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1
Systemic Lupus Erythematosus and DNA Methylation
Terrence ShinMCB 5255Dr. LynesMar. 28, 2012
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Systemic Lupus Erythematosus (SLE) Chronic autoimmune disorder
Affects skin, joints, kidneys, and others Joint pain and swelling Lupus nephritis
Cause – Unknown Ages: 10~50 More common in women African Americans and Asians are affected
more often
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Common Symptoms of SLE
Chest pain Fatigue Fever Hair loss Mouth sores Swollen lymph nodes Skin/Butterfly rash
Photosensitive
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Possible Body Parts Targeted by SLE Skin
Raynaud’s phenomenon Brain & nervous system Lungs Heart
Arrhythmias Tachycardia Bradycardia
Digestive tract
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Diagnosis of SLE
CBC ANA Chest x-ray Urinalysis Renal biopsy
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Patients with SLE met at least four of revised criteria of the American College of Rheumatology.
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Treatment for SLE
No cure Control symptoms
Anti-inflammatory medication Corticosteroids Protection from sunlight
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Ultraviolet B exposure of peripheral blood mononuclear cells of patients with systemic lupus erythematosus inhibits DNA methylation
GS Wang, M Zhang, XP Li, H Zhang, W Chen, M Kan and YM Wang
Lupus 2009
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Background
Sunlight can induce exacerbation of SLE Ultraviolet B (UVB): 290~320 nm
SLE cells are hypomethylated Promoters of transcriptionally active gene
DNA methylation Suppressive effects on gene expression 5th position of the cytosine ring Catalyzed by DNMT1
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Specific Aims
What are the effect of UVB on DNA methylation in SLE? What is its significance in the pathogenesis of
SLE ?
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Materials & Methods
Study participants Isolation of PBMCs Irradiation protocol DNA extraction and HPCE RNA isolation and RT-PCR Statistical analysis
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Study Participants
45 patients with SLE 40 females, 5 males Mean age: 36 years; range: 18~61 years Active = SLEDAI ≥ 10 (21 out of 45 patients)
20 healthy volunteers (control) Sex- and age-matched 18 females, 2 males Mean age: 31 years, range: 22~46 years
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Isolation of PBMCs
Total volume of 20 ml of ethylenediaminetetraacetic acid (EDTA)-K2-preserved venous peripheral blood drawn from patients & controls Ficoll gradient centrifugation
PBMCs
PBMCs cultured in RPMI 1640 medium Supplemented with 10% heat-inactivated FBS, 2
mM sodium pyruvate, 100 IU/ml penicillin and 100 μg/ml streptomycin
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Irradiation Protocol
UVB irradiation Waldman UV109B lights with TL-12 lamps
(Waldman Lighting Ltd., Germany) Emit within the UVB range (290–320 nm) with an
emission peak at 311 nm
PBMC were irradiated in PBS with different doses of UVB (0, 50 and 100 mJ/cm2) PBS removed RPMI 1640 containing 10% FBS
added cultured (24 h) DNA & RNA extractions
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DNA Extraction and HPCE
Five deoxynucleoside standards purchased from International Laboratory (CA, USA) dA = 2’-deoxyadenosine dT = 2’-deoxythymidine dG = 2’-deoxyguanosine dC = 2’-deoxycytidine mdC = 5-methyl-2’-deoxycytidine
All nucleosides were dissolved in ddH2O water
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DNA Extraction and HPCE (cont.) DNA extraction
gDNA extraction kit (QIAmp, DNA mini kit; Qiagen, Hilden, Germany)
RNA digestion Added 20 μg/μl RNase A (Sigma-Aldrich, St. Louis, MO)
DNA hydrolysis Heated 18 μl of DNA samples for 2 min in boiling water bath
cooled rapidly in ice Added 4.5 μl of 10 mM ZnSO4 and 7.5 μl of nuclease P1 (Sigma-
Aldrich, St. Louis, MO) Incubated at 37°C for 16 h Added 7.5 μl of Tris (0.5 M, pH 8.3), and 4.5 μl of alkaline
phosphatase (Sigma-Aldrich, St. Louis, MO) and 50 U/ml in 2.5 M (NH4)2SO4
Incubated at 37°C for 2 h
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DNA Extraction and HPCE (cont.) CE system (Beckman P/ACETM MDQ)
