酚类化合物对不同组织细胞DNA损伤的研究

应用单细胞凝胶电泳技术 ,研究了酚类化合物对不同组织细胞DNA的损伤 .试验结果表明 ,酚类化合物均能引起不同组织细胞不同程度的DNA损伤 ,并呈现剂量效应关系 .其高剂量组与对照组相比 ,均有极显著性差异 (P <0 0 1 ) .不同组织细胞对同一种药物呈现出不同的敏感性 .酚类化合物遗传毒性效应与其结构密切相关     

Integral assessment of estrogenic potentials in sediment-associated samples

Background, aim, and scope  The enzyme-linked receptor assay (ELRA) detects estrogenic and anti-estrogenic effects at the molecular level of receptor binding and is a useful tool for the integrative assessment of ecotoxicological potentials caused by hormonally active agents (HAA) and endocrine disrupting compounds (EDC). The main advantage of the ELRA is its high sample throughput and its robustness against cytotoxicity and microbial contamination. After a methodological adaptation to salinity of the ELRA, according to the first part of this study, which increased its salinity tolerance and sensitivity for 17-β-estradiol, the optimised ELRA was used to investigate 13 native sediments characterised by different levels of salinity and chemical contamination. The applicability of the ELRA for routine analysis in environmental assessment was evaluated. Salinity is often a critical factor for bioassays in ecotoxicological sediment assessment. Therefore, salinity of the samples was additionally adjusted to different levels to characterise its influence on elution and binding processes of receptor-binding substances. Materials and methods  The ELRA was carried out with the human estrogen receptor α (ER) in a 96-well microplate format using the experimental setup known from the competitive immunoassay based on ligand–protein interaction. It is an important improvement that a physiologically relevant receptor was used as a linking protein instead of an antibody. The microplates were coated with a 17-β-estradiol-BSA conjugate, and dilution series of estradiol and of native sediment samples were added and incubated with the ER. After a washing step, a biotinylated mouse anti-ER antibody was added to each well. Receptor binding to estradiol, agonistic and antagonistic receptor binding, were determined by a streptavidin-POD-biotin complex with subsequent measurement of the peroxidase activity at the wavelength of 450 nm using a commercial ELISA multiplate reader. The sediment elutriates and pore water samples of sediments were tested in a dilution series to evaluate at which dilution step the receptor-binding potential ends. In the elution process (see Section 2.1 to 2.2), a method was developed to adjust the salinity to the levels of the reference testings, which offers an appropriate option to adjust the salinity in both directions. Statistical evaluation was made with a combination of the Mann–Whitney U test and the pT-method. Results  This part of the study characterised the environmental factor ‘salinity’ for prospective applications of the ELRA. Using reference substances such as 17-β-estradiol, the ELRA showed sigmoid concentration-effect relations over a broad range from 0.05 μg/l to 100 μg/l under physiological conditions. After methodological optimisation, both sensitivity and tolerance of the assay against salinity could be significantly raised, and the ELRA became applicable under salinity conditions up to concentrations of 20.5‰. The mean relative inter-test error (n = 3) was around 11% with reference substances and below 5% for single sediments elutriates in three replicates each. For sediment testings, the pore water and different salinity-adjusted elutriates of 13 sediments were used. A clear differentiation of the receptor-binding potential could be reached by application of the pT-method. Thereby, pT-values from one to six could be assigned to the sediments, and the deviation caused by the different salinity conditions was one pT-value. The mean standard deviation in the salinity adaptation procedure of the elutriates was below 5%. Discussion  Although the ELRA has already been used for assessments of wastewater, sludge and soil, its applicability for samples to different salinity levels has not been investigated so far. Even if the ELRA is not as sensitive as the E-screen or the YES-assay, with regard to reference substances like 17-β-estradiol, it is a very useful tool for pre-screening, because it is able to integrate both estrogenic as well as anti-estrogenic receptor-binding effects. According to the results of sediment testing, and given the integrative power to detect different directions of effects, the ELRA shows sufficient sensitivity and salinity tolerance to discriminate receptor-binding potentials in environmental samples. Conclusions  The optimised ELRA assay is a fast, cost-effective, reliable and highly reproducible tool that can be used for high-throughput screening in a microplate format in detecting both estrogenic and anti-estrogenic effects. Additionally, the ELRA is robust against microbial contaminations, and is not susceptible towards cytotoxic interferences like the common cell-culture methods. The general applicability and sufficient sensitivity of the ELRA was shown in freshwater environments. Marine and brackish samples can be measured up to salinity levels of 20.5‰. Recommendations and perspectives  In view of the proven sensitivity, functionality and the fastness of the ELRA, it is recommendable to standardise the test method. At the moment, no adequate in vitro test procedure exists which is standardised to DIN or ISO levels. The E-screen and the yeast estrogen/androgen screens (YES/YAS) sometimes underlie strong cytotoxic effects, as reported in the first part of this study. Further development of an ELRA assay using human androgen receptors appears to be very promising to gain information about androgenic and anti-androgenic effects, too. This would offer a possibility to use the ELRA as a fast and reliable pre-screening tool for the detection of endocrine potentials, thus minimising time and cost-expensive animal experiments.     

