β-内酰胺类抗生素的环境行为与制药行业源头控制技术研究进展

β-内酰胺类抗生素是目前生产量和使用量最大的抗生素类型之一,在不同的环境基质中都能检出其残留、相关抗药菌和抗性基因,具有潜在的环境风险。中国是世界上最大的β-内酰胺类抗生素原料药生产国,每年产生大量的制药废水和菌渣。如何有效去除制药废水中残留抗生素及效价,并实现制药菌渣资源化利用是行业发展的技术瓶颈。在查阅文献的基础上,梳理了β-内酰胺类抗生素的环境污染来源和污染特征方面的研究进展,阐述了抗生素在环境中的迁移、吸附、水解等环境行为,并从环境抗性的产生和传播角度分析了β-内酰胺类抗生素的环境影响;重点梳理了废水和菌渣中β-内酰胺类抗生素的控制技术方面的研究进展,在此基础上,从降解产物与抗性关系、抗生素和效价的控制目标、废水抗生素和抗性基因控制多级屏障技术体系和制药菌渣无害化及资源化等方面提出展望,以期为环境中β-内酰胺类抗生素的环境管理和风险控制提供参考。     

β-环糊精强化二氧化钛光催化降解双酚F研究

研究了双酚F在β-环糊精存在的TiO_2光催化体系中的光降解行为,结果表明:双酚F能与β-环糊精形成1:1稳定的包结物,其包结常数为6.33×10~3L/mol,β-环糊精可以使双酚F的光催化降解效率可以提高21%,同时研究了双酚F光降解的动力学规律及pH、β-环糊精浓度、双酚F初始浓度对双酚F的光催化降解的影响。β-环糊精对双酚F光催化降解的强化作用源于β-环糊精促进双酚F在TiO_2表面的吸附。     

The amplification refractory mutation system (ARMS): A rapid and direct prenatal diagnostic technique for β-thalassaemia in Singapore

β-Thalassaemia major patients have chronic anaemia and since 3–4 per cent of Singaporeans carry the β-gene, prenatal diagnosis is essential. We evaluated the amplification refractory mutation system (ARMS) technique as a routine test for prenatal diagnosis of β-major. Six mutations along the β-gene were studied—41–42 (-TCTT), IVSII #654 (C-T), 17β (A-T), – 28 TATA (A-G), IVSI #5 (G-C), and IVSI #1 (G-T). Our results indicate that prenatal diagnosis using these mutations can be offered to 90 per cent (35/39) of our Chinese couples and 54·6 per cent (12/22) of our Malay couples at risk. Confirmation of ARMS results was carried out using allele-specific oligonucleotide hybridization. Prenatal diagnosis using ARMS was successfully carried out in nine cases which included a set of triplets and twins. The triplets were diagnosed with the β-trait carrying the 41–42 mutation. The couple with twins possessed the #654 mutation and one twin was diagnosed with the β-trait and the other with #654 homozygosity. Genomic sequencing of the undefined mutations in the Chinese couples revealed rarer mutations at − 29 and an ATG-AGG base substitution at the initiation codon for translation. In the Malay couples, genomic sequencing detected mutations at codon 15 (TGG-TAG) and codon 26 (GAG-AAG). We conclude that ARMS with its direct detection of amplified products by gel electrophoresis provides an accurate, rapid, and simpler method for our β-thalassaemia prenatal diagnosis programme in Singapore.     

催化动力学光度法测定工业废水中的Cr（Ⅵ）

采用β-环糊精作为H₂O₂氧化茜素红褪色反应的增敏剂,建立了催化动力学光度法测定工业废水中Cr（Ⅵ）的新方法。该方法最佳反应条件为：反应体系总体积25 mL,0.1 mol/L的H₂SO₄溶液加入量2.0 mL,1.0×10^-3 mol/L茜素红溶液加入量1.5 mL,30%的H₂O₂溶液加入量4.0 mL,100 g/L的β-环糊精溶液加入量3.0 mL。在最大吸收波长554 nm处测定反应前后溶液的吸光度,Cr（Ⅵ）的质量浓度与吸光度差值（ΔA）在4.0×10^-4~5.4×10^-2 mg/L范围内符合比尔定律,线性回归方程为：ΔA=18.52ρ+ 0.018,相关系数为0.996 6,检出限为3.5×10^-4 mg/L,加标回收率为99.46%~101.3%,6次测定的相对标准偏差小于等于2.4%。该法的测定结果与GB/T 7467-1987中的二苯碳酰二肼分光光度法相近。     

Effects of biodegradation and sorption by humic acid on the estrogenicity of 17β-estradiol

The removal of 17β-estradiol (E2) by biodegradation and sorption onto humic acid (HA) was examined at various HA concentrations. Subsequently, estrogenicity associated with E2 removal was estimated using E-screen bioassay. Results showed that E2 biodegradation and its subsequent transformation to estrone (E1) were significantly reduced with increasing HA concentration. In addition, the presence of nutrients enhanced the biodegradation of E2. Overall, E2 biodegradation was the dominating contributor to its removal, which demonstrated a significantly negative correlation with E2 sorption at various HA concentrations. The sorption of E2 by HA was significantly enhanced with increasing HA concentration. Estrogenicity associated with residual E2 showed that there existed a significant difference among various HA concentrations, with the lowest value in the absence of HA. The findings suggest that the presence of HA and nutrients in natural waters should be considered in assessing estrogenicity of environmental samples due to complex sorption and biodegradation processes.     