Uncoated fused-silica capillary (60 cm × 75 μm, effective length 57 cm) Connected to Millennium data-processing station Buffer: 48 mM NaHCO3 (pH 9.6) containing 60 mM SDS Constant voltage (20 kV) and temperature (25°C) Pressure injected for 5 s Hydrolysed DNA or 0.1 mM free deoxynucleoside standard was injected into
a HPCE analysis system equipped with photodiode array (PDA) detection Absorbance was monitored at 256 nm
Capillary conditioning Washed with 1 M NaOH (2 min) washed with 1 mM NaOH (1 min) filled with
the running buffer (3 min) Buffers and washing solutions were filtered through 0.45 μm pores
Hydrolyzed samples Injected hydrostatically (30 s) from 9.8 cm above the cathode
Comparison of migration time & peak area of each sample with the standards Can calculate DNA methylation levels
Quantification of the relative methylation of each DNA sample mdC/(dC + mdC) x 100%
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RNA Isolation and RT-PCR
Total RNA Isolated from PBMCs
Trizol reagent (Invitrogen, Carlsbad, CA, USA) Reverse transcription
Reverse Transcription System (Promega, Madison, WI, USA)
cDNA synthesis 1.0 μg total RNA—single round reverse transcriptase
reaction (TV = 20 μl) containing 0.5 μg oligo (dT) 15 primer, 2.0 μl dNTPs, 2.0 μl reverse transcriptase 10x buffer, 15 μl AMV reverse transcriptase and 0.5 μl recombinant RNasin ribonuclease inhibitor.
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RNA Isolation and RT-PCR (cont.) RT-PCR
ABI Prism 7500 Sequence Detection System Using SYBR Premix Ex Taq Kit (TaKaRa Bio Inc.)
10 μl of 2x SYBR green Master Mix, 0.2 μM primers, 5 μl 1:5 dilution of prepared cDNA, 20 μl of water
40 cycles at 94°C (30 s), 60°C (40 s), and 72°C (60 s)
Primers used: β-actin (forward & reverse), DNMT1 (forward & reverse)
Purchased from TaKaRa Bio Inc
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Statistical Analysis
Mann-Whitney U-test or one-way ANOVA Equality of means—to compare values
Spearman’s rank correlation Examine the relationship between two continuous
variables
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Figure 1: Electrophoretogram of nucleosides separated by HPCE
A. Electrophoretogram—standard nucleosides
B. Electropherogram of hydrolyzed gDNA from SLE patients
Five deoxynucleosides could be distinguished under the given conditions
(running buffer of 48 mM NaHCO3, at pH 9.6, containing 60mM SDS, with a separation voltage of 20 kV, injection pressure of 0.7 psi, at 25 °C and pressure injection of 5 s)
22
Figure 2: Calibration curves
A. dC regression B. mdC regression
• Different quantities of dC and mdC were added to a mixture of dA, dT and dG (0.1 mM) to obtain the concentrations of dC, and mdC
23
Figure 3: DNA methylation in SLE patients and controls
•Significant decrease in DNA methylation level in A and S compared to C
•No difference between A & S SLE patients
A=active; S=stable; C=control
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All groups showed decreased DNA methylation levels
•Active SLE group showed significant decrease after 50 mJ/cm2
•Stabe SLE group showed significant decrease after 100 mJ/cm2
•Control group showed significant decrease after 100 mJ/cm2
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Figure 4: Electrophoretograms of nucleosides from irradiated PBMC
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Figure 5: DNMT1 mRNA expression of irradiated PBMC
• No significant differences could be found in the expression of DNMT1 before and after UVB radiation
27
• Decrease in DNA methylation levels for all patients after UVB irradiation irrespective of their clinical characteristics
• Patients with malar rashes have lower DNA methylation levels than patients without rashes
• Patients with leucopenia had significantly lower DNA methylation levels after UVB irradiation than that in patients with normal leucocyte numbers
•No obvious differences were observed between patients with or without thrombocytopenia
28
Discussion & Unknowns
SLE patients have significantly lower levels of methylated DNA compared to controls (without UVB irradiation) Does down-regulation of DNA methylation play a role in the
pathogenesis of SLE? DNA methylation levels decreased after UVB
exposure Especially for patients with facial rash and leucopenia Does UVB play a role in pathogenesis of SLE by
decreasing DNA methylation?
