage23,29,30. While ageing affects expression of several transcription factors, mechanisms that attenuate pro-B cell development in old mice have not been identified31,32,33,34. To reveal cell-intrinsic mechanisms of chromatin organization that account for changes in pro-B cells with age, we assayed chromosome conformation by Hi-C in pro-B cells obtained from young (8–12 weeks) and old (100–110 weeks) recombination activating gene 2 (Rag2)-deficient mice (Supplementary Table 1)35,36. Absence of variable (V), diversity (D) and joining (J) gene recombination in this strain (or mice lacking Rag1) blocks development at the pro-B cell stage and ensures a homogeneous cell population for epigenetic studies.
Results
Compartment changes in old pro-B cells
Pro-B cell numbers in old Rag2-deficient mice were approximately twofold lower than in young mice (Extended Data Fig. 1a–c), comparable with previously noted reductions in normal C57Bl/6J mice37. Hi-C analysis revealed that compartment level interactions (≥10 Mb) were increased in old pro-B cells whereas those associated with TADs and loops (<10 Mb) were reduced in old pro-B cells (Fig. 1a,b). More than a hundred genomic loci transitioned from euchromatic compartment A to heterochromatic compartment B and vice versa in old pro-B cells (Mahalanobis distance (MD) P < 0.01) (Fig. 1c). To probe epigenetic states that accompanied compartment changes, we carried out chromatin immunprecipitation followed by sequencing (ChIP–seq) with anti-H3K27ac and anti-H3K27me3 antibodies. H3K27ac levels were reduced in regions that switched from A to B and increased in those that changed from B to A; however, H3K27me3 levels were unaltered (Fig. 1d).
RNA-seq analysis using young and old pro-B cells showed that genes located within regions that switched from compartment B to A with age were expressed, on average, at higher levels (Fig. 1e). One such gene is Ncam1 (Extended Data Fig. 1d). Only 6 out of 310 genes annotated to compartments that changed from A to B with age were downregulated in old pro-B cells (fold change >2, P < 0.01; Supplementary Table 2), accounting for the absence of a statistically significant difference in average gene expression for A to B compartment changes in old pro-B cells (Fig. 1e).
Compartmental changes impact Ebf1
The most significant A to B transitioning genomic region contained the Ebf1 gene that encodes a transcription factor that is required for commitment of hematopoietic precursors to B lineage differentiation38. Ebf1 expression was reduced in old pro-B cells (Fig. 1f) accompanied by lower levels of H3K27ac, but unchanged H3K27me3, at the Ebf1 locus (Fig. 1f). We reasoned that age-associated defects in Ebf1 expression may underlie some aspects of impaired B cell development in aged mice. Hi-C contact maps of this region in young pro-B cells revealed multiple interactions of the Ebf1 promoter with intragenic and distal enhancers marked with H3K27ac modifications (Fig. 1g). These interactions were markedly reduced in old pro-B cells and replaced by interactions between intronic and promoter-distal CTCF-bound sites (Fig. 1g). We surmise the latter interactions reflect an ‘off’ state for Ebf1 expression. Ebf1 undergoes radial re-positioning from the nuclear periphery to a more central location concomitant with B cell commitment at the pro-B cell stage9. We found that the Ebf1 locus moved closer to the nuclear periphery in old pro-B cells (Fig. 1h,i). In contrast, the Foxo1 locus, encoding a co-regulated factor, did not change its radial position or proximity to heterochromatin-associated γ-satellite repeats in old pro-B cells (Fig. 1h and Extended Data Fig. 1e). Foxo1 compartmentalization was also unaffected by age (Extended Data Fig. 1f). Our observations reveal large-scale conformational changes in pro-B cell genomes during ageing, some of which directly impact key transcriptional regulators of B cell development.
To evaluate the contribution of Ebf1 downregulation to age-associated chromatin and gene expression changes, we first carried out Hi-C and transcriptomic analyses using Ebf1 heterozygote Rag2-deficient pro-B cells (Ebf1+/−). In these cells Ebf1 expression is reduced but not eliminated (Extended Data Fig. 2a)39,40, reflecting the state of old pro-B cells. Hi-C analysis revealed changes at compartment (≥10 Mb), TAD and loop (<10 Mb) levels (Fig. 2a). Ebf1+/− pro-B cells shared some structural features with old pro-B cells, such as reduced intra-TAD interactions, but not others such as accentuated compartments (Fig. 1a and Fig. 2a,b). We infer that, Ebf1 does not lie at the apex of chromatin reorganization in old pro-B cells. Accordingly, Ebf1 heterozygosity only recapitulated some differences noted between young and old pro-B cells. For example, the Mmrn1 gene switched from compartment A to B and its expression was reduced in old pro-B cells as well as in Ebf1+/− pro-B cells (Fig. 2c), whereas at the Minar1/Temed3 locus a new loop coincided with increased Temed3 RNA in old and Ebf1+/− pro-B cells (Fig. 2d). Contributions of such loci to the properties of old pro-B cells remain to be determined. Deleting one allele of Pax5, a B cell regulator implicated in altering chromatin structure41, in Ebf1+/− pro-B cells did not further alter the chromatin state (Extended Data Fig. 2b).
Transcriptomic analyses of Ebf1+/− pro-B cells also revealed similarities to gene expression changes in old pro-B cells (Fig. 2e). We also found that over 50% of previously identified Ebf1 target genes were altered in old pro-B cells (Supplementary Table 3)42, and several genes associated with B cell development were downregulated in both Ebf1+/− cells as well as old pro-B cells. (Fig. 2f). To evaluate the contribution of Ebf1 to gene expression changes in old pro-B cells, we re-expressed Ebf1 in young and old pro-B cells from Rag2−/− mice (Extended Data Fig. 2c,d). We found that ex vivo culture of primary pro-B cells in interleukin 7 (IL-7) required for retroviral transduction obliterated most of the differences between freshly isolated young and old pro-B cells (Extended Data Fig. 2e). However, of the 68 age-associated genes that remained differentially expressed, Ebf1 transduction restored expression of 50 (Extended Data Fig. 2f). Taken together, we conclude that reduced expression of Ebf1 associated with relocation of the locus from compartment A to B with age, induces chromatin and gene expression changes that negatively impact B cell development during ageing.
