生物阴极式碳纸隔膜微生物燃料电池的反硝化和产电性能

为了探讨生物阴极式廉价隔膜微生物燃料电池(microbial fuel cell,MFC)的基本性能,首先以生物反硝化作用为基础构建了生物阴极MFC,并进一步以涂布聚四氟乙烯(PTFE)的廉价碳纸代替昂贵的质子交换膜(PEM)构建碳纸隔膜生物阴极式MFC。研究结果显示,对于生物阴极式MFC,阴极室中最适宜反硝化细菌生长的NO-3-N浓度为99.2 mg/L,此时输出电压最高可达0.11 V,1 h内NO-3-N的去除率达到80.0%,COD去除率为62.8%;以涂PTFE的碳纸代替PEM的生物阴极式MFC与有PEM的MFC最高输出电压基本一致(均达到0.22 V,外阻500Ω),但碳纸隔膜MFC的产电更稳定。结果验证了廉价隔膜生物阴极式MFC的可行性,并为其应用于污水脱氮奠定基础。     

阴极液及底物浓度对AFB-MFC同步废水处理及产电性能影响

为了提高厌氧流化床微生物燃料电池（AFB-MFC）的性能，并为双室MFC寻找价廉、易得、无污染的阴极液，在曝气量16～24 L/h、温度（35±2）℃、回流量10.2 L/h、阴极底边距阴极室内底部17.3 cm、外电阻250 Ω、水力停留时间（HRT）14.0～14.9 h以及进水pH 7.81～8.37下，研究了阴极液及底物浓度对系统产电及废水处理性能的影响。结果表明，使用缓冲溶液、阳极室出水和自来水作阴极液时，自来水的产电性能最佳，阴极液种类不影响系统有机基质的去除。以自来水为阴极液时，阴极液pH及电导率随运行时间增加而增加，COD去除率为80.11%～89.29%，输出电压及功率密度开始随运行时间增加而增加，之后稳定在440～452 mV和48.40～51.08 mW/m²之间。增加底物浓度对COD去除率影响不大，而输出电压及功率密度随底物浓度增加而下降；底物COD浓度由3 307.09 mg/L增至9 520 mg/L时，COD去除率在85.77%～94.44%之间，输出电压及功率密度则分别由449 mV和50.40 mW/m²下降至406 mV和41.21 mW/m²。自来水作阴极液可避免二次污染及阴极液对阳极室微生物的影响，并得到高的产电能力。     

厌氧折流板式微生物燃料电池堆影响因素研究

微生物燃料电池(MFC)中输出电压/电流的提升,以及反应器体积的扩展放大是其工程化应用的关键。本文构建了一个总体积为6.4 L的新型厌氧折流板式微生物燃料电池堆(ABSMFC)。以葡萄糖作为底物,探讨了阳极材料、液面高程差和水力停留时间(HRT)等因素对ABSMFC性能的影响。结果表明,碳纤维毡作为阳极时,电池单体外电路平均分压(R_(ex)=1 000Ω)为210 mV,填充石墨颗粒后增加到319.8 mV。格室间存在液面高程差时,电池单体、串联和并联的功率密度分别为207.1、181.1和215.7 mW/m~2,当无液面高程差(即水力相连)时为205.8、69.5和151.5 mW/m~2。4个电池单体串联和并联连接时,HRT对ABSMFC的产电稳定性无影响,溶解性COD的去除率和库仑效率均随HRT的增加而升高,且并联效果优于串联。     

重金属Cr(VI)、Pb及Cu胁迫对双齿围沙蚕体腔细胞的DNA损伤

为探讨重金属Cr(VI)、Pb以及Cu对沙蚕体腔细胞DNA的毒性效应,以双齿围沙蚕为受试动物,重金属按不同剂量水平,Cr(VI):10、100和200 mg·L~(-1),Pb:5、50和100 mg·L~(-1),Cu:1、10和20 mg·L~(-1),分别胁迫沙蚕24 h,以不加任何重金属离子的海水为对照,采用单细胞凝胶电泳技术,检测其体腔细胞DNA损伤程度。结果表明,与空白对照组相比,3种重金属离子的各浓度组都能引起沙蚕体腔细胞DNA损伤,且3种重金属胁迫浓度与细胞DNA损伤程度之间存在显著的剂量-效应关系。双齿围沙蚕可以作为单细胞凝胶电泳的实验材料用于重金属所致环境污染的生物监测指示生物。     

