Zakour H R, Landolt M L, Kocan R M
Basic Life Sci. 1984;29 Pt B:493-508. doi: 10.1007/978-1-4684-4892-4_1.
The genotoxicity of environmental contaminants and test compounds to aquatic and marine fish has primarily been assessed by in vivo techniques that require sacrifice of the test organism for analysis. The major objective of this research was to develop an in vitro sister chromatid exchange (SCE) assay which would utilize cultured peripheral blood leukocytes (PBLs) of a coldwater marine fish species. Use of PBLs in cytogenetic genotoxicity tests has several advantages, the major one being that the experimental fish need not be sacrificed for sample collection. In addition, this nondestructive method of tissue collection permits the investigator to take multiple samples from a single individual and thereby allows the use of an individual as its own control and to monitor its SCE frequency over time. A suitable in vitro culture method for fish PBLs was a prerequisite for cytogenetic analysis of this tissue. The in vitro culture conditions necessary to provide a sufficient number of dividing cells for performance of the SCE assay were established in our laboratory for the PBLs of the Pacific staghorn sculpin (Leptocottus armatus), a common bottom-dwelling Puget Sound fish. The major components of this culture system are heparinized whole blood, fetal bovine serum-supplemented enriched tissue culture medium (RPMI 1640), purified protein derivative of tuberculin as a mitogen, and an incubation temperature of 13.5 degrees C. This in vitro PBL culture system is unique because it involves cultured blood cells from a coldwater marine fish species. Using this culture method, SCE induction was investigated in Pacific staghorn sculpin PBLs which had been exposed in vitro to N-methyl-N'-nitro-N-nitrosoguanidine (MNNG), a known direct-acting inducer of SCEs. Cultured cells exposed in vitro responded to MNNG in a dose-related manner in regard to SCE induction, and the frequency of "outlier" cells increased at the higher concentrations of MNNG. With further development, this technique may be adaptable for use with in vivo genotoxicity studies and provide information concerning the induction and persistence of chemically induced SCEs in fish. This PBL/SCE assay may also be a feasible assessment tool for detecting exposure of marine fish to genotoxic environmental contaminants in laboratory and field situations.
环境污染物和受试化合物对水生及海洋鱼类的遗传毒性,主要通过体内技术进行评估,而这些技术需要处死受试生物以进行分析。本研究的主要目的是开发一种体外姐妹染色单体交换(SCE)试验,该试验将利用一种冷水海洋鱼类的培养外周血白细胞(PBLs)。在细胞遗传毒性试验中使用PBLs有几个优点,主要优点之一是无需处死实验鱼来采集样本。此外,这种非破坏性的组织采集方法使研究者能够从单个个体采集多个样本,从而可以将个体自身作为对照,并随时间监测其SCE频率。适合鱼类PBLs的体外培养方法是对该组织进行细胞遗传学分析的前提条件。我们实验室为太平洋鹿角杜父鱼(Leptocottus armatus,普吉特海湾一种常见的底栖鱼类)的PBLs建立了体外培养条件,以提供足够数量的分裂细胞用于进行SCE试验。该培养系统的主要成分包括肝素化全血、添加胎牛血清的富集组织培养基(RPMI 1640)、作为促有丝分裂原的结核菌素纯蛋白衍生物以及13.5摄氏度的孵育温度。这种体外PBL培养系统很独特,因为它涉及来自冷水海洋鱼类的培养血细胞。使用这种培养方法,研究了体外暴露于N-甲基-N'-硝基-N-亚硝基胍(MNNG,一种已知的SCE直接诱导剂)的太平洋鹿角杜父鱼PBLs中的SCE诱导情况。体外培养的细胞在SCE诱导方面对MNNG呈剂量相关反应,并且在较高浓度的MNNG下“异常值”细胞的频率增加。随着进一步发展,该技术可能适用于体内遗传毒性研究,并提供有关化学诱导的SCEs在鱼类中的诱导和持久性的信息。这种PBL/SCE试验也可能是在实验室和野外情况下检测海洋鱼类暴露于遗传毒性环境污染物的一种可行评估工具。