TAD alterations in old pro-B cells
We identified 2,781 TADs in young pro-B cells. By quantifying the proportion of pair-end tags (PETs) that fell within or outside TAD boundaries as a measure of TAD ‘strength’ (enrichment score; ES), we found 240 TADs with significantly lower ES (young specific) and 84 TADs with significantly higher ES (old specific) in old pro-B cells (MD P < 0.01) (Fig. 3a and Supplementary Table 4). The TAD containing the immunoglobulin heavy chain (Igh) gene locus was most reduced in old pro-B cells (Fig. 3a and Extended Data Fig. 3a). Other important B cell regulatory genes, such as Ebf1 and Pax5, were also located within reduced TADs (Fig. 3a,b and Extended Data Fig. 3a,b). The 240 young-specific TADs were associated with reduced H3K27ac within the TAD body (Fig. 3c) and less H3K27me3 at TAD boundaries in old pro-B cells (Fig. 3d). CTCF binding was unchanged; however, Rad21 levels were lower throughout bodies of young-specific TADs in old pro-B cells (Fig. 3e,f). Global reduction of Rad21 recruitment to chromatin in old pro-B cells (Fig. 3g), correlated with increased expression of Wapl, the cohesin off-loader (Fig. 3h and Extended Data Fig. 3c). Increased Wapl expression in old pro-B cells was independent of Ebf1 dysregulation since no changes were evident in Ebf1+/− pro-B cells (Extended Data Fig. 3d). Several genes associated with B cell development, including Ebf1, Pax5, Bach2 and Bcl11a, that were located within reduced TADs were expressed at lower levels (Fig. 3h and Extended Data Fig. 3c), although average gene expression was unchanged (Fig. 3i).
We tested the effects of changing Wapl levels in a recombinase deficient pro-B cell line (Extended Data Fig. 4a,b). Twofold higher Wapl expression resulted in lower genomic contacts in the 50–300-kb range, typical of intra-TAD interactions (Extended Data Fig. 4c). A total of 341 TADs were significantly reduced, including the TAD encompassing the Igh locus (Extended Data Fig. 4d,e). RNA-seq from control and Wapl-overexpressing cells showed that differential gene expression patterns were similar to those seen by reducing Ebf1 levels or in old pro-B cells (Extended Data Fig. 4f). We conclude that altered levels of Wapl induce TAD changes during ageing that impair multiple aspects of pro-B cell differentiation and function.
Reduced levels of H3K27ac within young-specific TADs prompted us to probe H3K27ac dynamics more deeply during ageing. We observed reduced H3K27ac (young selective) at over 10,000 sites genome wide in old pro-B cells. The majority (78%) were annotated as enhancers (Fig. 4a). Conversely, approximately 1,200 sites gained H3K27ac in old pro-B cells (Fig. 4a). Total H3K27ac levels were comparable in young and old pro-B cells (Extended Data Fig. 5a). Young- or old-selective H3K27ac peaks mapped to largely unique sets of genes (Fig. 4b) with opposite expression patterns (Fig. 4c). Examples of genes with young- and old-selective H3K27ac peaks are shown in Fig. 4d. p300, the enzyme that acetylates H3K27ac, had altered recruitment genome-wide in old pro-B cells (Extended Data Fig. 5b), with majority of sites that lost p300 coinciding with sites of reduced H3K27ac in old pro-B cells (Extended Data Fig. 5c). By contrast, recruitment of the chromatin remodeller, Brg1, was very similar in young and old pro-B cells (Extended Data Fig. 5d).
We carried out anti-H3K27ac HiChIP in young and old bone marrow pro-B cells to probe chromatin looping. Interactions involving young- or old-selective H3K27ac sites were on average reduced or increased, respectively, in old pro-B cells compared with interactions of H3K27ac sites that did not change with age (Fig. 4e). This trend was maintained after segregating enhancer- or promoter-associated differential H3K27ac sites (Fig. 4f,g). Enhancer–promoter interactions in several genes critical for B cell development were affected with age (Fig. 4h and Extended Data Fig. 5e).
Reduced Igh TAD strength
The most reduced TAD in old pro-B cells encompassed the 3 Mb Igh locus (Fig. 5a,b). Two prominent age-associated differences were obvious at the Igh locus. First, a ‘stripe’ that extends throughout the TAD was reduced in old pro-B cells (Fig. 5c). Location of this stripe coincides with a cluster of CTCF-bound sites (3′ CTCF-binding elements; 3′ CBEs in Fig. 5d) that have been proposed to mark the 3′ end of the Igh locus43,44. Second, sub-TADs within the Igh TAD were reduced in old pro-B cells (Fig. 5c). We have previously proposed that such sub-TADs represent one level of compaction of the part of the locus that encodes variable (VH) gene segments and facilitates VDJ recombination of distally located gene segments45,46. H3K27ac and Rad21 levels were lower throughout the 2.5 Mb VH region (Fig. 5d,e) in old pro-B cells, as was the prominent H3K27ac peak corresponding to the Eμ enhancer (Fig. 5d). By contrast, CTCF binding through the VH region, at intergenic control region 1 (IGCR1)47 and at the 3′ CBEs43 was minimally affected by age (Fig. 5d,e). We also found that a patch of H3K27me3 corresponding to the 3′ VH gene segments was lower in old pro-B cells (Fig. 5d,e). Fluorescence in situ hybridization (FISH) analysis provided independent evidence for reduced sub-TAD formation in old pro-B cells (Fig. 5f,g). We conclude that widespread loss of H3K27ac and Rad21 and reduced interactions mark the Igh TAD in old pro-B cells.
To more deeply probe the interactions within the Igh TAD, we carried out capture Hi-C using young and old pro-B cells (Supplementary Table 5). Consistent with whole-genome Hi-C, we found that intra-TAD interactions, as well as interaction of the 3′ Igh domain with the rest of the locus, were reduced in old pro-B cells (Fig. 6a). Virtual 4C representation of the Hi-C data showed that interactions of distal regions with the 3′ end of the locus were most prominently reduced in old pro-B (Fig. 6b). To investigate the impact of Ebf1 downregulation on Igh structure, we carried out Hi-C analysis of Ebf1+/− pro-B cells (Fig. 6c). Virtual 4C showed 3′ CBEs contact till the middle of the VH region in Ebf1+/+, probably due to their proliferative phenotype48. These contacts were further reduced in Ebf1+/− cells whereas interactions with Eμ and IGCR1 were unaffected (Fig. 6c,d). We conclude that interactions between the 5′ and 3′ ends of the Igh locus are reduced in old pro-B cells, in part mediated by reduced Ebf1 expression with age.