双室微生物燃料电池处理硝酸盐废水

基于双室微生物燃料电池(microbial fuel cell,MFC),针对阴极分别接种活性污泥(A-MFC)和反硝化细菌(D-MFC),研究其产电情况和硝酸盐废水去除效果。结果表明,在产电的同时都可有效去除废水中的硝酸盐污染物。在外接电阻100Ω的情况下,2种MFC均具有良好的产电性能,A-MFC和D-MFC达到的最大输出电压分别为119.6 mV和117.2mV,最大功率密度分别为23.40 mW/m2和26.63 mW/m2;同时两者在阴极室的平均反硝化速率分别为1.86 mg/(L.d)和2.19 mg/(L.d),阳极室的平均COD去除率分别为81.9%和82.4%。另外,通过扫描电镜观察可知,A-MFC和D-MFC阴极碳布表面形貌存在差异,并且阳极与阴极碳布表面形貌差异显著。     

Metabolism of the Nonylphenol Isomer [Ring-U-14c]-4-(3′,5′-Dimethyl-3′-Heptyl)-Phenol by Cell Suspension Cultures of Agrostemma githago and Soybean

Abstract

The biotransformation of the nonylphenol isomer [ring-U-¹⁴C]-4-(3′,5′-dimethyl-3′-heptyl)-phenol (4-353-NP, consisting of two diastereomers) was studied in soybean and Agrostemma githago cell suspension cultures. With the A. githago cells, a batch two-liquid-phase system (medium/n-hexadecane 200:1, v/v) was used, in order to produce higher concentrations and amounts of 4-353-NP metabolites for their identification; 4-353-NP was applied via the n-hexadecane phase. Initial concentrations of [¹⁴C]-4-353-NP were 1 mg L^?1 (soybean), and 5 and 10 mg L^?1 (A. githago). After 2 (soybean) and 7 days (A. githago) of incubation, the applied 4-353-NP was transformed almost completely by both plant species to four types of products: glycosides of parent 4-353-NP, glycosides of primary 4-353-NP metabolites, nonextractable residues and unknown, possibly polymeric materials detected in the media. The latter two products emerged especially in soybean cultures. Portions of primary metabolites amounted to 19–22% (soybean) and 21–42% of applied ¹⁴C (A. githago). After liberation from their glycosides, the primary 4-353-NP metabolites formed by A. githago were isolated by HPLC and examined by GC-EIMS as trimethylsilyl derivatives. In the chromatograms, eight peaks were detected which due to their mass spectra, could be traced back to 4-353-NP. Seven of the compounds were side-chain monohydroxylated 4-353-NP metabolites, while the remaining was a (side-chain) carboxylic acid derivative. Unequivocal identification of the sites of hydroxylation/oxidation of all transformation products was not possible. The main primary metabolites produced by A. githago were supposed to be four diastereomers of 6′-hydroxy-4-353-NP (about 80% of all products identified). It was concluded that plants contribute to the environmental degradation of the xenoestrogen nonylphenol; the toxicological properties of side-chain hydroxylated nonylphenols remain to be examined.     

Uptake of cadmium into cells in culture∗

Cadmium has been recognized as pollutant of the environment for many years and numerous studies on its toxic effects have been carried out. Little, however, is known about its metabolic behaviour e.g. why the metal is accumulated so extremely rapidly into the organs of men and animals. Since the study of the individual metabolic steps is very difficult in vivo cell cultures may be used to obtain first indications of what happens in the whole animal.

We used CHO cells in monolayer culture to study the conditions under which the uptake of cadmium occurs. From serumfree medium the metal is accumulated rapidly in the cells. The uptake is inhibited very strongly by the presence of serum or albumin. Accumulation occurs against a concentration gradient and is dependent on the incubation temperature. Below 10°C no cadmium uptake is seen. Several substances which are known to affect cell metabolism have been used to influence cadmium accumulation. Neither inhibitors of energy production nor microtubule or microfilament disruptors showed any substantial effect. In contrast SH‐group blocking agents markedly reduced cadmium uptake.