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IL-6 Modulates CD5 Expression in B Cells from Patients with Lupus by Regulating DNA Methylation
Soizic Garaud, Christelle Le Dantec, Sandrine Jousse-Joulin, Catherine Hanrotel-Saliou, Alain Saraux, Rizgar A. Mageed, Pierre Youinou and Yves Renaudineau
The Journal of Immunology, 2009
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Background
Features of autoimmunity in SLE B cell hyperactivity Spontaneous lymphocyte proliferation Production of antibodies to self-antigens
B cell abnormalities in SLE Excess cytokine production Autoantigen presentation to T cells Modulation of the function of other immune cells
SLE is considered as a B cell disease Therapies target B cells
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Background (cont.)
CD5 isoforms CD5-E1A CD5-E1B
Demethylated in B cells of SLE patients CD5-E1B mRNA is transcribed at the expense of CD5-E1A
mRNA transcription
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Specific Aims
Does the engagement of the BCR with constitutive IL-6 down-regulate the level of membrane CD5, which negatively regulates BCR signaling, in SLE B cells? Does this signal promote the activation and
expansion of autoreactive B cells in SLE patients?
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Materials & Methods
B lymphocyte isolation FACS analysis Cell culture mRNA extraction and quantitative RT-PCR RACE Methylation-specific PCR Bisulfite sequencing Chromatin immunoprecipitation (ChIP) Computational promoter analysis Statistics
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B Lymphocyte Isolation
PBMCs from the blood of 25 SLE patients and HCs Centrifugation on
Ficoll-Hypaque Active = SLEDAI
≥ 5
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B Lymphocyte Isolation (cont.) Cells permeabilized with 70% methanol
intracellular staining FITC-anti-CD19 (clone J4-119) and PE-anti-CD5 (clone
BL1a) Obtained from Beckman-Coulter
Anti-DNMT1 and anti-p27kip1
Obtained from Abcam CD5-CD19+ B cells
Sorted on an Epics Elite FACS (Beckman-Coulter) 98% CD19+
Daudi human B cell line Purchased from American Type Culture Collection
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FACS Analysis
Number of CD5 molecules per cell Quantum Simply Cellular kit
Amount of Ab binding to the cells (ABC) at saturating concentrations
FACS analysis 50μl calibrated microspheres stained with 20 μl of
the same anti-CD5 Ab Mean fluorescence intensity standard ABC curve
arbitrary ABC value
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Cell Culture
B cells (sorted via FACS) Suspended in RPMI 1640
Supplemented with 10% heat-inactivated FCS, 2 mM L-glutamine, 200 U/ml penicillin and 100 μg/ml streptomycin.
B lymphocytes were seeded at 2 x 105 cells per well Incubated with 1 μg/ml anti-IgM Ab-coated Sepharose beads
(BioRad) and 10 U/ml IL-2 In the presence or absence of 10–40 ng/ml anti-IL-6RAb (R&D
Systems), or 100 ng/ml rhIL-6 (Immuno Tools). Repression of DNMTs
Incubated with 50 μM of the ras signal blocker PD98059 Detected IL-6 and IFN-ɣ in sera Detected IL-6 in the supernatant of cultured cells using ELISA kits
(Beckman Coulter).
38
mRNA Extraction and qRT-PCR Total mRNA
Extracted using the RNAble method (Eurobio) cDNA synthesis
Reverse transcription 20 μl volume with Superscript II RNase H-RT (Invitrogen
Corporation). Quantitative RT-PCR
Conducted in 20 μl mixtures 50 ng template cDNA 1X Sybr Green PCR Master mix (Applied Biosystems) 500 nM of each primer (Table II)
All assays included a negative and positive controls CT method
Comparison of cycle thresholds 18S as an internal control
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mRNA Extraction and qRT-PCR (cont.)