To identify functional consequences of altered chromatin interactions with age, we quantified VH rearrangements in purified pro-B cells from young and old C57BL/6J mice49,50. We scored VDJ and DJ junctions in two replicate experiments, each carried out with pro-B cells pooled from four to six mice. We found that the most proximal VH gene segments were over-represented and the most distal ones were under-represented in old pro-B cells (Fig. 6e,f). DH gene segment utilization was minimally affected in old pro-B cells (Extended Data Fig. 6a). The proportion of VDJ compared to DJ recombined alleles (Fig. 6g) and levels of productive VDJ junctions were reduced in old pro-B cells (Fig. 6h). Though total number of CDR3 regions were reduced in old pro-B cells, CDR3 length distribution was not altered with age (Extended Data Fig. 6b,c). We propose that the predominant effect of age on distal VH gene segment usage and recombination frequency results from reduced interactions between 5′ and 3′ ends of the Igh locus in old pro-B cells. Because ageing does not affect chromatin topology of the 3′ Igh domain, within which DH rearrangements occur, DH usage and frequency are less affected by age.
Discussion
Our studies reveal large-scale age-associated chromatin reorganization at a critical juncture of B cell development. These include increased interactions at the compartment level, transitions between compartments and substantially reduced TAD interactions that are accompanied by altered histone modifications and gene expression. The trends we observed during physiological ageing were quantitatively similar to chromatin changes noted for other biological processes, such as ES cell differentiation in vitro7. However, each chromatin feature identified here was shared with only a subset of studies of cellular senescence18 and recent investigations into age-associated chromatin reorganization51,52,53,54. Our observations highlight the unique chromatin state of old pro-B cells, mechanisms by which it is generated and its functional consequences.
Chromatin structure changes in aged pro-B cells identified here were more extensive than those previously reported for pre-B cells37. One possibility is that only a small proportion of pro-B cells in old mice that lack the perturbations reported here, differentiate into pre-B cells. These pre-B cells may therefore reflect the epigenetic state of the ‘young-like’ precursor pro-B cells. Alternatively, pre-B cells that develop in old mice may acquire a more youthful chromatin state during the transition. Our observations identify the pro-B cell stage as a selective target of epigenetic alterations that negatively impact B cell development during ageing.
Changes stemming from Ebf1 re-compartmentalization, radial positioning and downregulation of expression impact two key features of old pro-B cells. First, expression of B lineage affirming transcription factors (E2A, Ebf1, Pax5 and Bcl11a) and suppressors of other lineages (Bach2) is reduced, resulting in a gene expression profile that skews towards myeloid and erythroid differentiation55,56,57,58,59. This may explain, in part, myeloid skewing of hematopoietic stem cells during ageing60 and for the previously noted retardation of pro- to pre-B cell differentiation in young Ebf1+/− mice39. Our observations with genetically reduced Ebf1 expression suggest that chromatin structural changes drive Ebf1 dysregulation and its downstream consequences during ageing.
Second, immunoglobulin gene assembly and expression of IgH protein in pro-B cells is a key checkpoint during B cell development55,61. Pro-B cells that fail to express IgH do not differentiate further and are lost by apoptosis. We found that changes in Igh locus structure in old pro-B cells negatively impact this checkpoint by reducing diversity and efficiency of variable (VH) gene segment recombination. Several of these features were recapitulated in Ebf1+/− pro-B cells, indicating that they resulted from reduced Ebf1 expression in old pro-B cells.
Global weakening of TADs in old pro-B cells was accompanied by reduced genome-wide recruitment of Rad21 and loss of promoter/enhancer interactions. Reduced TADs and increased compartments, as observed in old pro-B cells, were previously noted in cell lines depleted of Rad21 or CTCF62,63. Although both these genes were comparably expressed in young and old pro-B cells, Rad21-binding levels were lower in old pro-B cells and may contribute to loss of TAD strength. We also found increased expression of Wapl, the cohesin off-loader, in old pro-B cells64,65. This may be the result of reduced Pax5 expression, a proposed repressor of Wapl, in old pro-B cells41. De-repression of Wapl by genetic manipulation has been previously shown to adversely affect TADs in pro-B cells, similar to our observation in old pro-B cells41,48. Because ectopic expression of Wapl in pro-B cells recapitulated several features of ageing, we hypothesize that increased Wapl and reduced Rad21 binding during physiologic ageing of B lymphocyte progenitors reduces TAD strength via increased disruption of cohesin-dependent chromatin loop extrusion. Age-associated epigenetic dysregulation of B cell development identified here may impact antibody-dependent immunity in older individuals.
Methods
This study is compliant with all the relevant ethical regulations. All mouse experiments were performed under protocols approved by National Institute on Aging (NIA) Institutional Animal Care and Use Committees (338-LMBI-2022).
Mice
Young (8–12 weeks) recombination activating gene 2-deficient (Rag2−/−) mice35,36 were purchased from Jackson Lab (stock no. 008449) and maintained to be old (100–110 weeks) in house by NIA Comparative Medicine Section. Young (8–12 weeks) and old (100–110 weeks) C57BL/6J mice were provided by the NIA Aged Rodent Colonies. The mice used in the experiments comprised both males and females, and for each experiment, the sexes of both young and old mice were matched. In each experiment, two to six mice were pooled on the basis of the required cell count and the actual number of cells obtained.
Mouse husbandry was conducted under standard circadian rhythms of 12 h of darkness followed by 12 h of light, at a constant temperature of 22 ± 2 °C and humidity ranging between 45% and 70%.
Cell lines
Rag2−/−Ebf1+/+Pax5+/+, Rag2−/−Ebf1+/−Pax5+/+ and Rag2−/−Ebf1+/−Pax5+/− pro-B cells are cultured as previous described40.
The wild-type D345 cell line was generously provided by David G. Schatz of Yale University. These cells were maintained in RPMI1640 (Gibco) supplemented with 10% foetal bovine serum (FBS, Gemini) and a 1× penicillin–streptomycin solution (Gibco).
293T human embryonic kidney cells used for lentiviral expression was purchased from ATCC (cat. no. CRL-3216) and cultured in Dulbecco’s modified Eagle medium (Gibco) with 10% FBS (Gemini) and 1× penicillin–streptomycin solution (Gibco).
