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A B C D ** CpG-free Luc -7,200 -5,900 e2piNOS-luc -4,900 e1piNOS-luc

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Presentation on theme: "A B C D ** CpG-free Luc -7,200 -5,900 e2piNOS-luc -4,900 e1piNOS-luc"— Presentation transcript:

1 A B C D ** CpG-free Luc -7,200 -5,900 e2piNOS-luc -4,900 e1piNOS-luc
-11,000 e3piNOS-luc A Figure 1. NF-κB-mediated iNOS transactivation is affected by the CpG methylation of specific enhancer regions in human chondrocytes. (A) Different NF- κB enhancer elements were inserted in the CpG-free vector containing the iNOS promoter and transfected into C28/I2 cells. (B-D) Luciferase activity was measured before and after in vitro methylation as described in material and methods. Values are expressed as mean ± SD (n = 3 independent experiments, each performed in duplicate). * = P < 0.05 by analysis of variance with post hoc t-test.

2 * Figure 2. Attenuated p65 binding to the NF-κB enhancer region at -5.8 kB in the presence of CpG methylation. ChIP assays were performed using cell lysates from C28/I2 cells that had been stably transfected with unmethylated vector (Meth-) and with methylated vector (Meth+) e1piNOS construct (Input) and the expression vector encoding p65. Binding of transcription factor to the human iNOS enhancer element was analysed by qPCR reaction using primers specifically bracketing NF-κB-binding sites. The results were quantified and are shown as the percentage input. Values are the mean ± SEM of 3 experiments and represent the fold-change versus IgG. * = P < 0.05.

3 * A B C Figure 3. DNA demethylation of the −5.8 kb NF-κB enhancer element and aberrant iNOS expression following long-term culture in 5-azadeoxycytidine (5-aza-dC) in healthy and OA human chondrocytes. (A) iNOS expression in primary human chondrocytes was analysed by quantitative reverse transcription-polymerase chain reaction. (B-C) Pyrosequencing analysis of the DNA methylation status of CpG sites in the NF-κB binding element at −5.8 kb. NOF = 7 and OA = 5; * = P < 0.05 by Wilcoxon’s signed rank test.

4 P = 0.013 P = 0.002 P = 0.159 Figure 4. Loss of methylation at the CpGs localised at −5.8 kb NF-κB enhancer element increase chondrocytic cell line proliferation. MTT assay was performed in C28/I2 cells after transfection with Met-e1piNOS and e1piNOS plasmids for 48 hours. Control bar represents cells transfected with empty vectors. Values are expressed as mean ± SD (n = 3 independent experiments, each performed in triplicate). * = P < 0.05 by analysis of variance with post hoc t-test.

5 A B * * G0/G1: 64.1% G0/G1: 59.4% S: 23.8% S: 21.9% G2/M: 6.9%
Figure 5. NF-κB-mediated iNOS transactivation is affected by the loss of CpG methylation of specific CpG sites in human chondrocytes and results in an alteration in cell cycle distribution. Results shown are from cell cycle analysis of C28/I2 cells stably transfected with methylated vector (e1piNOS-Met) and with unmethylated vector (e1piNOS). Values are expressed as mean ± SD. * = P < 0.05 by analysis of variance with post hoc t-test.

6 p = 0.009 p < 0.009 p = 0.006 A B C Figure 6. Cell cycle specific gene expression in primary human chondrocytes obtained from control subjects with femoral neck fracture and patients with osteoarthritis (OA). Differential expression of A: CCDN1; B: CDK6 C: CDKN2A in primary human chondrocytes obtained from control subjects with femoral neck fracture (#; n = 11) and from OA patients (n = 11), analysed by quantitative reverse transcription–polymerase chain reaction. Values are the mean ± SD of triplicate determinations per sample.

7 Cell cycle progression
Healthy chondrocytes OA chondrocytes CDK6 p50 p65 S G2 M −5.8 Kb iNOS G0 Cell cycle exit p16 Pro-inflammatory Responses (NO, IL-1β, TNF-α) Differentiation Cell cycle progression Proliferation G1 Cyclin D1 Figure 7. Proposed model of NF-κB-iNOS, cell cycle and DNA hypomethylation signalling in chondrocytes. Loss of methylation at specific CpG sites localised at the −5.8 kb NF-κB of the iNOS gene in OA chondrocytes permits binding of NF-κB transcription factor activating the expression of iNOS with implications in the OA chondrocyte pro-inflammatory responses, and via cell cycle regulation, propagation of the aberrant OA phenotype to daughter cells.

8 Supplementary Figures
epiNOS-luc Met-epiNOS-luc p50 p65 Supplementary Figure 2 p = p = CCDN CDK CDKN2A

9 Supplementary Table Gene Sequence (5'-3') qPCR GAPDH
F CCAGGTGGTCTCCTCTGACTTC R TCATACCAGGAAATGAGCTTGACA iNOS F GAGGAGCAGGTCGAGGACTAT R TCTTCGCCTCGTAAGGAAATAC CCND1 F CTACCGCCTCACACGCTT R CTTGGGGTCCATGTTCTGC CDK6 F TTTCGTGGAAGTTCAGATGTTG R CATCTCTAGGCCAGTCTTCTTCT CKN2A F GTGGACCTGGCTGAGGAG R CTTTCAATCGGGGATGTCTG Pyrosequencing Enhancer -5.8 kB F GTTTTTTTTGGTTTTGGGAAAGTT R TTAACCCAATTCTAAACCCCCTAT S TTATAAAGTGTATTGGAATGAG Cloning Promoter F ATTAGATCTTTTGCTTCTCAACTTCTCCCTAAT R ATACCATGGAGTTTTCGACTCGCTACAAAGTTA Enhancer 1 F ATTCCTGCAGGGGATACAAGAGGGTGGGCTTAG R ATTAGATCTGGGCGTGGCTCTTACTCTCTA Enhancer 2 F ATTCCTGCAGGTTGTCTGCCATCA R ATTAGATCTGATGCTGATCCAAGAAGT Enhancer 3 F ATTCCTGCAGGTAATGAGGAGTTCTT R ATTAGATCTCAATAGAGATGGCAAGATG ChIP RelA F GGGCTTATGTGGCCTAACCAA R CCACCAGGGAACTTGAAAAA

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