40
RACE
mRNA 5’ transcript ends Amplified with SMART-RACE kit (Clontech)
cDNA first strand synthesis Sense UPM primer and the gene-specific antisense primer CD5 E5 (Table II)
PCR protocol Initial denaturation at 94°C for 5 min 5 touchdown-PCR cycles of
denaturation at 94°C for 30 s Annealing at 72°C for 3 min Another 5 cycles at 94°C for 30 s, 70°C for 30 s, 72°C for 3 min decreasing temperature for 35 cycles of 94°C or 30 s, 68°C for 30 s, 72°C for 3 min.
Nested PCR Sense NUP primer and the gene-specific antisense primer CD5 E3 Second PCR round:
40 cycles at 94°C for 30 s, 56°C for 1 min, and 72°C for 1 min with a final extension at 72°C for 10 min.
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RACE (cont.)
NUP Primer
UPM Primer
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Methylation-specific PCR
Genomic DNA Purification – QIAmp 96 DNA blood kit (Qiagen) Digestion – 20 U of the methylation-sensitive REs (HpaII, HaeII, FauI, HgaI)
or the methylation insensitive restriction enzyme (MspI) – 37°C for 3 h Undigested Genomic DNA
Positive control PCR primers
Positioned upstream and downstream of E1A and E1B promoter recognition sites E1A and E1B of CD5, CD19 CD70, Pax5, Syk, and HRES-1 genes (Table II)
PCR protocol Initial denaturation at 94°C for 5 min 35 cycles of denaturation at 94°C for
30 s, annealing at 56°C for 1 min, and primer extension at 72°C for 1 min final extension at 72°C for 10 min.
Products separated on agarose gel Visualized with 0.5 g/ml ethidium bromide.
43
Methylation-specific PCR (cont.)
44
Bisulfite Sequencing
Methylation status of DNA Non-methylated cytosines were converted to uridines by bisulfite treatment
EZ-DNA methylation-Gold kit (Zymo Research) Unmodified DNA (100 ng)
Amplified 40 times at 56°C using specific primers Sequenced using specific primers
Bisulfite-converted DNA Amplified by nested PCR using two rounds of 40 cycles each at 56°C with
primers specific for methylated cytosines (Table II) PCR products
Purification – high pure PCR product purification kit (Roche) Sequencing – Internal primers
BigDye Terminator Cycle Sequencing kit using an automated ABI-310 genetic analyzer (Applied Biosystems)
Electrophoregram Quantification of T and C peaks Determination of methylation status = [peak (C)/peak (T) + peak (C)] x 100
45
Bisulfite Sequencing (cont.)
46
ChIP
EpiQuik kit (Epigentek Group) Evaluation of the activation of the CD5-E1B promoter Sonicated DNA (200–1000 bp)
Transferred into strip wells Precoated with mouse anti-RNA polymerase II, or with a nonspecific mouse IgG, used as a
negative control Incubated for 90 min at room temperature, then washed Precipitated DNA-protein complexes
Treated with 250 μg/ml proteinase K in the DNA release buffer for 15 min Left in the same buffer for 90 min at 65°C
Collection of DNA samples P-spin columns, washed with ethanol, and eluted
PCR Template – purified DNA GAPDH & CD5-E1B specific primers (Table II) 40 cycles at 56°C Products were separated on agarose gel
Visualized with 0.5 g/ml ethidium bromide.
47
ChIP (cont.)
48
Computational Promoter Analysis Identification of putative transcription factor
binding sites Alibaba (v2.1) TESS (transcription element search system) Genomatix
49
Statistical Analysis
Results as arithmetic means with SD Mann-Whitney U test
Unpaired data Wilcoxon test
Paired data Spearman’s rank correlation
50
Figure 1: CD5 expression in B cells
A. Percentage of CD5-expressing B cells
B. Anti-CD5 Ab bound to the cell membrane
Scattergrams
C. FACS profile of one SLE patient and one HC: cell surface expression of CD5
51
Figure 1: CD5 expression in B cells (cont.)
D. Histograms from qRT-PCR; B-cells were stimulated with anti-IgM (24h) increase in CD5-E1B transcription
Incubating HC IgM with PD98059 upregulation of CD5-E1B
Expression of CD5-E1A also increased in both
52
Figure 1: CD5 expression in B cells (cont.)
