除草剂阿特拉津生物降解研究进展

本文综述了近年来国内外在阿特拉津降解菌及降解途径方面的研究进展,及在微生物产生的阿拉拉津降解酶,其操作基因方面的研究现状,并提出了阿特拉津生物降解的研究趋势.     

腐殖酸和铁对阿特拉津光降解影响的研究

为考察除草剂在水体中的自净性能,对模拟太阳光(λ> 290 nm)下腐殖酸和铁元素对阿特拉津的光化学降解进行了研究。结果表明,单独辐照阿特拉津几乎不降解。在分别加入3、5和10 mg/L的腐殖酸时,阿特拉津的降解率分别为34.36 %、40.74%和15.66 %;在Fe(Ⅲ)投加量从0.01 mmol/L增加到0.2 mmol/L时,阿特拉津的降解率从24.36 %增加到34.97 %。而在当腐殖酸与铁共存时,阿特拉津降解率则进一步提高。紫外可见光谱和荧光光谱均表明,腐殖酸-铁络合物的形成及其光化学作用,促进了阿特拉津的降解。     

基于绿色合成法的纳米铁/活性炭复合材料降解阿特拉津的动力学

为了综合处理水中的阿特拉津,以绿茶萃取液为还原剂,以活性炭为载体,采用液相还原法绿色合成了纳米铁/活性炭复合材料,研究了活性炭投放量、阿特拉津的初始浓度、溶液初始pH值及反应时间对阿特拉津去除率的影响,探讨了不同影响因素下阿特拉津的降解动力学。结果表明:阿特拉津降解反应近似符合二级反应动力学,反应速率常数0.001 08~0.002 73 L·(mg·min)~(-1)。在纳米铁/活性炭复合材料去除阿特拉津过程中,纳米铁的还原和活性炭的吸附共同作用。     

静态环境下阿特拉津的生物降解研究

从农药厂阿特拉津生产车间污泥中分离出菌种AT菌,进行了系列降解实验.不同温度的降解实验表明,在4～20℃的实验温度范围内,AT菌能够降解代谢污染质,并随温度的升高,降解能力增强.20℃时降解率为38.84%;AT菌在外加氮源、碳源及以阿特拉津为惟一碳源和氮源等条件时对农药污染质阿特拉津均具有降解能力,且在以阿特拉津为惟一氮源(外加碳源)条件下的降解效果最好,此时的降解率为30.39%.     

静态环境下阿特拉津的生物降解研究

从农药厂阿特拉津生产车间污泥中分离出菌种AT菌，进行了系列降解实验。不同温度的降解实验表明，在4～20℃的实验温度范围内，AT菌能够降解代谢污染质，并随温度的升高，降解能力增强。20℃时降解率为38．84％；AT菌在外加氮源、碳源及以阿特拉津为惟一碳源和氮源等条件时对农药污染质阿特拉津均具有降解能力，且在以阿特拉津为惟一氮源（外加碳源）条件下的降解效果最好，此时的降解率为30．39％。     

饮用水原水中微量阿特拉津去除方法试验研究

饮用水中微量有机物的污染是关系饮用水生态安全的重要问题。以饮用水中微量的内分泌干扰类除草剂阿特拉津为研究对象,分别采用微生物降解技术和光催化氧化技术对其进行降解,考察温度对阿特拉津降解效果的影响。研究结果表明：阿特拉津浓度为1 mg/L时,3种温度条件下,除锰功能菌MB4对阿特拉津均有明显的去除效果,降解时间为7 d时,阿特拉津的去除率达到65%。底物浓度为200 μg/L,3种温度条件下,活性炭负载二氧化钛（TiO₂/PAC）催化剂光降解阿特拉津30 min时,其去除率均达到90%。光催化氧化技术协同微生物降解技术在饮用水中微量的内分泌干扰物的去除中有广阔的应用前景。     

