强碱脱蛋白能否替代碱性单细胞凝胶电泳（彗星试验）中的标准裂解步骤（pH>13）？

Could a strong alkali deproteinization replace the standard lysis step in alkaline single cell gel electrophoresis (comet) assay (pH>13)?

作者信息

Vivek Kumar P R, Cheriyan V D, Seshadri M

机构信息

Low Level Radiation Research Laboratory, Radiation Biology and Health Science Division, Bhabha Atomic Research Centre, Kollam 691 001, Kerala, India.

出版信息

Mutat Res. 2009 Aug;678(1):65-70. doi: 10.1016/j.mrgentox.2009.06.007. Epub 2009 Jun 27.

DOI:10.1016/j.mrgentox.2009.06.007

PMID:19563911

Abstract

The alkaline version of single cell gel electrophoresis (comet) assay is widely used for evaluating DNA damage at the individual cell level. The standard alkaline method of the comet assay involves deproteinization of cells embedded in agarose gel using a high salt-detergent lysis buffer, followed by denaturation of DNA and electrophoresis using a strong alkali at pH>13 [N.P. Singh, M.T. McCoy, R.R. Tice, E.L. Schneider, A simple technique for quantitation of low levels of DNA damage in individual cells, Exp. Cell. Res. 175 (1988) 184-191]. However, a recent report showed that a strong alkali treatment results in simultaneous deproteinization of cells and denaturation of genomic DNA [P. Sestili, C. Martinelli, V. Stocchi, The fast halo assay: an improved method to quantify genomic DNA strand breakage at the single cell-level, Mutat. Res. 607 (2006) 205-214]. This study was carried out to test whether the strong alkali deproteinization of cells could replace the high salt-detergent lysis step used in the standard method of the alkaline comet assay. Peripheral blood lymphocytes from 3 healthy individuals were irradiated with gamma rays at doses varying between 0 and 10 Gy. Following irradiation, the comet assay was performed according to the standard alkaline method (pH>13) and a modified method. In the modified method, agarose embedded cells were treated with a strong alkali (0.3M NaOH, 0.02 M Trizma and 1mM EDTA, pH>13) for 20 min to allow deproteinization of cells and denaturation of DNA. This was followed by electrophoresis using the same alkali solution to obtain comets. DNA damage expressed in terms of comet tail length, percentage of DNA in comet tail and tail moment obtained by the standard alkaline method and the modified method were compared. In both methods, DNA damage showed a good correlation with the dose of gamma ray. The results indicate a satisfactory sensitivity of the modified method in detecting radiation-induced DNA damage in human peripheral blood lymphocytes.

摘要

单细胞凝胶电泳（彗星试验）的碱性版本被广泛用于在单个细胞水平评估DNA损伤。彗星试验的标准碱性方法包括使用高盐去污剂裂解缓冲液对包埋在琼脂糖凝胶中的细胞进行脱蛋白处理，随后使DNA变性，并在pH>13的强碱条件下进行电泳[N.P.辛格、M.T.麦科伊、R.R.蒂斯、E.L.施耐德，一种定量单个细胞中低水平DNA损伤的简单技术，《实验细胞研究》175（1988）184 - 191]。然而，最近一份报告显示，强碱处理会导致细胞同时脱蛋白和基因组DNA变性[P.塞斯蒂利、C.马丁内利、V.斯托奇，快速晕圈试验：一种在单细胞水平定量基因组DNA链断裂的改进方法，《突变研究》607（2006）205 - 214]。本研究旨在测试细胞的强碱脱蛋白处理是否可以替代碱性彗星试验标准方法中使用的高盐去污剂裂解步骤。对3名健康个体的外周血淋巴细胞进行0至10 Gy不同剂量的γ射线照射。照射后，按照标准碱性方法（pH>13）和改良方法进行彗星试验。在改良方法中，用强碱（0.3M NaOH、0.02M三羟甲基氨基甲烷和1mM EDTA，pH>13）处理包埋在琼脂糖中的细胞20分钟，以使细胞脱蛋白和DNA变性。随后用相同的碱溶液进行电泳以获得彗星图像。比较了通过标准碱性方法和改良方法获得的以彗星尾长、彗星尾中DNA百分比和尾矩表示的DNA损伤。在两种方法中，DNA损伤均与γ射线剂量呈现良好的相关性。结果表明改良方法在检测人外周血淋巴细胞辐射诱导的DNA损伤方面具有令人满意的灵敏度。