The Platinum-E (Plat-E) cell line used for retroviral expression was purchased from Cell Biolabs (cat. no. RV-101) and cultured in Dulbecco’s modified Eagle medium (Gibco) with 10% FBS (Gemini), 1× penicillin–streptomycin solution (Gibco), 10 mM HEPES and 0.3 μg ml−1 l-glutamine. All cells were cultured at 37 °C in a humidified atmosphere with 5% CO2.
Antibodies
Flow cytometry
Phycoerythrin (PE) anti-CD19 (BioLegend, 6D5, cat. no. 115508, 1:100), Brilliant Violet 421 (BV421) anti-B220 (BioLegend, RA3-6B2, cat. no. 103240, 1:100), fluorescein isothiocyanate (FITC) anti-IgM (BioLegend, RMM-1, cat. no. 406506; 1:50), PE anti-CD43 (BD Biosciences, S7, cat. no. 553271, 1:100), H3K27ac-AF488 conjugated (Cell Signaling Technology, cat. no. 15485S. 1:50) and IgG isotype control-AF488 conjugated (Cell Signaling Technology, cat. no. 4340S; 1:50) were used.
ChIP–seq and HiChIP
Anti-H3K27ac (Active Motif, cat. no. 39133; 1:500), anti-H3K27me3 (Diagonode, cat. no. C15410195; 1:500), anti-CTCF (Abcam, cat. no. ab70303; 1:250), anti-Rad21 (Abcam, cat. no. ab992; 1:500), anti-Brg1 (Abcam, cat. no. ab110641; 1:200) and anti-p300 (Cell Signaling Technology, cat. no. 57625S; 1:333) were used.
Pro-B cell purification
For Rag2−/− mice, total bone marrow was extracted from tibia and femurs, and erythrocytes were lysed. Pro-B cells were purified by combining positive selection using CD19+ selective beads (Stem Cell Technology, cat. no. 18954) and sorting by CD19+ and B220+ markers.
For C57BL/6J mice, total bone marrow was extracted from tibia and femurs, and erythrocytes were lysed. Cells were pre-purified using CD19+ selective beads (Stem Cell Technology, cat. no. 18954) and sorted with IgM−B220+CD43+ markers. Flow cytometry experiments were performed on BD FACSAria II Cell Sorter. FlowJo software was used for data analysis.
In situ Hi-C
Genome-wide in situ Hi-C was performed with Rag2−/− young and old primary pro-B cells, and Rag2−/−Ebf1+/+Pax5+/+, Rag2−/−Ebf1+/−Pax5+/+, Rag2−/−Ebf1+/−Pax5+/−, D345-BFP control and D345-Wapl-BFP pro-B cell lines, using the Arima Hi-C Kit (Arima Genomics), including KAPA Hyper Prep indexing and library amplification (cat. no. KK8500, Roche Molecular Systems Inc) according to the manufacturer’s instructions. For each assay, 1 × 106 cells were used as the input materials and two biological replicates were performed for each group. Samples were sequenced 2 × 150 bp on an Illumina NovaSeq instrument at the Single Cell and Transcriptomics Core at Johns Hopkins University.
RNA-seq
Total RNA was prepared using the Direct-zol RNA Miniprep Kit (Zymo Research, cat. no. R2051) according to manufacturer’s instructions. The RNA libraries for young and old Rag2−/− primary pro-B cells (four biological replicates for each group) were prepared using the NEXTFLEX Rapid Directional RNA-Seq Kit (PerkinElmer, cat. no. NOVA-5138-07) and sequenced 2 × 75 bp on an Illumina NovaSeq instrument at the Single Cell and Transcriptomics Core at Johns Hopkins University.
RNA libraries for Rag2−/−Ebf1+/+Pax5+/+, Rag2−/−Ebf1+/−Pax5+/+, Rag2−/−Ebf1+/−Pax5+/− and D345-BFP control and D345-Wapl-BFP pro-B cell lines (two replicates for each group) were prepared using SMARTer Stranded Total RNASeq Kit v2 (Takara, cat. no. 634412) and sequenced 1 × 100 bp on an Illumina NovaSeq instrument at the Single Cell and Transcriptomics Core at Johns Hopkins University.
RNA libraries for pro-B cells infected with Ebf1-GFP or GFP-containing retrovirus were prepared using the SMART-Seq mRNA kit (Takara, cat. no. 634773) and sequenced 2 × 100 bp on an Illumina NovaSeq instrument at the Computational Biology and Genomics Core in NIA.
ChIP–seq
For the ChIP of histone modifications, CTCF and Rad21, both young and old primary Rag2−/− pro-B cells underwent crosslinking with 1% formaldehyde (Sigma) for 10 min at room temperature. The reaction was subsequently quenched with 125 mM glycine, and cell lysis was initiated in a buffer containing 1% sodium dodecyl sulfate. Chromatin was then sheared using a Bioruptor (Diagenode) in cycles of 30 s on and 30 s off, totalling 15 min of shearing time. Immunoprecipitation was performed using specific antibodies, with 1 × 106 cells used for each assay, and antibody dilutions followed established protocols.
As for Brg1 and p300 ChIPs, we followed the protocol by Bossen et al.66, with some modifications. In this case, two million young and old primary Rag2−/− pro-B cells were first crosslinked with 1.5 mM ethylene glycol bis(succinimidyl succinate) at room temperature with rotation for 15 min. Subsequently, the cells were fixed with 1% formaldehyde (Sigma) for 15 min at room temperature with rotation and quenched with 200 mM glycine. After two phosphate-buffered saline (PBS) washes, the cells were lysed in a buffer containing 1% sodium dodecyl sulfate. Notably, we extended the sonication time to a total of 20 min of shearing time, while the subsequent steps of the protocol mirrored the previously mentioned procedure.
RT–PCR
Total RNA was isolated as previously described. A total of 100 ng of RNA was used to generate complementary DNA (cDNA) with SuperScript III (Thermo Fisher Scientific, cat. no. 18080051) using random hexamers according to the manufacturer’s protocol. Quantitative polymerase chain reaction (RT–PCR) was performed with iTaq Universal SYBR (Bio-Rad, cat. no. 1725125) using primers described in Supplementary Table 6. Three independent experiments were carried out. Cobp2 was used as a control37. Data were processed by the delta–delta CT method.