水中腐殖酸可见光降解阿特拉津的动力学研究

探讨了天然水体中存在的腐殖酸(HA)可见光降解水中阿特拉津的动力学特征和影响因素。结果表明,pH对HA可见光降解阿特拉津具有明显影响,水中HA质量浓度为5.0mg/L时,pH为3、5、7、9的条件下,受可见光照6.00h后阿特拉津(初始质量浓度5mg/L)的去除率分别为75.5%、77.3%、91.7%、84.9%,中性条件下阿特拉津可见光降解效果最佳;当HA质量浓度分别为1.5、3.0、5.0、10.0mg/L时,HA对水中阿特拉津的可见光降解均表现为促进作用,且降解过程符合一级反应动力学方程,其一级反应动力学常数分别为0.337 0、0.361 4、0.445 4、0.314 6h-1,HA为5.0mg/L时阿特拉津的可见光降解效果最佳。实际应用中,可以通过优化HA与阿特拉津的浓度比值,发挥HA促进阿特拉津可见光降解的最佳效能。     

羟基氧化铁催化臭氧氧化去除水中阿特拉津

以实验室制备的羟基氧化铁(FeOOH)为催化剂,研究了其催化臭氧氧化去除水中痕量阿特拉津的效能,并对影响催化效果因素及降解机理进行了探讨。在本实验条件下,反应8 min时催化氧化阿特拉津的去除率比单独臭氧氧化高出63.2%,而FeOOH对阿特拉津的吸附量很小,结果表明,FeOOH对臭氧氧化水中的痕量阿特拉津具有明显的催化活性。探讨了催化剂投量、pH、阿特拉津初始浓度和重碳酸盐碱度对催化氧化阿特拉津的影响。催化剂最佳投量为150 mg/L,去除率随pH和阿特拉津初始浓度的增加而升高,重碳酸盐浓度为200 mg/L时催化作用受到明显抑制。通过研究叔丁醇对催化反应的影响间接推断了催化反应的机理,叔丁醇作为羟基自由基抑制剂有效地抑制了水中羟基自由基的生成和它对阿特拉津的氧化反应,间接证明这种催化作用遵循羟基自由基的反应机理。     

2种低温等离子体降解土壤中乙草胺和阿特拉津

研究了沿面放电和平板介质阻挡放电处理土壤中阿特拉津和乙草胺的效果。主要以沙子作为研究体系,考察了水分、氧气流速、活性炭和过硫酸钠对降解的影响。结果表明:沿面放电装置和平板介质阻挡放电都能高效降解沙子中的乙草胺、阿特拉津;水分和氧气流速对降解的影响较大,在一定限度内,它们的增加能迅速提高降解效果,但过多的水分反而会抑制污染物的降解。活性炭显著抑制沿面放电降解乙草胺和阿特拉津效果,过硫酸钠与沿面放电、平板介质阻挡放电联用方法没有表现出协同效应。     

一种新嗜冷菌JLNY02降解地下水中阿特拉津的研究

从某农药厂排污口采集污泥样品，通过富集培养，从中分离筛选出一株阿特拉津高效降解菌JLNY02，并进一步对其降解的影响因素进行研究。在10℃的条件下降解阿特拉津，其降解率可达81.8%，而在高温下的降解率较低，仅31．4％。     

Biodegradation of atrazine by Rhodococcus sp. BCH2 to N-isopropylammelide with subsequent assessment of toxicity of biodegraded metabolites

