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用苯并[a]芘或其二醇环氧化物处理后,小鼠组织和人类白细胞中DNA加合物的免疫细胞化学可视化。一种定量方法。

Immunocytochemical visualization of DNA adducts in mouse tissues and human white blood cells following treatment with benzo[a]pyrene or its diol epoxide. A quantitative approach.

作者信息

van Schooten F J, Hillebrand M J, Scherer E, den Engelse L, Kriek E

机构信息

Division of Chemical Carcinogenesis, The Netherlands Cancer Institute, Amsterdam.

出版信息

Carcinogenesis. 1991 Mar;12(3):427-33. doi: 10.1093/carcin/12.3.427.

DOI:10.1093/carcin/12.3.427
PMID:1901249
Abstract

The formation and stability of benzo[a]pyrene DNA adducts were studied in tissues of BALB/c mice exposed to benzo[a]pyrene (B[a]P). The DNA adducts were visualized with an immunocytochemical peroxidase staining technique using an antiserum specific for the major B[a]P-derived adduct in DNA [(+/-)trans-7,8-dihydroxy-anti-9,10-epoxy-7,8,9,10- tetrahydrobenzo[a]pyrene (BPDE-N2-dG)]. The nuclear staining density was measured by microdensitometry. When mice were treated with an increasing dose of B[a]P the nuclear staining increased in the tissues studied (lung, heart and kidney). A linear relationship was found between the immunocytochemical nuclear staining signal and the actual DNA adduct level in the lung as measured by 32P-postlabeling. Maximum adduct formation was found 5 days after a single i.p. injection of B[a]P. Adduct levels decreased gradually after 7 days, but even after 61 days a slight specific staining was still present, suggesting that not all adducts had disappeared at that time. As judged from the disappearance of [3H]thymidine from prelabeled DNA the loss of adducts from the lung was not a result of DNA repair but one of cell turnover. In human white blood cells B[a]P-derived adducts could be detected after in vitro incubation with the reactive metabolite of B[a]P (BPDE). Dose-response studies demonstrated a positive relationship between BPDE-DNA adduct formation, the immunocytochemical staining signal and the BPDE concentration in the culture medium.

摘要

在暴露于苯并[a]芘(B[a]P)的BALB/c小鼠组织中研究了苯并[a]芘DNA加合物的形成和稳定性。使用针对DNA中主要的B[a]P衍生加合物[(+/-)反式-7,8-二羟基-反式-9,10-环氧-7,8,9,10-四氢苯并[a]芘(BPDE-N2-dG)]的抗血清,通过免疫细胞化学过氧化物酶染色技术使DNA加合物可视化。通过显微密度测定法测量核染色密度。当用递增剂量的B[a]P处理小鼠时,在所研究的组织(肺、心脏和肾脏)中核染色增加。通过32P后标记法测量发现,肺中免疫细胞化学核染色信号与实际DNA加合物水平之间存在线性关系。在单次腹腔注射B[a]P后5天发现加合物形成达到最大值。7天后加合物水平逐渐下降,但即使在61天后仍存在轻微的特异性染色,这表明此时并非所有加合物都已消失。根据预标记DNA中[3H]胸苷的消失判断,肺中加合物的损失不是DNA修复的结果,而是细胞更新的结果之一。在人白细胞中,与B[a]P的活性代谢物(BPDE)体外孵育后可检测到B[a]P衍生的加合物。剂量反应研究表明,BPDE-DNA加合物形成、免疫细胞化学染色信号与培养基中BPDE浓度之间呈正相关。

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