滇池底泥微生物菌群对微囊藻毒素的生物降解

采用滇池水华蓝藻中提取提纯的微囊藻毒素（microcystins，MCs）作为微生物生长的碳源和氮源，从长期暴露于蓝藻水华的滇池底泥中，通过从含低浓度到高浓度MCs的逐步培养驯化，获得了高效降解MCs的微生物混合菌群，在初始MC-RR和LR浓度大约分别为50mg／L和30mg／L下，3d内可将MCs全部降解。进一步活性研究显示，不同含碳和含氮化合物虽然能够促进混合微生物菌群的生长，但对降解MCs却无明显的促进作用，说明MCs既可以作为微生物生长的碳源，又可以作为微生物生长的氮源，在富含有机物的天然水体中并不一定能够促进微生物对MCs的生物降解。     

微囊藻毒素的生物降解综述

从微囊藻毒素降解菌、降解途径和影响降解的因素三方面，对国内外微囊藻毒素生物降解的研究现状及发展趋势作一介绍。     

滇池底泥微生物菌群对微囊藻毒素的生物降解

采用滇池水华蓝藻中提取提纯的微囊藻毒素(microcystins,MCs)作为微生物生长的碳源和氮源,从长期暴露于蓝藻水华的滇池底泥中,通过从含低浓度到高浓度MCs的逐步培养驯化,获得了高效降解MCs的微生物混合菌群,在初始MC-RR和LR浓度大约分别为50 mg/L和30 mg/L下,3 d内可将MCs全部降解.进一步活性研究显示,不同含碳和含氮化合物虽然能够促进混合微生物菌群的生长,但对降解MCs却无明显的促进作用,说明MCs既可以作为微生物生长的碳源,又可以作为微生物生长的氮源,在富含有机物的天然水体中并不一定能够促进微生物对MCs的生物降解.     

富营养化淡水水体中微囊藻毒素的研究进展

微囊藻毒素（Microcystins，MCYSTs，MCs）为富营养化淡水体中最常见的藻类毒素，从毒理学，环境科学，生物学及化学等方面对MCs的研究已有较多报道。本文综述了关于MCs在产生机理，毒理效应，分离检测方法和水处理过程中的去除方法等方面的研究进展，并对目前研究的不足提出了几点意见。     

光反应器中UV/Fenton光降解湖水中微囊藻毒素的研究

在光催化反应器中,采用UV/Fenton光催化氧化技术,对湖水中微囊藻毒素的光催化降解过程中各影响因子分析表明:微囊藻毒素光催化氧化降解率受光照强度、氧化剂种类及浓度、溶液pH和不同光催化体系等多因素的影响.光促催化氧化体系对MC-LR藻毒素降解具有显著的作用,在紫外光与氧化剂的协同作用下,紫外光照强度越高,越易于促进MC-LR藻毒素快速降解,降解率可到达80%以上.     

高效降解微囊藻毒素食酸戴尔福特菌USTB-04的培养与活性研究

主要针对筛选的高效降解微囊藻毒素(microcystins,MCs)的食酸戴尔福特菌USTB-04(Delftia acidovorans,DA菌)的培养方法进行了研究.结果表明,以葡萄糖、甘油和乙醇作为惟一碳源时,与氯化铵和尿素相比,酵母粉是支持DA菌生长的较好氮源.在以酵母粉作为惟一氮源时,与甘油和乙醇相比,葡萄糖是提高DA菌生长速度的较好碳源.进一步研究显示,以葡萄糖和酵母粉作为碳源和氮源时,可以支持DA菌的快速稳定生长,但在以甘油和酵母粉作为碳源和氮源时.培养出的DA菌降解MCs的比活性最高.此研究在培养高细胞浓度DA菌作为生物催化剂用于饮用水源中的MCs去除方面具有重要意义.     