Atrazine is a persistent organic pollutant in the environment which affects not only terrestrial and aquatic biota but also human health. Since its removal from the environment is needed, atrazine biodegradation is achieved in the present study using the bacterium Rhodococcus sp. BCH2 isolated from soil, long-term treated with atrazine. The bacterium was capable of degrading about 75 % atrazine in liquid medium having pH 7 under aerobic and dark condition within 7 days. The degradation ability of the bacterium at various temperatures (20–60 °C), pH (range 3–11), carbon (glucose, fructose, sucrose, starch, lactose, and maltose), and nitrogen (ammonium molybdate, sodium nitrate, potassium nitrate, and urea) sources were studied for triumph optimum atrazine degradation. The results indicate that atrazine degradation at higher concentrations (100 ppm) was pH and temperature dependent. However, glucose and potassium nitrate were optimum carbon and nitrogen source, respectively. Atrazine biodegradation analysis was carried out by using high-performance thin-layer chromatography (HPTLC), Fourier transform infrared spectroscopy (FTIR), and liquid chromatography quadrupole time-of-flight (LC/Q-TOF-MS) techniques. LC/Q-TOF-MS analysis revealed formation of various intermediate metabolites including hydroxyatrazine, N-isopropylammelide, deisopropylhydroxyatrazine, deethylatrazine, deisopropylatrazine, and deisopropyldeethylatrazine which was helpful to propose biochemical degradation pathway of atrazine. Furthermore, the toxicological studies of atrazine and its biodegraded metabolites were executed on earthworm Eisenia foetida as a model organism with respect to enzymatic (SOD and Catalase) antioxidant defense mechanism and lipid peroxidation studies. These results suggest innocuous degradation of atrazine by Rhodococcus sp. BCH2 in nontoxic form. Therefore the Rhodococcus sp.BCH2 could prove a valuable source for the eco-friendly biodegradation of atrazine pesticide.     

Influence of microbial and synthetic surfactant on the biodegradation of atrazine

The present study reports the effect of surfactants (rhamnolipids and triton X-100) on biodegradation of atrazine herbicide by strain A6, belonging to the genus Acinetobacter. The strain A6 was able to degrade nearly 80 % of the 250-ppm atrazine after 6 days of growth. The bacterium degraded atrazine by de-alkylation process. Bacterial cell surface hydrophobicity as well as atrazine solubility increased in the presence of surfactant. However, addition of surfactant to the mineral salt media reduced the rate and extent of atrazine degradation by decreasing the bioavailability of herbicide. On the contrary, addition of surfactant to atrazine-contaminated soil increased the rate and extent of biodegradation by increasing the bioavailability of herbicide. As compared to triton X-100, rhamnolipids were more efficient in enhancing microbial degradation of atrazine as a significant amount of atrazine was removed from the soil by rhamnolipids. Surfactants added for the purpose of hastening microbial degradation may have an unintended inhibitory effect on herbicide degradation depending upon contiguous condition, thus highlighting the fact that surfactant must be judiciously used in bioremediation of herbicides.     

Using polymer mats to biodegrade atrazine in groundwater: laboratory column experiments

Large-scale column experiments were undertaken to evaluate the potential of in situ polymer mats to deliver oxygen into groundwater to induce biodegradation of the pesticides atrazine, terbutryn and fenamiphos contaminating groundwater in Perth, Western Australia. The polymer mats, composed of woven silicone (dimethylsiloxane) tubes and purged with air, were installed in 2-m-long flow-through soil columns. The polymer mats proved efficient in delivering dissolved oxygen to anaerobic groundwater. Dissolved oxygen concentrations increased from <0.2 mg l(-1) to approximately 4 mg l(-1). Degradation rates of atrazine in oxygenated groundwater were relatively high with a zero-order rate of 240-380 microg l(-1) or a first-order half-life of 0.35 days. Amendment with an additional carbon source showed no significant improvement in biodegradation rates, suggesting that organic carbon was not limiting biodegradation. Atrazine degradation rates estimated in the column experiments were similar to rates determined in laboratory culture experiments, using pure cultures of atrazine-mineralising bacteria. No significant degradation of terbutryn or fenamiphos was observed under the experimental conditions within the time frames of the study. Results from these experiments indicate that remediation of atrazine in a contaminated aquifer may be achievable by delivery of oxygen using an in situ polymer mat system.     

Effect of ozonation on the biodegradability of atrazine in GAC columns

Abstract

The biodegradation of atrazine as influenced by preozonation was studied in biological GAC columns. Metabolism of isopropyl‐¹⁴C atrazine produced more ¹⁴CO₂ than ring‐UL‐¹⁴C atrazine, indicating dealkylation was more rapid than ring cleavage. Preozonation increased mineralization of ring‐UL‐¹⁴C atrazine and, consequently, enhanced the performance of the GAC columns. Sixty‐two percent of the influent atrazine was converted to ¹⁴CO₂ in columns that received ozonated atrazine and ozonated surface water, while 50% of the influent atrazine was converted to ¹⁴CO₂ in columns that received untreated atrazine and ozonated surface water, and only 38% of the influent atrazine was converted to ¹⁴CO₂ in columns with untreated influent.     

