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The degradation process of acephate in aqueous solution with OH and eaq? produced by 60Co-γ irradiation and electron pulse radiolysis was studied in the present paper. In the aqueous solution, acephate reacted with eaq? and transformed to transient species which can absorb weakly in the wavelength range of 300–400?nm and decay very fast. According to the decay of hydrated electron, the reaction rate constant of eaq? and acephate is (3.51?±?0.076)?×?109?dm3·mol?1·s?1. The transient species produced in the reaction of OH and acephate do not distinctly absorb the light in the wavelength range of 300–700?nm, so the decay and kinetics of the transient species cannot determinedirectly. The competing reaction of KSCN oracephate with OH were studied to obtain the reaction rate constant of OH and acephate, which is (9.1?±?0.11)?×?108?dm3·mol?1·s?1. Although acetylamide and inorganic ions were determined in the products of the reaction of acephate with OH or eaq?, the concentration of inorganic ions in the products of the reaction of acephate with OH is higher than that in the product of the reaction of acephate with eaq?. Moreover, there were sulfide in the products of the reaction of acephatewith eaq?. The degradation pathways of acephate by OH and eaq? were also proposed based on the products from GC-MS.  相似文献   
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应用3天种群增长实验方法,在(25±1)℃、无光照、以3.0×106 cells/mL的斜生栅藻为轮虫的食物等条件下,研究了亚致死浓度(0.01、0.1、1.0、10.0、100.0、1000.0和10000.0 µg/L)的甲胺磷和乙酰甲胺磷对萼花臂尾轮虫实验种群动态的影响。结果显示,甲胺磷和乙酰甲胺磷显著地影响萼花臂尾轮虫的种群增长率、混交雌体数与非混交雌体数的比值和混交率。甲胺磷显著地影响萼花臂尾轮虫种群中的带卵雌体数与不带卵雌体数的比值,但乙酰甲胺磷对其无显著的影响。和对照组相比,浓度为100.0 µg/L 的甲胺磷和浓度为1.0-10,000.0 µg/L 的乙酰甲胺磷均使轮虫种群增长率显著增大,而浓度为1000.0 µg/L和10000.0 µg/L的甲胺磷却使之显著减小;1000.0 µg/L 的甲胺磷使轮虫种群中的带卵雌体数与不带卵雌体数的比值显著上升,0.1 µg/L的甲胺磷和10.0-10000.0 µg/L的乙酰甲胺磷均使轮虫种群中的混交雌体数与非混交雌体数的比值显著上升,0.1µg/L 的甲胺磷和10 µg/L的乙酰甲胺磷均使轮虫的混交率显著增大,10.0-0000.0 µg/L 的乙酰甲胺磷使轮虫休眠卵产量显著提高。上述结果表明,亚致死浓度的甲胺磷和乙酰甲胺磷对萼花臂尾轮虫实验种群动态具有显著的影响。  相似文献   
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The organophosphorous insecticide acephate was tested for its ability to induce in vitro cytogenetic effect in human peripheral lymphocytes by using the chromosomal aberrations (CAs), sister chromatid exchange (SCE) and micronuclei (MN) assay. The level of nuclear DNA damage of acephate was evaluated by using the comet assay. Concentrations of 12.5, 25, 50, 100 and 200 μg mL−1 of acephate were used. All concentrations of acephate induced significant increase in the frequency of CAs and in the formation of MN dose dependently (r = 0.92 at 24 h, r = 0.95 at 48 h for CAs, r = 0.87 for MN). A significant increase was observed in induction of SCE at 50, 100 and 200 μg mL−1 concentrations during 24 h treatment and at all concentrations (except 12.5 μg mL−1) during 48 h treatment period in a dose-dependent manner (r = 0.84 at 24 h, r = 0.88 at 48 h). Acephate did not affect the replicative index and cytokinesis-block proliferation index (CBPI). However, it significantly decreased the mitotic index at all three highest concentrations (50, 100, 200 μg mL−1) for 24 h treatment and at all concentrations (except 12.5 μg mL−1) for 48 h treatment, dose-dependently (r = 0.94 at 24 h, r = 0.92 at 48 h). A significant increase in mean comet tail length was observed at 100 and 200 μg mL−1 concentrations compared with negative control in a concentration-dependent manner (r = 0.94). The mean comet tail intensity was significantly increased at only 200 μg mL−1 concentration. The present results indicate that acephate is a clastogenic, cytotoxic agent and it causes DNA damage at high concentrations in human lymphocytes in culture.  相似文献   
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