富营养化淡水水体中微囊藻毒素的研究进展

微囊藻毒素（Microcystins,MCYSTs,MCs）为富营养化淡水水体中最常见的藻类毒素,从毒理学、环境科学、生物学及化学等方面对MCs的研究已有较多报道。本文综述了关于MCS在产生机理、毒理效应、分离检测方法和水处理过程中的去除方法等方面的研究进展,并对目前研究的不足提出了几点意见。     

白腐菌S.commune降解微囊藻毒素-LR的研究

为研究真菌对微囊藻毒素的降解作用,以白腐菌S.commune为降解菌,微囊藻毒素-LR(MC-LR)为降解目标进行生物降解,考察了白腐菌预培养方式及降解过程中的培养方式、充氧方式、温度、初始pH以及MC-LR初始浓度对降解效果的影响.结果表明,白腐菌可有效降解MC-LR,经液体预培养白腐菌对MC-LR的降解效果好于固体预培养,白腐菌静置培养过程中每天充入纯氧1min有助于MC-LR的降解,白腐菌降解MC-LR的最佳初始pH为4.5,适宜温度为30～35℃.白腐菌对MC-LR的降解能力随MC-LR初始浓度的增加而降低.在最佳条件下,当MC-LR初始质量浓度为1 mg/L时,其完全降解需要2d；当MC-LR初始质量浓度为15 mg/L时,其完全降解需要7d.高浓度MC-LR(30 mg/L以上)会对白腐菌生长产生抑制作用.MC-LR降解中间产物的具体结构尚不清楚,有待未来深入分析研究.     

越南伯克霍尔德菌降解水中微囊藻毒素-LR

探讨利用越南伯克霍尔德菌(Burkholderia Vietnamiensis)降解微囊藻毒素-LR(MC-LR)的可能性和降解机理。结果表明,在1 mg/L的MC-LR溶液中投加体积分数为5%菌株,初始pH为5,温度为30℃的好氧条件下,经过48 h培养后对MC-LR的降解效率达到97.6%。首先,降解溶液的液相色谱分析结果发现,MC-LR在238 nm的特征峰消失。其次,动力学研究发现降解过程符合一级动力学反应方程。最后,SEM、FTIR表征技术对菌株降解前后样品进行分析发现微生物形态和降解产物。因此,Burkholderia Vietnamiensis可能将水中的MC-LR作为碳、氮源利用从而将其降解,Burkholderia Vietnamiensis作为生物降解MC-LR的一种途径是有效的。     

一株微囊藻毒素降解菌的分离与鉴定

以水华蓝藻细胞中提取的微囊藻毒素为筛选物质,从太湖水华腐烂蓝藻中富集筛选出1株微囊藻毒素降解菌。该菌株革兰氏染色呈阴性,细胞细长杆状,菌落黄色,圆形,不透明,接触酶、氧化酶实验均呈阳性。16S rRNA基因序列的长度为1 416 bp(GenBank登录号为FJ976656)。系统发育树显示,该菌株与微嗜酸寡养单胞菌(Stenotrophomonas acidam-iniphila)的亲缘关系最近。通过菌株形态特征、生理生化特征和16S rRNA基因序列分析,将此菌株鉴定为微嗜酸寡养单胞菌,不同于已报道的微囊藻毒素降解菌属种。微囊藻毒素降解实验表明,该菌株5 d内将15.4 mg/L的微囊藻毒素完全降解,降解能力高于假单胞菌。     

Degradation of microcystins in aqueous solution with in situ electrogenerated active chlorine

A new and efficient method for the degradation of microcystins (one family of blue algal toxins) was developed and studied. Microcystins (MCs) in water were directly and effectively removed by active chlorine transformed in situ from the naturally existing Cl- in water resource using electrochemical method. Titanium coated with RuO2 and TiO2 was used as the anode. Microcystin-RR (MCRR) and Microcystin-LR (MCLR) were chosen as the model compounds of MCs. The results suggested that 20.87 mgl(-1) MCs (12.58 mgl(-1) MCRR and 8.29 mgl(-1) MCLR) in aqueous solution with 1.85 mM Cl- could be synchronously decomposed within 15 min electrolysis under the condition of the current density 8.89 mAcm(-2), 20 degrees C and pH 7.00. The qualitative analysis showed that the heptapetide ring and the Adda group of both treated MCs were changed. The results also indicated that the removal rates of both MCs increased with the increasing of chloride concentration and applied current density, but decreased with the increasing of initial concentration of MCs and initial pH of electrolyte. In the absence of Cl-, only a small fraction of both MCs were decomposed by direct anodic oxidation, while their almost complete removals could be obtained in the case of indirect electrooxidation with in situ electrogenerated active chlorine from Cl- in water.     