Atrazine removal in agricultural infiltrate by bioaugmented polyvinyl alcohol immobilized and free Agrobacterium radiobacter J14a: a sand column study

Bench-scale sand column breakthrough experiments were conducted to examine atrazine removal in agricultural infiltrate by Agrobacterium radiobacter J14a (J14a) immobilized in phosphorylated-polyvinyl alcohol compared to free J14a cells. The effects of cell loading and infiltration rate on atrazine degradation and the loss of J14a were investigated. Four sets of experiments, (i) tracers, (ii) immobilized dead cells, (iii) immobilized cells, and (iv) free cells, were performed. The atrazine biodegradation at the cell loadings of 300, 600, and 900 mg dry cells L(-1) and the infiltration rates of 1, 3, and 6 cm d(-1) were tested for 5 column pore volumes (PV). The atrazine breakthrough results indicated that the immobilized dead cells significantly retarded atrazine transport. The atrazine removal efficiencies at the infiltration rates of 1, 3, and 6 cm d(-1) were 100%, 80-97%, and 50-70%, respectively. Atrazine degradation capacity for the immobilized cells was not significantly different from the free cells. Both infiltration rate and cell loading significantly affected atrazine removal for both cell systems. The bacterial loss from the immobilized cell system was 10-100 times less than that from the free cell system. For long-term tests at 50 PV, the immobilized cell system provided consistent atrazine removal efficiency while the atrazine removal by the free cells declined gradually because of the cell loss.     

Atrazine biodegradation by Arthrobacter strain DAT1: effect of glucose supplementation and change of the soil microbial community

The objective of this study was to investigate the impact of glucose supplementation on the soil microbiota inoculated with the atrazine-degrading Arthrobacter strain DAT1. Soil microcosms with different treatments were constructed for biodegradation tests. The impact of glucose supplementation on atrazine degradation capacity of the strain DAT1 and the strain’s survival and growth were assessed. The densities of the 16S rRNA gene and the atrazine-metabolic trzN gene were determined using quantitative PCR. The growth of the strain DAT1 and the bacterial community structure were characterized using terminal restriction fragment length polymorphism. Glucose supplementation could affect atrazine degradation by the strain DAT1 and the strain’s trzN gene density and growth. The density of the16S rRNA gene decreased during the incubation period. Glucose supplementation could alter the bacterial community structure during the bioaugmentation process. Glucose supplementation could promote the growth of the autochthonous soil degraders that harbored novel functional genes transforming atrazine. Further study will be necessary in order to elucidate the impact of exogenous carbon on autochthonous and inoculated degraders. This study could add some new insights on atrazine bioremediation.     

Toxicity of atrazine and its bioaccumulation and biodegradation in a green microalga,Chlamydomonas mexicana

This study evaluated the toxicity of herbicide atrazine, along with its bioaccumulation and biodegradation in the green microalga Chlamydomonas mexicana. At low concentration (10 μg L^?1), atrazine had no profound effect on the microalga, while higher concentrations (25, 50, and 100 μg L^?1) imposed toxicity, leading to inhibition of cell growth and chlorophyll a accumulation by 22 %, 33 %, and 36 %, and 13 %, 24 %, and 27 %, respectively. Atrazine 96-h EC50 for C. mexicana was estimated to be 33 μg L^?1. Microalga showed a capability to accumulate atrazine in the cell and to biodegrade the cell-accumulated atrazine resulting in 14–36 % atrazine degradation at 10–100 μg L^?1. Increasing atrazine concentration decreased the total fatty acids (from 102 to 75 mg g^?1) and increased the unsaturated fatty acid content in the microalga. Carbohydrate content increased gradually with the increase in atrazine concentration up to 15 %. This study shows that C. mexicana has the capability to degrade atrazine and can be employed for the remediation of atrazine-contaminated streams.     