FISH
FISH was performed as previously described45,46. Briefly, cells were fixed on poly-l-lysine coated slides using 1.5 × 106 cells per slide. Slides were kept for 15 min at 37 °C, followed by fixation with 4% paraformaldehyde in PBS. Cells were further washed with 0.1 M Tris–HCl (pH 7.4), followed by PBS. Fixed cells were treated with 100 μg ml−1 RNase A in PBS, permeabilized using 0.5% saponin/0.5% Triton X-100/PBS for 30 min at room temperature. Probes were listed in Supplementary Table 6.
Labelled probes were denatured at 75 °C for 5 min and applied to cells that were denatured in formamide at 73 °C, followed by incubation in a dark humid chamber. Images were acquired using a Nikon Eclipse Ti2 microscope equipped with a 60× lens. Depending on the size of the nucleus, 40–50 serial optical sections spaced by 0.2 μm were acquired. The datasets were deconvolved using NIS-Elements software (Nikon). For RI, RII and RIII spatial distance measurements, we calculated the centre-to-centre distances between the parent and child, specifically focusing on the child’s nearest parent. To measure the distances between the nuclear periphery and the centres of Foxo1 or Ebf1 probes67, we used DAPI as the reference point. The nuclei of individual cells were delineated through DAPI staining, and the measurements were based on the child (Foxo1 or Ebf1 probes) intersecting with the parent (DAPI-stained nuclei). For the distances between Foxo1 and γ-satellite signals, we measured the centre-to-centre distances between the parent and child, focusing on the child’s nearest parent. We selected the minimum distances for each parent since γ-satellite has multiple signals. While each parent can have more children, each child has only one parent for Nikon measurements.
Retroviral expression of Ebf1
Retrovirus was produced by transfection of Plat-E cells with retroviral plasmids containing Ebf1 cDNA and a selective green fluorescent protein (GFP) marker (pMYs-Ebf1-IRES-EGFP)42, or with GFP-only plasmids as the control (pMSCV-IRES-GFP, Addgene cat. no. 20672). Supernatants were collected at both 48 and 72 h post-transfection and subsequently concentrated using the Retro-X Concentrator (Takara, cat. no. 631456), following the manufacturer’s instructions. Young and old Rag2−/− CD19+ cells were cultured with 2 ng ml−1 of IL-7 for three days and then exposed to the resuspended virus with the supplement of 10 μg ml−1 polybrene. The cells were cultured for an additional 72 h and subsequently sorted on the basis of GFP expression before subsequent analysis.
Lentiviral expression of Wapl
Lentivirus was produced by transfection of 293T cells with the pHIV-Wapl-IRES-BFP and pHIV-IRES-BFP plasmids. To make these plasmids, the BFP DNA fragment was amplified from plasmid pEJS614_pTetR-P2A-BFPnls/sgNS (Addgene, cat. no. 108650), and then integrated into pHIV-IRES-Zsgreen (Addgene, cat. no. 18121) using the NEBuilder HiFi DNA Assembly Master Mix (New England Biolabs, cat. no. E2621S) as per the manufacturer’s instructions, resulting in the generation of pHIV-IRES-BFP plasmids. Subsequently, Wapl cDNA was introduced into pHIV-IRES-BFP, creating the pHIV-Wapl-IRES-BFP. Supernatants were collected at both 48 and 72 h post-transfection and subsequently concentrated using the Lenti-X Concentrator (Takara, cat. no. 631232). D345 cells were infected with the resuspended lentivirus with the addition of 8 μg ml−1 polybrene. After infection, the cells were cultured for 72 h and sorted on the basis of BFP expression. The sorted cells were then cultured for 2–3 additional days to obtain an increased number of BFP-positive cells for experimental purpose.
H3K27ac HiChIP
The H3K27ac HiChIP procedure was executed employing the Arima Hi-C+ Kit (Arima Genetics Inc. cat. no. A101020), strictly adhering to the manufacturer’s guidelines outlined in the Arima-HiC+ documents A160168 v00 (HiChIP) and A160169 v00 (library preparation). In each sample, a total of 5 × 106 cells were utilized. These libraries were individually barcoded and then combined for sequencing on an Illumina NovaSeq instrument.
Intracellular staining of H3K27ac
Total bone marrow cells were obtained from young and old Rag2−/− mice to evaluate H3K27ac levels through intracellular staining. Cell surface markers were stained with PE anti-CD19 and BV421 anti-B220, washed twice with PBS and then stained in PBS with the eBioscience Fixable Viability Dye eFluor 780 (Invitrogen, cat. no. 65-0865-14). Following this, cells were washed with PBS and fixed and permeabilized using the Fix/Perm buffer provided by the Transcription Factor Buffer Set (BD, cat. no. 562725) according to the manufacturer’s instructions. Fixed and permeabilized cells were then washed twice with the Perm/Wash buffer form the Transcription Factor Buffer Set and stained with either anti-H3K27ac or IgG isotype control antibodies. Subsequently, the cells were washed three times with Perm/Wash buffer before being subjected to flow cytometry analysis for H3K27ac quantification.
Capture Hi-C
Whole-genome Hi-C libraries were first generated as previously described. To enrich the Igh locus (mm10, chr12: 113,201,001–116,030,000), SureSelect Target Enrichment probes (Supplementary Table 5) with 2× tiling density were designed and manufactured by Agilent (Agilent Technologies, Inc.). Hi-C libraries were hybridized to probes as specified by the manufacturer. Enriched libraries were sequenced using Illumina NextSeq sequencer to generate 2× 150 bp reads.
VDJ-seq
VDJ-seq was performed following the HTGTS-Rep-Seq protocol49,50. Briefly, 200 ng to 2 μg of genomic DNA isolated from primary pro-B cells sorted from young and old C57BL/6J mice was sonicated with Covaris using the setting of Durations 10 s, Peak power 50, Duty Factor 20%, Cycles/Burst 200. Sheared DNA was linearly amplified using a biotinylated JH1 primer and enriched with streptavidin C1 beads (Thermo Fisher Scientific). A bridge adaptor was ligated to enriched single stranded DNA to the 3′ end and then amplified by a nested primer set. Products were further amplified using P5–I5 and P7–I7 primers to be final libraries and sequenced by Illumina MiSeq sequencer to generate paired-end 250 bp reads. Primers or oligos used are listed in Supplementary Table 6.
Sequencing data bioinformatics analysis
For all analyses, we utilized the mouse reference genome mm10 and annotations from GENCODE (M21)68. The RNA-seq data and ChIP–seq data generated in this study were pre-processed from raw reads to expression level, differentially expressed genes analysis, mapped reads or tracks (bigWig files) following the procedures outlined in our previous studies69,70.
