Literature DB >> 8700178

Interlaboratory validation of a new assay for DNA-protein crosslinks.

M Costa1, A Zhitkovich, M Gargas, D Paustenbach, B Finley, J Kuykendall, R Billings, T J Carlson, K Wetterhahn, J Xu, S Patierno, M Bogdanffy.   

Abstract

In 1992, a simple and sensitive assay for detecting DNA-protein crosslinks was developed [1]. In an effort to facilitate the greater use of the assay, a number of studies were conducted to evaluate its reliability and reproducibility. During this work, the assay was used to assess whether various metals and other compounds could induce crosslinks in cultured human lymphocytes (Epstein-Barr virus-transformed Burkitt's Lymphoma cell line). Potassium permanganate, mercury chloride, lead nitrate, magnesium perchlorate, aluminum chloride, and cadmium chloride did not induce DNA-protein crosslinks at either cytotoxic or non-cytotoxic levels. Copper sulfate, arsenic trioxide, and potassium chromate induced DNA-protein crosslinks only at cytotoxic concentrations. Acute lethality of the cells was assessed immediately after exposure to metals by trypan blue exclusion while long-term lethality was assessed by cell proliferation and trypan blue exclusion following an incubation period of 5 days after exposure to the metal compound. All metals exhibited more toxicity in the long-term lethality assay compared to the short-term assay. The cultured human lymphocytes treated with various doses of lead acetate, cadmium chloride, arsenic trioxide and copper sulfate, as well as cis-platinum and chromate, were sent to four different laboratories to compare the reliability and reproducibility of the DNA-protein crosslink assay. Depending on the chemical studied, there were quantitative differences in the results observed among the various laboratories using the assay. However, all laboratories generally showed that cis-platinum, chromate, arsenic trioxide and copper sulfate induced DNA-protein crosslinks at levels that produced acute cytotoxicity, whereas cadmium chloride and lead acetate did not.

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Year:  1996        PMID: 8700178     DOI: 10.1016/s0165-1218(96)90043-9

Source DB:  PubMed          Journal:  Mutat Res        ISSN: 0027-5107            Impact factor:   2.433


  14 in total

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3.  Roles of Bacillus subtilis RecA, Nucleotide Excision Repair, and Translesion Synthesis Polymerases in Counteracting Cr(VI)-Promoted DNA Damage.

Authors:  Fernando Santos-Escobar; Hilda C Leyva-Sánchez; Norma Ramírez-Ramírez; Armando Obregón-Herrera; Mario Pedraza-Reyes
Journal:  J Bacteriol       Date:  2019-03-26       Impact factor: 3.490

4.  The impact of FANCD2 deficiency on formaldehyde-induced toxicity in human lymphoblastoid cell lines.

Authors:  Xuefeng Ren; Zhiying Ji; Cliona M McHale; Jessica Yuh; Jessica Bersonda; Maycky Tang; Martyn T Smith; Luoping Zhang
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Review 5.  DNA-protein crosslink formation by endogenous aldehydes and AP sites.

Authors:  Jun Nakamura; Mai Nakamura
Journal:  DNA Repair (Amst)       Date:  2020-02-10

6.  A Surge of DNA Damage Links Transcriptional Reprogramming and Hematopoietic Deficit in Fanconi Anemia.

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Journal:  Mol Cell       Date:  2020-12-17       Impact factor: 17.970

7.  Detection of DNA-protein crosslinks (DPCs) by novel direct fluorescence labeling methods: distinct stabilities of aldehyde and radiation-induced DPCs.

Authors:  Mahmoud I Shoulkamy; Toshiaki Nakano; Makiko Ohshima; Ryoichi Hirayama; Akiko Uzawa; Yoshiya Furusawa; Hiroshi Ide
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8.  DNA-protein cross-links as a biomarker of Cr(VI) exposure.

Authors:  D J Paustenbach; B L Finley
Journal:  Environ Health Perspect       Date:  1999-10       Impact factor: 9.031

Review 9.  Oxidative stress in toxicology: established mammalian and emerging piscine model systems.

Authors:  K A Kelly; C M Havrilla; T C Brady; K H Abramo; E D Levin
Journal:  Environ Health Perspect       Date:  1998-07       Impact factor: 9.031

10.  Utilization of DNA-protein cross-links as a biomarker of chromium exposure.

Authors:  A Zhitkovich; V Voitkun; T Kluz; M Costa
Journal:  Environ Health Perspect       Date:  1998-08       Impact factor: 9.031

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