Adsorption of microcystins by carbon nanotubes

The production of cyanobacterial toxins microcystins (MCs) by cyanobacterial bloom which may promote the growth of tumor in human liver is a growing environmental problem worldwide. In this paper, the adsorption of MC-RR and LR, which were extracted from cyanobacterial cells in Dianchi Lake in China, by carbon nanotubes (CNTs), wood-based activated carbon (ACs) and clays were investigated. Compared with ACs and clay materials of sepiolite, kaolinite and talc tested, CNTs were found to have a strong ability in the adsorption of MCs. At the concentrations of 21.5 mg l(-1) MC-RR and 9.6 mg l(-1) MC-LR in 50 mmol phosphate buffer solution (pH 7.0), the adsorption amounts of MCs by CNTs with the range of outside diameter from 2 to 10nm were 14.8 and 5.9 mg g(-1), which were about four times higher than those by other adsorbents tested. It was shown that with the decrease of CNTs outside diameters from 60 to 2 nm, the adsorption amount of MCs was apparently increased, however the size of CNTs particles formed in solution declined. This result implies that the size of CNTs tube pore that is fit for the molecular dimension of MCs plays a dominant role. Furthermore the specific surface area of CNTs was also found to be a factor in the adsorption of MCs. The results suggested that the selection of suitable size of CNTs as a kind of adsorbent is very important in the efficient eliminating MCs from drinking water in future.     

Blooming of Microcystis aeruginosa in the reservoir of the reclaimed land and discharge of microcystins to Isahaya Bay (Japan)

Purpose

In the reservoir created in the reclaimed land in Isahaya Bay, Japan, Microcystis aeruginosa, which produces microcystins (MCs), bloomed every year, and the water with high levels of MCs in the reservoir has been often drained to Isahaya Bay to adjust the water level. The principal aims of this study are to clarify the water conditions suitable for blooming of M. aeruginosa in the reservoir, to follow the amount of distribution of MCs inside and outside the reservoir, and to discuss how blooming of M. aeruginosa is controlled in the reservoir and how MCs produced by Microcystis spread or accumulate in the aquatic environment.

Method

We monitored the water quality (temperature, salinity, dissolved inorganic nitrogen (DIN), and dissolved inorganic phosphorus) in the reservoir with seasonal blooming of microalgae including phytoplankton and M. aeruginosa using the concentrations of chlorophyll ?? and MCs, respectively, and collected the surface sediment in the reservoir and the bay to determine the MC content using the ELISA method.

Result

M. aeruginosa bloomed in extremely low DIN conditions of the water in warm seasons (spring and late summer to autumn). The year-mean standing stock of MCs was approximately 34.5?kg in the water and 8.4?kg in the surface sediment in the reservoir. Approximately 64.5?kg of MCs was discharged with the effluent to the bay in a year.

Conclusion

Since a large amount of MCs always suspends in the water in the reservoir and it has been discharged to the bay, suspension-feeding animals are exposed most seriously to the high levels of MCs occurring in these areas. We need to pay attention to the danger of widespread dispersal of MCs and biological concentration of MCs by fish and clam inside and outside the reservoir.     

