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首页> 外文期刊>Mutation Research: International Journal on Mutagenesis, Chromosome Breakage and Related Subjects >Alkaline, Endo III and FPG modified comet assay as biomarkers for the detection of oxidative DNA damage in rats with experimentally induced diabetes.
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Alkaline, Endo III and FPG modified comet assay as biomarkers for the detection of oxidative DNA damage in rats with experimentally induced diabetes.

机译:碱性,Endo III和FPG修饰的彗星测定法可作为生物标记物,用于检测实验性糖尿病大鼠的氧化性DNA损伤。

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摘要

Increased production of reactive oxygen species under diabetic condition underlines the higher oxidatively damaged DNA in different tissues. However, it is practically difficult to assess the oxidatively damaged DNA in different internal organs. Therefore, the present study was aimed to evaluate the extent of oxidative stress-induced DNA damage in different organs with the progression of diabetes. Diabetic and control Sprague Dawley rats were sacrificed in time-dependent manner and the lung, liver, heart, aorta, kidney, pancreas and peripheral blood lymphocytes (PBL) were analyzed for both alkaline and modified comet assay with endonuclease-III (Endo III) and formamidopyrimidine-DNA glycosylase (FPG) (hereafter called modified comet assay) for the detection of oxidative DNA damage. The statistically significant increase in olive tail moment (OTM) was found in all the tested tissues. The extent of DNA damage was increased with the progression of diabetes as revealed by the parameter of OTM in alkaline and modified comet assay. Further, the positive correlations were observed between OTM of the lung, liver, heart, aorta, kidney and pancreas with PBL of diabetic rat in the alkaline and modified comet assay. Moreover, significant increase in the 8-oxodG positive nuclei in the lung, liver, heart, aorta, kidney and pancreas was observed in 4th and 8th week diabetic rat as compared to control. Results of the present study clearly indicated the suitability of alkaline and modified comet assay for the detection of multi-organ oxidative DNA damage in streptozotocin (STZ)-induced diabetic rat and showed that damaged DNA of PBL can be used as a suitable biomarker to assess the internal organs response to DNA damage in diabetes.
机译:在糖尿病条件下增加的活性氧的产生强调了不同组织中较高的氧化损伤DNA。但是,实际上很难评估不同内部器官中被氧化破坏的DNA。因此,本研究旨在评估随着糖尿病的发展,氧化应激诱导的不同器官DNA损伤的程度。以时间依赖性方式处死糖尿病和对照Sprague Dawley大鼠,并使用核酸内切酶-III(Endo III)分析肺,肝,心脏,主动脉,肾脏,胰腺和外周血淋巴细胞(PBL)的碱性和改良彗星试验和甲酰胺基嘧啶-DNA糖基化酶(FPG)(以下称为修饰彗星试验)用于检测氧化性DNA损伤。在所有测试的组织中,发现橄榄尾矩(OTM)的统计显着增加。 DNA损伤的程度随着糖尿病的进展而增加,如碱性和改良彗星试验中OTM的参数所揭示。此外,在碱性和改良彗星试验中,观察到肺,肝,心脏,主动脉,肾脏和胰腺的OTM与糖尿病大鼠的PBL之间呈正相关。此外,与对照组相比,在第4周和第8周的糖尿病大鼠中,观察到肺,肝,心脏,主动脉,肾脏和胰腺中8-oxodG阳性核的显着增加。本研究的结果清楚地表明,碱性和改良彗星试验适用于检测链脲佐菌素(STZ)诱导的糖尿病大鼠中多器官氧化DNA损伤,并表明PBL的损伤DNA可作为评估其的生物标志物。糖尿病引起的内脏器官对DNA损伤的反应。

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