Simultaneous analysis of free and sulfo-conjugated steroid estrogens in artificial urine solution and agricultural soils by high-performance liquid chromatography

A simple and robust analytical method was developed to simultaneously detect and quantify 17β-estradiol (E2), estrone (E1), 17β-estradiol-3-sulphate (E2-3S), and estrone-3-sulphate (E1-3S) in aqueous solutions (calcium chloride and artificial urine solutions) and agricultural soils using high performance liquid chromatography and UV detection. The standards for all four compounds were linear in the range of 0.01 to 1.0 μg mL^?1 (n = 6) and 1.0 to 20 μg mL^?1 (n = 6), respectively, with correlation coefficients > 0.999. The on-column limits of detection at an injection volume of 50 μL and S/N (signal: noise) ratio of 3 were: 9.0 ng mL^?1, 10 ng mL^?1, 5.0 ng mL^?1, and 7.0 ng mL^?1 for E2-3S, E1-3S, E2 and E1, respectively. The limit of detection and quantification in artificial urine solution and CaCl₂ solution was 1.0 ng mL^?1 for all four compounds. Method detection limits for the compounds in the 3 soils ranged from 2 to 2.4 ng g^?1 (E2-3S and E1-3S), and 1.0 to 2.9 ng g^?1 (E2 and E1), respectively.     

气相色谱/负离子化学电离质谱法测定地表水中硫丹及其代谢物

采用气相色谱/负离子化学电离质谱法测定地表水中的硫丹及其代谢物,用正己烷提取,外标法定量。α-硫丹、β-硫丹及硫丹硫酸酯在0.200μg/L～10.0μg/L范围内线性良好,方法检出限分别为0.010μg/L、0.008μg/L及0.010μg/L,空白加标平行测定的RSD为3.9%～4.8%,地表水样品加标回收率为85.5%～93.8%。     

基于ELISA的受体竞争结合法检测环境雌激素(Competitive Estrogen Receptor Binding Based ELISA for Detection of Estrogen in Environment)

为建立环境雌激素的体外快速筛选方法,采用免疫测定介导受体竞争结合试验定量检测环境雌激素.将17β-雌二醇-BSA固定在微孔板上,环境雌激素与微孔板上的17β-雌二醇-BSA竞争性地与雌激素受体结合,与微孔板上17β-雌二醇-BSA结合的受体与雌激素受体的抗体、雌激素受体抗体的二抗形成一个三明治形式的复合物,通过显色剂显色,最后用比色法对试验结果进行定量.结果表明,环境雌激素的浓度与溶液吸光度值成负相关.定量研究可以得到环境雌激素剂量-效应关系曲线,在一定浓度范围内(10ng·L-1～100μg·L-1),溶液的吸光度值与环境雌激素的浓度直接呈现良好的线性关系(R2=0.9583).利用这种方法能检测到的标准品雌二醇的最低浓度为10ng·L-1.以上结果表明,本方法检测环境雌激素操作简便,具有广泛的应用前景.     

Noninvasive prenatal diagnosis of β-thalassaemia using individual fetal erythroblasts isolated from maternal blood after enrichment

Single nucleated red blood cells (NRBCs) isolated from maternal circulation were used for prenatal diagnosis of β-thalassaemia. The study included 22 pregnant women in the first trimester, 6 carriers at risk for β-thalassaemia and 16 noncarriers. Methodology involved enrichment of NRBCs by magnetic cell sorting (MACS) and microdissection of single NRBCs with a laser micromanipulation system. Single-cell genotyping based on nested real-time PCR for genotyping β-globin gene mutations was performed followed by a multiplexed minifingerprinting to confirm the origin of the isolated cells and possible contamination. Two polymorphic markers (D13S314 and GABRB3) facilitated the identification of fetal NRBCs through comparison of allele sizes found in the respective parents. In this study, 224 single NRBCs were detached and transferred into individual PCR tubes. Allele amplification in at least one microsatellite marker was achieved in 128/224 cells. Minifingerprinting analysis showed that 22 cells were fetal, 26 maternal and 80 were noninformative due to ADO or homozygosity. In 6 NRBCs the β-globin gene was amplified and in 2, coming from the same pregnancy, only the paternal mutation was detected. The low PCR success when genotyping isolated NRBCs was possibly due to the poor quality of fetal NRBCs and the relatively large size of the β-globin gene product. Copyright © 2007 John Wiley & Sons, Ltd.