This manuscript incorporates heatmaps generated from pooled and down-sampled reads, ensuring equal representation from Hi-C or HiChIP data. Related statistical tests were performed with function in Python SciPy71 package. If not specially mentioned, most plots were generated by the matplotlib72 and seaborn73.
RNA-seq analysis
RNA-seq raw reads of young and old Rag2−/− primary pro-B cells were trimmed and mapped to the mouse reference genome (mm10) using STAR (v2.7.3a)74 and calculated the raw count using featureCounts package (gene-level) and fragments per kilobase of transcript per million mapped reads (or transcript per million) using RSEM package75.
For the rest of those RNA-seq experiments, raw reads were trimmed and mapped to mm10 by STAR (v2.7.3a)74 and quantified into reads per kilobase per million mapped reads with Cufflinks (v2.2.1)76. Bigwig tracks were also generated by STAR as signal quantified as reads per kilobase per million mapped reads. RNA-seq tracks were shown by IGV77.
ChIP–seq analysis
ChIP–seq raw reads were mapped to the mouse reference genome mm10 by Bowtie2 (v2.3.5)78. Only non-redundant reads with mapping quality score ≥10 were saved as BED files for the following analysis. Bigwig tracks were generated by bamCoverage in deepTools (v3.3.0)79 with parameters of --ignoreDuplicates --minMappingQuality 10 --normalizeUsing CPM for visualization and quantification aggregation analysis. Visualization of ChIP–seq tracks were performed by IGV77 or the cLoops2 plot module (v0.0.2)80. ChIP–seq peaks were identified using the cLoops2 callPeaks module. For H3K27me3, CTCF, Rad21, Brg1 and p300 ChIPs, the key parameters -eps 150 and -minPts 20,50 were employed. For H3K27ac data, the parameters -eps 150,300, -minPts 20,50 and -sen were used. Peak identification was performed on each replicate individually, followed by the compilation of a union set encompassing both conditions (young and old) and overlapping replicates. Differential peaks were identified for young and old conditions using a Poisson test. The test utilized average counts from replicates for each peak and considered normalized total reads of 30 million. A P value cut-off of <1 × 10−5 and a fold change cut-off of ≥2 were used to identify significant differential peaks. ChIP–seq peak or domain regions aggregation analyses, including heatmaps and average profile plots, were generated using the computeMatrix and plotHeatmap commands from the deepTools (v3.3.0) package. Quantification of ChIP–seq signals in Hi-C compartments was performed by the cLoops2 quant module. H3K27ac peak annotations were performed by the anoPeaks.py script in cLoops2 package, which is available at https://github.com/YaqiangCao/cLoops2/blob/master/scripts/anoPeaks.py. H3K27ac peaks within a 2-kb range upstream or downstream of the transcription start site (TSS) are annotated as promoters, while those outside this range are labelled as enhancers for the downstream analysis.
Hi-C, H3K27ac HiChIP and capture Hi-C analysis
Hi-C, H3K27ac HiChIP and capture Hi-C raw reads were processed to the mouse reference genome mm10 by HiCUP (v0.7.2)81 with the settings of Arima. High-quality and unique paired-end tags (PETs) from HiCUP were further processed to the HIC file through Juicer (v1.6.0)82 for visualization with Juicebox83. These PETs were also processed with cLoops2 (v0.0.2)80 for quantifications. Chromosome X was excluded from the analysis. Replicates from H3K27ac HiChIP samples were combined and down-sampled equally to 39 million PETs for all following analysis.
Hi-C compartment analysis of eigenvectors first principal component (PC1) was obtained by hicPCA in HiCExplorer3 package (v3.6)84 with parameters of -noe 1 at the resolution of 100 kb. We employed a two-pass Mahalanobis distance (MD) calculation, an effective method for outlier detection based on data point distribution, along with a chi-squared test for Hi-C compartment PC1 at the 100-kb bin level to detect PC1 sign flip bins. This approach aligns with the strategy employed in the recent study dcHiC85. The MD is calculated as \({\rm{MD}}={\rm{diag}}((X-{X}_{c})\times {C}^{-1}\times {\left(X-{X}_{c}\right)}^{T})\), where X is the matrix for PC1 obtained from the Hi-C compartment analysis. Each row represents a bin, and each column represents a sample (young or old). C−1 is the inverse covariance matrix of X, Xc is vector of row-wise mean of X and diag is the function used to extract a diagonal array from a matrix. We performed the chi-squared test with the MD, and a P value cut-off of 0.01 was set as the significance cut-off for detecting outliers. For the first pass calculation of MD, outliers were detected with all bins. For the second pass calculation, outliers were removed for calculation Xc and C−1. Then, MD distances were calculated for all bins on the basis of the first pass-outlier removed Xc and C−1. The code for the analysis to generate the MD distances and P values, the plot, significant changed bins and associated genes is implemented as the comparComp.py script in the cLoops2 package and is available at https://github.com/YaqiangCao/cLoops2/blob/master/scripts/compareComp.py.
Hi-C TADs were called by Juicer arrowhead with parameters of -r 25000 -k KR. We employed ESs to quantify TAD interaction strength. The ES is calculated by dividing the number of PETs interacting exclusively within a TAD by the number of PETs with one end within the TAD. Like the comparison of compartments, we implemented the two-passes MD calculation and chi-squared test to get the significant changed TADs. The MD is calculated as \({\rm{MD}}={\rm{diag}}((X-{X}_{c})\times {C}^{-1}\times {\left(X-{X}_{c}\right)}^{T})\), where X is the matrix for TAD ESs. Each row represents a TAD, and each column represents a sample (young or old). C−1 is the inverse covariance matrix of X, Xc is vector of row-wise mean of X, and diag is the function used to etract a diagonal array from a matrix. We performed the chi-squared test with the MD, and a P value cut-off of 0.01 was set as the significance cut-off for detecting outliers. For the first pass caculation of MD, outliers were detected with all TADs. For the second pass caculation, outliers were removed for calculation Xc and C−1. Then, MDs were caculated for all bins based on the first pass-outlier removed Xc and C−1. The TAD ES was calculated by dividing the number of intra PETs (PETs with both ends located in the TAD) by the number of inter PETs (PETs with only one end located in the TAD). We used the ES as a metric because we found that the IgH domain had the highest change, along with domains contain Ebf1 and Pax5 in the top. The code for the analysis to generate the MD distances and P values for the TADs, the plot, significantly changed TADs and associated genes is implemented as the compareDom.py script in the cLoops2 package and is available at https://github.com/YaqiangCao/cLoops2/blob/master/scripts/compareDom.py.