The results show that cadmium uptake does not occur by passive diffusion but by some active mechanism.     

不同酶强化污泥为燃料微生物燃料电池特性对比分析

采用单室无膜悬浮阴极微生物燃料电池(MFC),对比分析了蛋白酶和淀粉酶强化剩余污泥为燃料的MFC(ESMFC)产电特性、酶特性和污泥减量化效果。研究表明,投加蛋白酶的ESMFC最大功率密度比对照组增加106.2%,投加淀粉酶时ESMFC最大功率密度比对照组增加48%。蛋白酶作用主要体现在投加后的前12小时,而淀粉酶作用时间则较长,为投加后的前144小时,但在运行前期,由于高温作用,导致系统内的酶活性较强,投加的淀粉酶作用则不明显。投加蛋白酶的系统内TCOD、TSS和VSS去除率分别为82%、65%和85%,而投加淀粉酶的系统内TCOD、TSS和VSS去除率分别达到86%、67%和88%。此研究对于ESMFC中外加酶的选择具有一定意义。     

Telomere length in workers was effected by omethoate exposure and interaction between smoking and p21 polymorphisms

Abstract

Omethoate is an organophosphorus pesticide that poses a major health hazard, especially DNA damage. The purpose of this study was to investigate the factors affecting telomere length in workers exposed to omethoate by analyzing the interaction between cell cycle gene polymorphism and environmental factors. The exposure group consisted of 118 workers exposed to omethoate for 8–10?years, the control group comprised 115 healthy people without occupational toxicant exposure history. The telomere length of genomic DNA from peripheral blood leucocyte was determined with real-time PCR. Polymerase chain reaction and restriction fragment length polymorphism was used to detect the polymorphisms in p53, p21 and MDM2 gene. The telomere length in the (CA?+?AA) genotypes for p21 rs1801270 polymorphism was longer than that in the CC genotype in control group (P?=?0.015). The generalized linear model analysis indicated the interaction of the p21 rs1801270 polymorphic (CA?+?AA) genotypes and smoking has a significant effect on telomere length (β = ?0.258, P?=?0.085). The prolongation of telomere length in omethoate-exposed workers was associated with genotypes (CA?+?AA) of p21 rs1801270, and interactions of (CA?+?AA) genotypes and smoking factor.     

Influence of GSTM1 and GSTT1 genotypes and confounding factors on the frequency of sister chromatid exchange and micronucleus among road construction workers

In the present study, we have investigated the influence of polymorphism of GSTM1 and GSTT1 genes and confounding factors such as age, sex, exposure duration and consumption habits on cytogenetic biomarkers. Frequency of sister chromatid exchanges (SCEs), high frequency cell (HFC) and cytokinesis blocked micronuclei (CBMN) were evaluated in peripheral blood lymphocytes of 115 occupationally exposed road construction workers and 105 unexposed individuals. The distribution of null and positive genotypes of glutathione-S transferase gene was evaluated by multiplex PCR among control and exposed subjects. An increased frequency of CBMN (7.03 ± 2.08); SCE (6.95 ± 1.76) and HFC (6.28 ± 1.69) were found in exposed subjects when compared to referent (CBMN - 3.35 ± 1.10; SCE - 4.13 ± 1.30 and HFC - 3.98 ± 1.56). These results were found statistically significant at p < 0.05. When the effect of confounding factors on the frequency of studied biomarkers was evaluated, a strong positive interaction was found. The individuals having GSTM1 and GSTT1 null genotypes had higher frequency of CBMN, SCE and HFC. The association between GSTM1 and GSTT1 genotypes and studied biomarkers was found statistically significant at p < 0.05. Our findings suggest that individuals having null type of GST are more susceptible to cytogenetic damage by occupational exposure regardless of confounding factors. There is a significant effect of polymorphism of these genes on cytogenetic biomarkers which are considered as early effects of genotoxic carcinogens.