在DLK1-DIO3基因组区域的参与下,多发性骨髓瘤细胞改变骨髓间充质基质细胞的衰老表型。
Multiple myeloma cells alter the senescence phenotype of bone marrow mesenchymal stromal cells under participation of the DLK1-DIO3 genomic region.
作者信息
Berenstein Rimma, Blau Olga, Nogai Axel, Waechter Marlies, Slonova Ekaterina, Schmidt-Hieber Martin, Kunitz Annegret, Pezzutto Antonio, Doerken Bernd, Blau Igor Wolfgang
机构信息
Department of Hematology, Oncology and Tumourimmunology, Charité Universitätsmedizin Berlin, Hindenburgdamm 30, 12200, Berlin, Germany.
Department of Hematology, Oncology and Tumourimmunology, Helios Clinic Berlin-Buch, Berlin, Germany.
出版信息
BMC Cancer. 2015 Feb 18;15:68. doi: 10.1186/s12885-015-1078-3.
BACKGROUND
Alterations and senescence in bone marrow mesenchymal stromal cells of multiple myeloma patients (MM-BMMSCs) have become an important research focus. However the role of senescence in the pathophysiology of MM is not clear.
METHODS
Correlation between senescence, cell cycle and microRNA expression of MM-BMMSCs (n = 89) was analyzed. Gene expression analysis, copy number analysis and methylation specific PCR were performed by Real-Time PCR. Furthermore, cyclin E1, cyclin D1, p16 and p21 genes were analyzed at the protein level using ELISA. Cell cycle and senescence were analyzed by FACS. MiRNA transfection was performed with miR-485-5p inhibitor and mimic followed by downstream analysis of senescence and cell cycle characteristics of MM-BMMSCs. Results were analyzed by Mann-Whitney U test, Wilcoxon signed-rank test and paired t-test depending on the experimental set up.
RESULTS
MM-BMMSCs displayed increased senescence associated β-galactosidase activity (SA-βGalA), cell cycle arrest in S phase and overexpression of microRNAs. The overexpressed microRNAs miR-485-5p and miR-519d are located on DLK1-DIO3 and C19MC, respectively. Analyses revealed copy number accumulation and hypomethylation of both clusters. KMS12-PE myeloma cells decreased SA-βGalA and influenced cell cycle characteristics of MM-BMMSCs. MiR-485-5p was significantly decreased in co-cultured MM-BMMSCs in connection with an increased methylation of DLK1-DIO3. Modification of miR-485-5p levels using microRNA mimic or inhibitor altered senescence and cell cycle characteristics of MM-BMMSCs.
CONCLUSIONS
Here, we show for the first time that MM-BMMSCs have aberrant methylation and copy number of the DLK1-DIO3 and C19MC genomic region. Furthermore, this is the first study pointing that multiple myeloma cells in vitro reduce both the senescence phenotype of MM-BMMSCs and the expression of miR-223 and miR-485-5p. Thus, it is questionable whether senescence of MM-BMMSCs plays a pathological role in active multiple myeloma or is more important when cell interaction with myeloma cells is inhibited. Furthermore, we found that MiR-485-5p, which is located on the DLK1-DIO3 cluster, seems to participate in the regulation of senescence status and cell cycle characteristics of MM-BMMSCs. Thus, further exploration of the microRNAs of DLK1-DIO3 could provide further insights into the origin of the senescence state and its reversal in MM-BMMSCs.
背景
多发性骨髓瘤患者骨髓间充质基质细胞(MM-BMMSCs)的改变和衰老已成为重要的研究焦点。然而,衰老在MM病理生理学中的作用尚不清楚。
方法
分析了89例MM-BMMSCs的衰老、细胞周期与微小RNA表达之间的相关性。通过实时PCR进行基因表达分析、拷贝数分析和甲基化特异性PCR。此外,使用ELISA在蛋白质水平分析细胞周期蛋白E1、细胞周期蛋白D1、p16和p21基因。通过流式细胞术分析细胞周期和衰老情况。用miR-485-5p抑制剂和模拟物进行miRNA转染,随后对MM-BMMSCs的衰老和细胞周期特征进行下游分析。根据实验设置,采用曼-惠特尼U检验、威尔科克森符号秩检验和配对t检验分析结果。
结果
MM-BMMSCs表现出衰老相关β-半乳糖苷酶活性(SA-βGalA)增加、S期细胞周期停滞和微小RNA过表达。过表达的微小RNA miR-485-5p和miR-519d分别位于DLK1-DIO3和C19MC上。分析显示这两个基因座均存在拷贝数积累和低甲基化。KMS12-PE骨髓瘤细胞降低了SA-βGalA并影响了MM-BMMSCs的细胞周期特征。在共培养的MM-BMMSCs中,miR-485-5p显著降低,同时DLK1-DIO3的甲基化增加。使用微小RNA模拟物或抑制剂改变miR-485-5p水平,可改变MM-BMMSCs的衰老和细胞周期特征。
结论
在此,我们首次表明MM-BMMSCs在DLK1-DIO3和C19MC基因组区域存在异常甲基化和拷贝数。此外,这是第一项指出体外多发性骨髓瘤细胞可降低MM-BMMSCs的衰老表型以及miR-223和miR-485-5p表达的研究。因此,MM-BMMSCs的衰老在活动性多发性骨髓瘤中是否起病理作用,或者在细胞与骨髓瘤细胞的相互作用受到抑制时是否更重要,这是值得怀疑的。此外,我们发现位于DLK1-DIO3基因座上的miR-485-5p似乎参与了MM-BMMSCs衰老状态和细胞周期特征的调节。因此,进一步探索DLK1-DIO3的微小RNA可为MM-BMMSCs衰老状态的起源及其逆转提供进一步的见解。
Zotero 插件