Randomized Terminal Linker-dependent PCR: A Versatile and Sensitive Method for Detection of DNA Damage

Objective To design and develop a novel, sensitive and versatile method for in vivo foot printing and studies of DNA damage, such as DNA adducts and strand breaks. Methods Starting with mammalian genomic DNA, single-stranded products were made by repeated primer extension, these products were ligated to a double-stranded linker having a randomized 3 overhang, and used for PCR. DNA breaks in p53 gene produced by restriction endonuclease AfaI were detected by using this new method followed by Southern hybridization with DIG-labeled probe. Results This randomized terminal linker-dependent PCR (RDPCR) method could generate band signals many-fold stronger than conventional ligation-mediated PCR (LMPCR), and it was more rapid, convenient and accurate than the terminal transferase-dependent PCR (TDPCR). Conclusion DNA strand breakage can be detected sensitively in the gene level by RDPCR. Any lesion that blocks primer extension should be detectable.

PDRG1 at the interface between intermediary metabolism and oncogenesis

PDRG1 is a small oncogenic protein of 133 residues. In normal human tissues, the p53 and DNA damageregulated gene 1(PDRG1) gene exhibits maximal expression in the testis and minimal levels in the liver. Increased expression has been detected in several tumor cells and in response to genotoxic stress. High-throughput studies identified the PDRG1 protein in a variety of macromolecular complexes involved in processes that are altered in cancer cells. For example, this oncogene has been found as part of the RNA polymerase Ⅱ complex, the splicing machinery and nutrient sensing machinery, although its role in these complexes remains unclear. More recently, the PDRG1 protein was found as an interaction target for the catalytic subunits of methionine adenosyltransferases. These enzymes synthesize S-adenosylmethionine, the methyl donor for, among others, epigenetic methylations that occur on the DNA and histones. In fact, downregulation of S-adenosylmethionine synthesis is the first functional effect directly ascribed to PDRG1. The existence of global DNA hypomethylation, together with increased PDRG1 expression, in many tumor cells highlights the importance of this interaction as one of the putative underlying causes for cell transformation. Here, we will review the accumulated knowledge on this oncogene, emphasizing the numerous aspects that remain to be explored.

p53和DNA损伤调节基因1在口腔癌组织中的表达及通过Wnt/β-catenin信号途径对口腔癌细胞自噬和凋亡的影响

目的:探讨p53和DNA损伤调节基因1(PDRG1)在口腔癌组织中的表达及通过Wnt/β-catenin信号途径对口腔癌细胞自噬和凋亡的影响。方法:收集2017年6月至2019年6月在河南省第二人民医院60例接受口腔癌切除手术的患者的癌组织标本及配对的癌旁组织,qRT-PCR和免疫印迹检测PDRG1在口腔癌组织中的mRNA和蛋白表达;同时体外培养正常人口腔角质形成细胞(NHOK)和口腔癌细胞系,qRT-PCR和免疫印迹检测PDRG1在口腔癌细胞系中的mRNA和蛋白表达;将口腔癌细胞系SCC-15细胞分为shNC组和shPDRG1组,细胞集落形成实验检测细胞增殖能力;免疫印迹检测细胞中LC3Ⅱ/LC3Ⅰ蛋白表达比例;透射电镜检测细胞中自噬体数量;流式细胞术检测细胞凋亡率;免疫印迹检测Wnt/β-catenin信号途径相关蛋白表达。结果:PDRG1在口腔癌组织和口腔癌细胞系中高表达;与shNC组相比,shPDRG1组SCC-15细胞中PDRG1 mRNA的表达显著下降,PDRG1蛋白的表达水平明显下调。与shNC组相比,shPDRG1组SCC-15细胞的集落数目明显减少,细胞中LC3Ⅱ/LC3Ⅰ的比例减少;与shNC组比较,shPDRG1组细胞中自噬体数量减少,细胞的凋亡率明显提高,细胞中β-catenin、c-Myc、cyclin D1蛋白表达水平下调。结论:PDRG1在口腔癌组织和口腔癌细胞系中高表达,沉默PDRG1抑制SCC-15细胞增殖和自噬,增强SCC-15细胞的凋亡率及抑制Wnt/β-catenin信号途径。

Human umbilical cord mesenchymal stem cells attenuate diabetic nephropathy through the IGF1R-CHK2-p53 signalling axis in male rats with type 2 diabetes mellitus

diabetes mellitus(DM)is a disease syndrome characterized by chronic hyperglycaemia.A long-term high-glucose environment leads to reactive oxygen species(ROS)production and nuclear DNA damage.human umbilical cord mesenchymal stem cell(HUcMSC)infusion induces significant antidiabetic effects in type 2 diabetes mellitus(T2DM)rats.Insulin-like growth factor 1(IGF1)receptor(IGF1R)is important in promoting glucose metabolism in diabetes;however,the mechanism by which HUcMSC can treat diabetes through IGF1R and DNA damage repair remains unclear.In this study,a DM rat model was induced with high-fat diet feeding and streptozotocin(STZ)administration and rats were infused four times with HUcMSC.Blood glucose,interleukin-6(IL-6),IL-10,glomerular basement membrane,and renal function were examined.Proteins that interacted with IGF1R were determined through coimmunoprecipitation assays.The expression of IGF1R,phosphorylated checkpoint kinase 2(p-CHK2),and phosphorylated protein 53(p-p53)was examined using immunohistochemistry(IHC)and western blot analysis.Enzyme-linked immunosorbent assay(ELISA)was used to determine the serum levels of 8-hydroxydeoxyguanosine(8-OHdG).Flow cytometry experiments were used to detect the surface markers of HUcMSC.The identification of the morphology and phenotype of HUcMSC was performed by way of oil red“O”staining and Alizarin red staining.DM rats exhibited abnormal blood glucose and IL-6/10 levels and renal function changes in the glomerular basement membrane,increased the expression of IGF1 and IGF1R.IGF1R interacted with CHK2,and the expression of p-CHK2 was significantly decreased in IGF1R-knockdown cells.When cisplatin was used to induce DNA damage,the expression of p-CHK2 was higher than that in the IGF1R-knockdown group without cisplatin treatment.HUcMSC infusion ameliorated abnormalities and preserved kidney structure and function in DM rats.The expression of IGF1,IGF1R,p-CHK2,and p-p53,and the level of 8-OHdG in the DM group increased significantly compared with those in the control group,and decreased after HUcMSC treatment.Our results suggested that IGF1R could interact with CHK2 and mediate DNA damage.HUcMSC infusion protected against kidney injury in DM rats.The underlying mechanisms may include HUcMSC-mediated enhancement of diabetes treatment via the IGF1R-CHK2-p53 signalling pathway.