H3K27ac HiChIP data viewpoints analysis was used to examine the changes in interactions for H3K27ac ChIP–seq peaks. For each viewpoint (H3K27ac peak), an ES was calculated using the H3K27ac HiChIP contact matrix at a 1-kb resolution. The ES was centred on the peak and incorporated 100-kb upstream and downstream regions as the background. A higher ES indicates stronger interactions originating from the viewpoint. To visually emphasize the signals, the upper right corner matrices of the ±100-kb contact matrices centred around each viewpoint (H3K27ac peak) were subjected to two rounds of log10 transformation and presented as heatmaps. cLoops2 plot module was utilized to generate visualizations of HiChIP data, including one-dimensional signal profiles, ChIP–seq tracks, arches depicting the number of PETs for combinations of H3K27ac peaks and heatmaps or scatter plots.
Virtual 4C analysis
Virtual 4C analysis was performed using Cooler2 to extract all contacts involving the 3′ CBE from the Hi-C contact maps86. The bin size used for this analysis was 5,000 bp and ‘VC_SQRT’ was used as the Hi-C normalization method. The bin used for the 3′ CBE bait was chr12:113220000-113225000 (mm10).
VDJ-seq analysis
VDJ-seq analysis was performed using HTGTS-Rep49,50. This computational pipeline determined the frequency of V and D gene usage for each HTGTS experiment. This pipeline was also used to determine the distribution of CDR3 lengths and the percent of productive versus non-productive recombination events.
Statistics and reproducibility
The presentation of data and the statistical tests utilized are detailed in each figure legend. For datasets with a sample size (n) less than three, individual data points are displayed, assuming a normal data distribution, but this was not formally tested. Unless otherwise specified, the statistical tests were performed using GraphPad Prism v.9.5.0. For Fig. 4f, all P values were reported as 0.000000 by scipy.stats.wilcoxon. No statistical method was used to predetermine sample size, but our sample sizes are similar to those reported in previous publications54. No data were excluded from the analysis. All biologically independent replicates are explicitly identified in the figure legends. The gating strategy of flow cytometry is shown in Supplementary Fig. 1. Fluorescence-activated cell sorting data and microscopy (FISH) images are representative of at least three independent biological replicates. Experiments were not randomized, and data collection and analysis were not performed blind to experimental conditions.
Reporting summary
Further information on research design is available in the Nature Portfolio Reporting Summary linked to this article.
Data availability
All sequencing data generated in this study, including RNA-seq, ChIP–seq, Hi-C, capture Hi-C, VDJ-seq and HiChIP data, have been deposited in the Gene Expression Omnibus (GEO) under accession codes GSE214438. Source data are provided with this paper.
Code availability
Hi-C compartment and domain comparison script comparComp.py and comparDom.py are integrated into the cLoops2 package and available via GitHub at https://github.com/YaqiangCao/cLoops2/blob/master/scripts/compareComp.py and https://github.com/YaqiangCao/cLoops2/blob/master/scripts/compareDom.py. The script used to show Fig. 4e is available via GitHub at https://github.com/YaqiangCao/cLoops2/blob/master/scripts/showAggVPs.py.
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Acknowledgements
This research was supported by the Intramural Research Program of the National Institute on Aging (R.S. and I.B.) and National Heart, Lung, and Blood Institute (K.Z.), as well as Max Planck for Immunobiology and Epigenetics (R.G.). Data analysis of this work utilized the computational resources of the NIH HPC Biowulf cluster (http://hpc.nih.gov). Special thanks to C. Dunn at the NIA Flow Core for assistance with FACS sorting, J. Fan and S. De at the NIA Computational Biology and Genomics Core, C. Sherman-Baust in the Laboratory of Molecular Biology and Immunology (LMBI) at NIA, and L. Orzolek at the Transcriptomics and Deep Sequencing Core in Johns Hopkins Medicine for their support with Illumina sequencing. Thanks to A. Lenaerts and H.-J. Schwarz at the Max Planck Institute for their assistance in preparing the pMYs-Ebf1-IRES-EGFP plasmid. We also appreciate the contributions of M. Kaileh in LMBI and the Comparative Medicine Section at NIA for animal care, A. Singh for insightful input on B cell development and C. Sasaki for assistance with ChIP–seq quality checks.
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Conceptualization was carried by F.M., Y.C. and R.S. Methodology was created by F.M., Y.C., F.Z.B., M.B. and H.D. Investigation was performed by F.M., F.Z.B., M.B., H.D., L.Z., R.R., S.N., X.Q. and A.H.B. Data analysis and visualization were performed by F.M., Y.C., N.O., B.P., R.R., D.S., A.Z. and A.H.B. Funding acquisition, project administration and supervision were carried out by I.B., K.Z., R.G. and R.S. Writing of the original draft was carried out by F.M., Y.C., N.O., H.D., B.P. and R.S. Writing—review and editing of the text—was performed by F.M., Y.C., F.Z.B., N.O., L.Z., R.R., I.B., K.Z., R.G. and R.S.
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Extended data
Extended Data Fig. 1 Pro-B cell number is reduced in aged mice.
(a) Representative flow cytometry plots showing the population of Rag2−/− pro-B cells from young and old bone marrow. Numbers indicate percentage of cells in the gates. Gating strategy was shown in Source Data. (b) Average total number of bone marrow cells from tibias and femurs of young and old Rag2−/− mice (n = 8). Data are presented as mean ± SEM. Unpaired two-sided t test was used, with P-values indicated. (c) Number of pro-B cells after CD19+ selection and CD19 + B220+ sorting from young and old Rag2−/− mice (n = 9). Each point represents an individual mouse. Data are presented as mean ± SEM. Unpaired two-sided t test was used, with P-values indicated. (d) An example locus transitioned from compartment B (young) to compartment A (old) with age. Top tracks show Hi-C PC1 of a segment of chromosome 9 that contains Ncam1 in pro-B cells at different ages; the region corresponding to the Ncam1 locus is expanded below. Normalized tracks for H3K27ac and H3K27me3 ChIP-Seq and RNA-Seq across the Ncam1 locus are shown with IGV. Arhgap20 (right) serves as a control gene located in compartment B that is unaffected by age. (e) Dot plots for distance between Foxo1 locus to the nuclear periphery (upper panel) or to the nearest γ-satellite signal (bottom panel). Median is shown in red line. N = 100. Unpaired two-sided t test was used, with P-values indicated. (f) Hi-C PC1 showing a segment of chromosome3 containing the Foxo1 locus at different ages.
