Effects of selected pesticides, metals and organometallics on development of blue crab (Callinectes sapidus) embryos

被引:14
作者
Lee, R [1 ]
Oshima, Y
机构
[1] Skidaway Inst Oceanog, Savannah, GA 31411 USA
[2] Kyushu Univ, Dept Fisheries, Fukuoka 812, Japan
关键词
D O I
10.1016/S0141-1136(97)00072-X
中图分类号
X [环境科学、安全科学];
学科分类号
08 ; 0830 ;
摘要
Blue crab embryos develop in egg sacs (nine stages) for 14 to 20 days after which they 'hatch' from the egg sacs into a swimming zoea stage (stage 10). Until they emerge from the egg sacs, embryos depend on lipids and lipovitellin stored within the eggs. A number of organic and inorganic toxicants,cere found to inhibit hatching. For example, at a fenvalerate concentration of 3.2 mu g l(-1) only, 50% of embryos hatched, while 90 to 95% of the controls hatched. Pesticides, including chlorphyrifos, cypermethrin, fenvalerate and diflubenzuron on, inhibited hatching at concentrations ranging fi om 1.8 to 5.9 mu g l(-1) (EC(50)s). The most toxic of the metals tested was mercuric chloride and the most toxic of all compounds tested was methyl mercury. The addition of mercuric chloride at concentrations above 4.0 mu g l(-1) to stage three embryos resulted in stage 7 embryos with no heart beat. Abnormal eye spots were produced by exposure to high concentrations of metals, Time lapse video with a high definition digital camera was used to follow and document both normal and abnormal developments of the eyes, hearts and hatching process. In addition, the time lapse video was used to determine the tints of the first appearance of a pulsating heart and eye spots. The advantages of crab embryos as a test for development toxicants include: (1) availability of embryos for most of the year: (2) sensitivity of embryos to toxicants; (3) nutrients for developing embryo are obtained from yolk so no external feeding is necessary, (4) good reproducibility of the assay; (5) use of culture plates allows the testing of many, toxicants and concentrations in a small space and at low cost, (6) tests take from 2 to 6 days depending on stage used at the beginning of the assay; (7) obvious end point of the assay, i.e. emergence of zoea front egg sac. (C) 1998 Elsevier Science Ltd. All rights reserved.
引用
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页码:479 / 482
页数:4
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