Exploring urine sediments as a non-invasive method for DNA methylation detection in bladder cancer

被引:2
|
作者
El Azzouzi, Meryem [1 ,2 ]
El Ahanidi, Hajar [1 ,2 ]
Alaoui, Chaimae Hafidi [1 ,5 ]
Chaoui, Imane [1 ]
Benbacer, Laila [1 ]
Tetou, Mohamed [2 ,3 ]
Hassan, Ilias [2 ,3 ]
Bensaid, Mounia [4 ]
Oukabli, Mohamed [2 ,4 ]
Ameur, Ahmed [2 ,3 ]
Al Bouzidi, Abderrahmane [2 ]
El Mzibri, Mohammed [1 ]
Attaleb, Mohammed [1 ]
机构
[1] CNESTEN, Biol & Med Res Unit, Rabat, Morocco
[2] Mohammed V Univ Rabat, Fac Med & Pharm Rabat, Rabat, Morocco
[3] Mohammed V Mil Teaching Hosp Rabat, Dept Urol, Rabat, Morocco
[4] Mohammed V Mil Teaching Hosp Rabat, Dept Pathol, Rabat, Morocco
[5] Mohammed V Univ Rabat, Fac Sci, Rabat, Morocco
关键词
DNA methylation; Non-invasive test; Bladder cancer; Urine sediments; EPIGENETIC BIOMARKERS; TMEFF2; TWIST1; GDF15; HTERT; VIM;
D O I
10.1186/s12301-022-00298-3
中图分类号
R5 [内科学]; R69 [泌尿科学(泌尿生殖系疾病)];
学科分类号
1002 ; 100201 ;
摘要
Background The main epigenetic event occurring during the bladder carcinogenesis process is DNA methylation, affecting genes involved in various metabolic pathways and cell regulation. The use of biological fluids such as urine sediments could be used as a non-invasive approach to enhance bladder cancer management. In this study, we aim to determine the promoter methylation status of a panel of genes in bladder cancer on tumor biopsies and urine sediments to evaluate the usefulness of urine samples as a non-invasive approach for methylation status assessment. Methods Using the methylation-specific PCR technique, we explored the promoter methylation status of hTERT, TWIST1, VIM and NID2 genes in 40 tumor biopsies and their paired urine samples from Moroccan bladder cancer patients. Results In this study, bladder tumors showed promoter hypermethylation frequency of individual genes as 90%, 85%, 62.5% and 72.5% in TWIST1, hTERT, NID2 and VIM genes, respectively. Interestingly, the specificity of methylation detection in urine samples was 100% and the sensitivity to detect hypermethylation of TWIST1, hTERT, NID2 and VIM genes reached 91.7%; 97.1%; 84% and 82.8%, respectively. Conclusions Our results clearly show that the assessment of promoter hypermethylation in urine samples is highly specific and has high sensitivity. Furthermore, urine sediments would be a useful approach to detect the DNA methylation status of genes and its potential association with bladder cancer development.
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页数:5
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