Extended Data Fig. 2 Ebf1 perturbation causes chromatin structure and expression changes in pro-B cells.
(a) Normalized tracks for RNA-Seq of Ebf1+/+ and Ebf1+/− pro-B cells across the Ebf1 locus are shown with IGV. “FC” represents fold change, and the Poisson test was applied with P values indicated (n = 2). (b) Average Hi-C contact plots (n = 2) derived from Ebf1+/+ and Ebf1+/− pro-B cells. Color shading refers to: compartments: pink, TADs and loops: green, and close interactions: yellow. (c) Experimental scheme for overexpressing Ebf1 in cultured pro-B cells. (d) Normalized tracks for RNA-Seq across the Ebf1 locus of different samples are shown with IGV. “FC” represents fold change, and the Poisson test was applied with P values indicated (n = 2). (e) Principal component analysis (PCA) plot depicting the distribution of RNA-Seq from different samples as indicated. (f) Schematic representation of differentially expressed gene counts across multiple comparisons.
Extended Data Fig. 3 Most decreased TADs in aged pro-B cells.
(a) A chart showing information of top 5 decreased TADs. TAD size is limited to be less than 5 Mb. B cell associated genes are in blue. (b) An example showing one of the top decreased TAD containing Ebf1 locus. Young (left) and old (right) Hi-C contact frequency heat maps are in 5 kb resolution. Normalized tracks for CTCF (left) and Rad21 (right) ChIP-Seq across the TAD are shown with IGV. ES (enrichment score) and RPKM values of the TAD are annotated. (c) Normalized expression levels of key genes involved in either chromatin structure maintenance (Ctcf, Rad21, Nipbl and Wapl) or B cell development (Pax5, Ebf1, Bach2 and Bcl11a) in young and old pro-B cells (n = 4). Copb2 is shown as a control. Data are presented as mean ± SEM. Unpaired two-sided t test was used and P-values were indicated. (d) Normalized expression levels of key genes involved in chromatin structure maintaining in Ebf1+/+, Ebf1+/− and Ebf1+/−Pax5+/− pro-B cells (n = 2). Bar graph represents the mean of two replicate experiments, with each replicate shown as a dot.
Extended Data Fig. 4 Wapl overexpression remodels the chromatin structure in the recombinase deficient pro-B cell line (D345).
(a) Flow cytometric analysis showing the D345 pro-B cell line with (left) or without (right) infection with Wapl-BFP lentivirus. The percentages of BFP+ and BFP- cells are indicated. BFP+ cells are sorted for experiments. (b) Normalized tracks for RNA-Seq across the Wapl locus are shown with IGV. “FC” represents fold change, and the Poisson test was applied with the P value indicated (n = 2). (c) Average Hi-C contact plots (n = 2) derived from BFP control and Wapl overexpressed D345 cells. Color shading refers to: compartments: pink, TADs and loops: green, and close interactions: yellow. (d) Quantitative comparison of TAD strength derived from Hi-C data of BFP control and Wapl overexpressed D345 cells. Similar analysis and the same cutoffs as in Fig. 3a were used. Representative genes from the top-ranked changed TADs are displayed. (e) Hi-C contact frequency heat maps (pooled from 2 biological replicates) showing the Igh TAD in BFP control and Wapl overexpressed D345 pro-B cells. A difference map (Wapl OE minus BFP control) for the same region is shown on the right; regions with increased and decreased interactions in old are colored red and blue, respectively. Schematics on top represent the Igh locus to scale; colors represent different parts of the locus as indicated to the right of the figure. (f) CellRadar (https://karlssong.github.io/cellradar/) plot derived from transcriptional changes identified in comparison of young and old pro-B cells (blue), Ebf1+/+ and Ebf1+/− pro-B cells (orange), and BFP control and Wapl overexpressed D345 cells. Differentially expressed genes (DEGs) with log2 fold change > 1 and P-value < 0.01 were used as input for young and old pro-B cells (blue), and Ebf1+/+ and Ebf1+/− pro-B cells. DEGs with P-value < 0.01 were used as input for BFP control and Wapl overexpressed D345 cells because of the limited number of DEGs by a more stringent cutoff.
Extended Data Fig. 5 H3K27ac mediated chromatin reorganization during aging.
(a) Measurement of H3K27ac levels in Rag2−/− young (blue) and old (red) pro-B cells via flow cytometry. The IgG isotype controls are shown in dotted lines. The dot plot on the bottom indicates the median fluorescence intensities (MFI) of H3K27ac levels in young and old pro-B cells. Data are presented as mean ± SEM. Unpaired two-sided t test was used, with the P-value indicated. (b) Age-selective p300 ChIP-Seq binding sites were identified in young and old pro-B cells. The analysis and cutoffs used were consistent with those in Fig. 4a. (c) Overlaps of young selective H3K27ac and p300 peaks.(d) Age-selective Brg1 ChIP-Seq binding sites were identified in young and old pro-B cells. The analysis and cutoffs used were consistent with those in Fig. 4a. (e) H3K27ac HiChIP heatmaps of the Ebf1 locus in young (upper) and old (lower) pro-B cells. The visualization elements are similar to that shown in Fig. 4h.
Extended Data Fig. 6 DH utilization and CDR3 length distribution are not affected by age.
(a) Average utilization of DH gene segments in VHDJH and DJH joins in young and old C57BL/6J pro-B cells by VDJ-Seq (Hu et al.49) using JH1 bait (n = 2). Clone names of DH gene segments are annotated. (b) Total CDR3 number in young and old C57BL/6J pro-B cells (n = 2). (c) CDR3 length distribution of productive VHDJH exons in young and old C57BL/6J pro-B cells by JH1 bait (n = 2). Bar graph represents the mean of two replicate experiments, with each replicate shown as a dot.
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Ma, F., Cao, Y., Du, H. et al. Three-dimensional chromatin reorganization regulates B cell development during ageing. Nat Cell Biol 26, 991–1002 (2024). https://doi.org/10.1038/s41556-024-01424-9
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DOI: https://doi.org/10.1038/s41556-024-01424-9