E. CD5-E1B = 639 bpCD5-E1A = 259 bp
• B cells from HCs
• BCR engagement induce CD5-E1A, but not CD5-E1B transcripts
• Stimulated with anti-IgM in the presence of PD98059 both are induced
53
Figure 2: Amplification of methylation sensitive, endonuclease-digested genomic DNA reveals methylation status of the alternative promoters of CD5 in resting B cells
A. Affected promoters and corresponding restriction enzymes
• CD5-E1B promoter arises from LTR• 1177-bp CD5-E1B amplicon contains six HpaII/MspI motifs and one
HaeII motif • 783-bp CD5-E1A amplicon contains one HgaI motif, one FauI motif
and two HpaII/MspI motifs
LTR
54
Figure 2: Amplification of methylation sensitive, endonuclease-digested genomic DNA reveals methylation status of the alternative promoters of CD5 in resting B cells (cont.)
B. Amplification of gDNA digested with methylation sensitive HaeII, HpaII, or methylation insensitive MspI enzymes
HaeII – demethylated CD5-E1B promoter only in SLE patients
HpaII – demethylation in two of six SLE patients
MspI (HpaII isoschizomer) – negative control; cut the CpG sequences no PCR products
Daudi – positive control
55
Figure 2: Amplification of methylation sensitive, endonuclease-digested genomic DNA reveals methylation status of the alternative promoters of CD5 in resting B cells (cont.)
C. Analysis of the CD5-E1A promoter region
CpG motifs – demethylated or hemimethylated in both SLE and HCs
56
Figure 3: The U3-LTR HERV-CD5 region is de-methylated in B cells from SLE patients
A. Circles = CpG; boxes = U3/R/U5 regions
HaeII site (4), HpaII sites (1, 7, 13) HERV U3-R-U5
regulatory elements may be de- methylated in B cells from SLE patients
57
Figure 3: The U3-LTR HERV-CD5 region is de-methylated in B cells from SLE patients (cont.)B. Bisulfite C T transition
• White = SLE patients; black = HCs
• Bisulfite sequencing of gDNA level of CpG methylation
• Five CpG sites (2~6) in the U3 region are hemi- or de-methylated.
• C residues near the E2/Rb binding sites (3, 4), and the CpG site (5), were significantly less affected by the bisulfite treatment in the SLE patients compared to HCs
*, p < 0.05; **, p < 0.001
58
Figure 3: The U3-LTR HERV-CD5 region is de-methylated in B cells from SLE patients (cont.)
C. SLE patients have an inverse correlation between CD5 cell surface expression and methylation status of CpG sites (3~5), but not site 6
White circles = SLE patients; black circles = HCs
59
Figure 4: Effect of BCR engagement on CD5 gene methylation
A, B. Effect of BCR engagement on methylation of the CD5 locus—FACS-sorted CD5-negative B cells stimulated with anti-IgM (24 h)
• BCR engagement did not alter SLE B cell methylation status• HCs stimulated with anti-IgM in the presence of PD98059 were demethylated• Not much change in the CD5-E1A for both
60
Figure 4: Effect of BCR engagement on CD5 gene methylation (cont.)
C. The level of CpG methylation (in SLE patients) measured by bisulfite sequencing
• White = with; black = without BCR engagement
• BCR engagement did not alter the methylation status
61
Figure 4: Effect of BCR engagement on CD5 gene methylation (cont.)
*, p < 0.05
D. CpG methylation in B cells of HCs—stimulated with anti IgM
• Gray = with PD98059; white = without PD98059
• Methylation of the CD5-E1B promoter at sites 3 & 4 with BCR engagement
• HCs stimulated with anti-IgM in the presence of PD98059
CpG sites 3, 4, and 5 were demethylated (similar to SLE B cells)
62
DNMT1, DNMT3a, DNMT3b, MBD2, and MBD4 levels in B cells were similar
63
Figure 5: Involvement of DNMTs on CD5-E1B expression
A. DNMT1 expression in B cells with BCR engagement Increased by 2.3 ± 0.2-fold in SLE patients Increased by 16.6 ± 13.4-fold in the controls
MBD expressions were not affected by BCR engagement or by the addition of PD98059
64
Figure 5: Involvement of DNMTs on CD5-E1B expression (cont.)