Modeling depth-variant and domain-specific sorption and biodegradation in dual-permeability media

A dual-permeability model (S_1D_DUAL) was developed to simulate the transport of land-applied pesticides in macroporous media. In this model, one flow domain was represented by the bulk matrix and the other by the preferential flow domain (PFD) where water and chemicals move at faster rates. The model assumed the validity of Darcian flow and the advective-dispersive solute transport in each of the two domains with inter-domain transfer of water and solutes due to pressure and concentration gradients. It was conceptualized that sorption and biodegradation rates vary with soil depth as well as in each of the two flow domains. In addition to equilibrium sorption, kinetic sorption was simulated in the PFD. Simulations were conducted to evaluate the combined effects of preferential flow, depth- and domain-variant sorption, and degradation on leaching of two pesticides: one with strong sorption potential (trifluralin) and the other with weak sorption potential (atrazine). Simulation results for a test case showed that water flux in the PFD was three times more than in the matrix for selected storm events. When equilibrium sorption was considered, the simulated profile of trifluralin in each domain was similar; however, the atrazine profile was deeper in the PFD than in the bulk matrix under episodic storm events. With an assumption of negligible sorption in the PFD, both the atrazine and the trifluralin profiles moved twice deeper into the PFD. The simulated concentrations of the chemicals were several orders higher in the PFD than in the matrix, even at deeper depths. The volume fraction of the macropores and the sorption and biodegradation properties of the chemicals could also affect the amount of pesticides leaving the root zone. For an intense storm event, slow sorption reaction rates in the PFD produced higher breakthrough concentrations of atrazine at the bottom of the simulated soil profile, thus posing the risk for breakthrough of chemicals from the root zone.     

Perspectives of using fungi as bioresource for bioremediation of pesticides in the environment: a critical review

Pesticides are used for controlling the development of various pests in agricultural crops worldwide. Despite their agricultural benefits, pesticides are often considered a serious threat to the environment because of their persistent nature and the anomalies they create. Hence removal of such pesticides from the environment is a topic of interest for the researchers nowadays. During the recent years, use of biological resources to degrade or remove pesticides has emerged as a powerful tool for their in situ degradation and remediation. Fungi are among such bioresources that have been widely characterized and applied for biodegradation and bioremediation of pesticides. This review article presents the perspectives of using fungi for biodegradation and bioremediation of pesticides in liquid and soil media. This review clearly indicates that fungal isolates are an effective bioresource to degrade different pesticides including lindane, methamidophos, endosulfan, chlorpyrifos, atrazine, cypermethrin, dieldrin, methyl parathion, heptachlor, etc. However, rate of fungal degradation of pesticides depends on soil moisture content, nutrient availability, pH, temperature, oxygen level, etc. Fungal strains were found to harbor different processes including hydroxylation, demethylation, dechlorination, dioxygenation, esterification, dehydrochlorination, oxidation, etc during the biodegradation of different pesticides having varying functional groups. Moreover, the biodegradation of different pesticides was found to be mediated by involvement of different enzymes including laccase, hydrolase, peroxidase, esterase, dehydrogenase, manganese peroxidase, lignin peroxidase, etc. The recent advances in understanding the fungal biodegradation of pesticides focusing on the processes, pathways, genes/enzymes and factors affecting the biodegradation have also been presented in this review article.     

Competitive biodegradation of dichlobenil and atrazine coexisting in soil amended with a char and citrate

The role of char nutrients in the biodegradation of coexisting dichlobenil and atrazine in a soil by their respective bacterial degraders, DDN and ADP, was evaluated. Under growing conditions, their degradation in soil extract was slow with <40% and <20% degraded within 64 h, respectively. The degradation in extracts and slurries of char-amended solids increased with increasing char content, due to nutritional stimulation on microbial activities. By supplementing soil extract with various major nutrients, the measured degradation demonstrated that P was the exclusive limiting nutrient. The reduction in the degradation of coexisting dichlobenil and atrazine resulted apparently from the competitive utilization of P by DDN and ADP. With a shorter lag phase, ADP commenced growing earlier than DDN with the advantage of utilizing P first in insufficient supply. This resulted in an inhibition on the growth of DDN and thus suppression on dichlobenil degradation.