发酵木糖产乙醇酵母菌的选育及其发酵特性

为了提高木质纤维素水解产物中戊糖的利用率,采用划线分离法、TTC(2,3,5-氯代三苯基四氮唑)法从多年生乔木下方土壤及林中朽木中筛选出4株能利用木糖产乙醇的酵母菌。其中1株产乙醇能力较佳,其发酵条件为150 r/m in、30℃、接种量12%、初始pH值6.0时,乙醇产量达4.88g/L,木糖转化率达理论值的24.3%。经初步鉴定,该菌为假单丝酵母属(Cand ida)。研究还表明,该菌株在pH 6.5,温度40℃仍能很好地发酵木糖产乙醇。     

甲基营养型酵母表达载体系统研究进展

酵母作为生产真核异源蛋白的宿主菌 ,具备了易于分子遗传操作 ,原核微生物的生长性质及真核蛋白的翻译后加工修饰等特点 .其中Ｓａｃｃｈａｒｏｍｙｃｅｓｃｅｒｅｖｉｓｉａｅ (酿酒酵母 )是第一个作为异源蛋白基因表达系统并加以应用的酵母 .人们认为Ｓ .ｃｅｒｅｖｉｓｉａｅ并非表达外源基因的最理想的酵母宿主菌 .在一群优于Ｓ .ｃｅｒｅｖｉｓｉａｅ的表达菌中 ,甲基营养型酵母Ｐｉｃｈｉａｐａｓｔｏｒｉｓ研究得最多 ,最具应用潜力 .在 2 0世纪 70年代期间 ,Ｐ .ｐａｓｔｏｒｉｓ是单细胞蛋白 (Ｓｉｎｇｌｅ ｃｅｌｌｐｒｏｔｅｉｎ…     

核受体超家族及其酵母双杂交检测技术

环境污染物的内分泌干扰问题近年来引起了极大的关注,大量研究证实:核受体是内分泌干扰的重要作用位点.论文在总结国内外相关研究基础上,对生物体内核受体超家族的组成、结构特征、作用模式进行了概括总结;对环境内分泌干扰物干扰核受体超家族最新研究进展给予了评述;对酵母双杂交检测技术的原理及其在核受体超家族和环境内分泌干扰效应研究中的应用进行了探讨,指出应将酵母双杂交检测技术与核受体超家族研究相结合,建立成组重组核受体基因双杂交酵母体系,应用于多种内分泌干扰效应和作用机制的系统研究.     

澳门城市垃圾焚烧底灰的重金属淋溶及其遗传毒性评价

应用美国国家环境保护局推荐的毒性特性溶出程序(toxicitycharacteristicleachingprocedure,TCLP),以及ICP-MS和ICP-AES技术研究了澳门城市垃圾焚烧底灰中重金属的淋溶,并结合蚕豆根尖微核试验评价了其潜在的生态与健康风险.结果显示,该底灰淋溶出来的重金属元素:铝(Al)、锰(Mn)、钴(Co)和汞(Hg)的浓度低于0.01mg·L-1,铁(Fe)、铜(Cu)和钼(Mo)的浓度低于0.1mg·L-1,而铬(Cr)、锌(Zn)、硒(Se)、锶(Sr)、钡(Ba)和铯(Cs)的浓度在0.11mg·L-1￣2.19mg·L-1之间.需要注意的是淋溶液中铅(Pb)的浓度异常高,最高可达19.06mg·L-1,超过了美国相关标准的上限(5mg·L-1);对比不同条件下底灰中重金属的淋溶情况,表明溶解作用和淋溶液的pH值是影响其淋溶的2个重要因素.蚕豆根尖微核试验显示各淋溶液处理组根尖细胞微核率明显升高,与阴性对照组相比具有显著性差异(p<0.05),表明各淋溶液具有遗传毒性;随着淋溶液中重金属浓度的增加,蚕豆根尖细胞所表现出来的毒性效应增强,表明重金属是淋溶液具有遗传毒性的重要原因.