B. FACS analyses—BCR engagement modified DNMT1 expression
• Resting B cells vs. B cells with anti-IgM (% DNMT1bright) Patients: 23.8 ± 7.9% 46.1 ± 7.8% HCs: 25.3 ± 12.3% 86.1 ± 12.2%
Induction of DNMT1 following BCR engagement is reduced in patients with SLE
65
Figure 6: The effect of IL-6 on CD5-E1B expression and promoter methylation
A. FACS-sorted B cells from six HCs were stimulated for 48 h with rhIL-6 in the presence or absence of anti-IgM
• Test if IL-6 requires BCR engagement
• CD5-E1B expression increased by 4.1 ± 3.13-fold in B cells cultured with rhIL-6, and by 54.8 ± 11.3-fold in B cells cultured with rhIL-6 and anti-IgM
• rhIL-6 negated DNMT1 mRNA induction by anti-IgM
66
Figure 6: The effect of IL-6 on CD5-E1B expression and promoter methylation (cont.)
B. CD5-E1B induction upon anti-IgM/rhIL-6 stimulation
RNA pol II was recruited to the CD5-E1B promoter upon stimulation
c- = nonspecific mouse IgG as negative controlc+ = mouse anti-RNA polymerase as positive control
67
Figure 6: The effect of IL-6 on CD5-E1B expression and promoter methylation (cont.)
C. DNMT1 and p27kip1 from the HCs incubated with IL-6 in the presence or absence of anti-IgM
• Number of DNMT1bright cells was reduced after anti-IgM stimulation in the presence of rhIL-6
Due to cell cycle blockade? Over-expression of p27kip1 in anti-IgM/rhIL-6-stimulated B cells
Control of CpG methylation by IL-6 (in SLE B cells) may be resulting from its effect on arresting cells at the late G1 phase of the cell cycle.
68
Figure 7: Anti-IgM-induced methylation of promoters for CD19, CD70, Pax5, Syk, and HRES-1 A. HC B cells incubated with anti-IgM in
the presence or absence of anti-IL-6R Ab
• Methylation of five promoters (determined by PCR) Known to be regulated by
methylation
Determine the effect of IL-6 on methylation
• Hypomethylated in resting B cells• Stimulation with anti-IgM only
increased the methylation of the HRES-1 Reversed when IL-6 was
present
HpaII = methylation-sensitive;MspI = methylation-insensitive
69
Figure 7: Anti-IgM-induced methylation of promoters for CD19, CD70, Pax5, Syk, and HRES-1 (cont.)
B. Methylation of the HpaII-digested bandsHRES-1 promoter undigested bands
*, p < 0.05
= (in six HCs)
70
Figure 8: IL-6-dependent modulation of methylation in SLE B cells
A. CD5 cell surface expression in relation to the detection level of IL-6
IL-6 decreased CD5 expression
B. CD5 cell surface expression in relation to the detection level of IFN-ɣ—not significant
71
Figure 8: IL-6-dependent modulation of methylation in SLE B cells (cont.)
C. FACS-sorted B cells cultured with anti-IgM in the presence or absence of up to 40 ng/ml anti-IL-6R Ab
Blocking IL-6 increased DNMT1, and decreased CD5-E1B expression as the dose of anti-IL-6R Ab went up
72
Figure 8: IL-6-dependent modulation of methylation in SLE B cells (cont.)
D. Effect of anti-IgM/anti-IL-6R (gray) on methylation status of CD5-E1B promoter
Blocking of IL-6 contributed to the methylation of the U3-LTR sites 3 ~ 5.
73
Discussion
B cells from SLE patients have reduced membrane CD5 levels Due to increased expression of CD5-E1B (retained in the
cytoplasm) CD5-E1B promoter (U3-LTR) is demethylated in SLE B cells
Differential methylation is more pronounced with BCR engagement
CD5-E1B mRNA is transcribed at the expense of CD5-E1A mRNA transcription
B cells (of SLE patients) cannot induce DNMT1 due to production of IL-6 Cannot methylate DNA Similar demethylation patterns of CpG islands when compared to
HCs stimulated with IL-6 or PD98059
74
Therapeutic Treatment?
IL-6 activates CD5-E1B transcription SLE patients with anti-IL-6R mAb could inhibit
autoreactive B cell expansion by restoring DNA methylation and cell cycle progression