Literature DB >> 7589245

Sizing highly fragmented DNA in individual apoptotic cells using the comet assay and a DNA crosslinking agent.

P L Olive1, J P Banáth.   

Abstract

TK6 human B lymphoblast cells exposed to ionizing radiation undergo apoptosis in a time and dose-dependent manner. The resulting highly fragmented DNA is easily detected using the comet assay, a sensitive microscopic gel electrophoresis method capable of measuring DNA strand breaks in individual cells. The degree of DNA fragmentation may be indicative of different stages in the fragmentation process, responses to different agents, and/or cell type-dependent differences. In an effort to determine the number of breaks present in each apoptotic cell, we first applied a DNA-crosslinking agent, mechlorethamine, to TK6 cells containing a known number of DNA double-strand breaks produced by X rays. As the concentration of mechlorethamine increased, crosslinked DNA was less able to migrate during gel electrophoresis. Exposure of TK6 cells to 5 microM mechlorethamine prior to irradiation with 20 Gy was sufficient to "hide" the presence of these breaks by preventing DNA from migrating during electrophoresis. However, in apoptotic TK6 cells, it was necessary to apply a dose of mechlorethamine several times higher in order to produce a similar degree of inhibition of DNA migration. Calibrations using either the alkaline or neutral comet assays indicate that the average DNA fragment size in apoptotic TK6 cells is about 50 kb. Even in cells containing only 10-20% of the original amount of DNA, the remaining fragments still averaged about 50 kb, indicating that fragmentation to much smaller sizes occurs in some parts of the genome before others. When Chinese hamster V79 cells were exposed to hyperthermia (45 degrees C for 20 min), necrosis was induced over a period of several days. The size of DNA fragments in these cells was considerably larger (200-400 kb) and heterogeneity in appearance of comets was larger than observed for TK6 cells. This crosslinking method may be useful in discriminating cells dying by apoptosis from cells damaged or dying by other mechanisms.

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Year:  1995        PMID: 7589245     DOI: 10.1006/excr.1995.1348

Source DB:  PubMed          Journal:  Exp Cell Res        ISSN: 0014-4827            Impact factor:   3.905


  16 in total

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3.  Transcriptional responses and embryotoxic effects induced by pyrene and methylpyrene in Japanese medaka (Oryzias latipes) early life stages exposed to spiked sediments.

Authors:  Iris Barjhoux; Jérôme Cachot; Patrice Gonzalez; Hélène Budzinski; Karyn Le Menach; Laure Landi; Bénédicte Morin; Magalie Baudrimont
Journal:  Environ Sci Pollut Res Int       Date:  2014-04-23       Impact factor: 4.223

4.  The radiomimetic enediyne, 20'-deschloro-C-1027 induces inter-strand DNA crosslinks in hypoxic cells and overcomes cytotoxic radioresistance.

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5.  Health indicators and contaminant levels of a critically endangered species in the Gironde estuary, the European sturgeon.

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6.  Induction of DNA-protein cross-links by Hippophae rhamnoides: implications in radioprotection and cytotoxicity.

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7.  Vitamin C and quercetin modulate DNA-damaging effect of N-methyl-N'-nitro-N-nitrosoguanidine (MNNG).

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8.  Radiofrequency electromagnetic fields (UMTS, 1,950 MHz) induce genotoxic effects in vitro in human fibroblasts but not in lymphocytes.

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Review 9.  Clinical value of DNA fragmentation evaluation tests under ART treatments.

Authors:  Ilkay Şafak Tavukçuoğlu; Tahani Al-Azawi; Amir Afshin Khaki; Arash Khaki; Ahmed Khalil; Safaa Al-Hasani
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10.  Estimates of DNA strand breakage in bottlenose dolphin (Tursiops truncatus) leukocytes measured with the Comet and DNA diffusion assays.

Authors:  Adriana Díaz; Sandra Carro; Livia Santiago; Juan Estévez; Celia Guevara; Miriam Blanco; Laima Sánchez; Liena Sánchez; Nirka López; Danilo Cruz; Ronar López; Elizabeth B Cuetara; Jorge Luis Fuentes
Journal:  Genet Mol Biol       Date:  2009-03-06       Impact factor: 1.771

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