Physiological and biochemical defense reactions of Vicia faba L.–Rhizobium symbiosis face to chronic exposure to cyanobacterial bloom extract containing microcystins

The presence of cyanotoxins, mainly microcystins (MCs), in surface freshwater represents a serious health risk to aquatic organisms living in the water body, as well as terrestrial animals and plants that are in contact with contaminated water. Consequently, the use of MCs contaminated water for irrigation represents a hazard for cultivated plants and could induce severe economical losses due to crops’ yield reduction. The experimental approach undertaken in this work was exposing Vicia faba seedlings (inoculated with a Rhizobium strain resistant to MCs), to water supplemented with cyanobacterial crude extract containing total microcystins at a concentration of 50 and 100 μg/L (environmental relevant concentrations of MCs dissolved in the raw irrigation water from Lalla Takerkoust Lake-Marrakesh region). After chronic MCs exposure (2 months), biological and physiological parameters (plant growth, nitrogen uptake, mineral assimilation, and oxidative defense mechanisms) were evaluated. The results obtained showed evidence that chronic exposure to cyanobacterial bloom extract containing MCs strongly affected the physiological and biological plants activities; reduction of dry matter, photosynthetic activity, nodule number, and nitrogen assimilation. At the same time, an increase of oxidative stress was observed, as deduced from a significant increase of the activities of peroxidase, catalase, polyphenoloxidase, and phenylalanine ammonia lyase in leaves, roots, and nodules of faba bean plants exposed to cyanotoxins, especially at 100 μg/L of MCs. This experimentation constitutes a simulation of the situation related to cyanotoxins chronic exposure of seedlings—plants via the contaminated irrigation water. For this reason, once should take into consideration the possibility of contamination of agricultural crops and the quality of irrigation water should be by the way monitored for cyanotoxins biohazard.     

Accumulation of free and covalently bound microcystins in tissues of Lymnaea stagnalis (Gastropoda) following toxic cyanobacteria or dissolved microcystin-LR exposure

Accumulation of free microcystins (MCs) in freshwater gastropods has been demonstrated but accumulation of MCs covalently bound to tissues has never been considered so far. Here, we follow the accumulation of total (free and bound) MCs in Lymnaea stagnalis exposed to i) dissolved MC-LR (33 and 100 μg L⁻¹) and ii) Planktothrix agardhii suspensions producing 5 and 33 μg MC-LR equivalents L⁻¹ over a 5-week period, and after a 3-week depuration period. Snails exposed to dissolved MC-LR accumulated up to 0.26 μg total MCs g⁻¹ dry weight (DW), with no detection of bound MCs. Snails exposed to MCs producing P. agardhii accumulated up to 69.9 μg total MCs g⁻¹ DW, of which from 17.7 to 66.7% were bound. After depuration, up to 15.3 μg g⁻¹ DW of bound MCs were detected in snails previously exposed to toxic cyanobacteria, representing a potential source of MCs transfer through the food web.     

Identification of microcystins from three collection strains of Microcystis aeruginosa

Microcystins (MCs) are toxic cyclic heptapeptides produced by various cyanobacteria genera, especially Microcystis. We identified 10 out of 12 MCs produced by three Microcystis aeruginosa strains from cyanobacteria collections, UTEX 2666, UTEX 2670 and UAM 1303, by using two analytical methods: Matrix-assisted Laser Desorption Ionization Time of Flight Mass Spectrometry (MALDI-TOF/MS) and HPLC Photodiode Array Detector coupled to a hybrid Quadrupole Time of Flight Mass Spectrometry (HPLC-PDA-QTOF/MS). MALDI-TOF/MS failed to detect non-polar MCs, such as MC-LY and MC-LW. HPLC-QTOF/MS permitted the accurate identification of most MCs present in methanolic extracts. Besides, three new MCs, namely: [D-Glu(OCH₃)⁶, D-Asp³] MC-LAba, MC-YL and MC-YM were detected by HPLC-QTOF/MS.     

Survey of cyanobacterial toxins in Czech water reservoirs—the first observation of neurotoxic saxitoxins

The environmental occurrence and concentrations of cyanobacterial toxins (cyanotoxins) were investigated in the Czech Republic. Concentrations of microcystins (MCs), cylindrospermopsin (CYN) or saxitoxins (STXs) were determined immunochemically by ELISA assays in 30 water samples collected from the surface layers of 19 reservoirs during the summer season of 2010. MCs were detected in 18 reservoirs and 83 % of samples, with median and maximal concentration being 1.5 and 18.6 μg/L, respectively. The high frequency of MC occurrence coincided with prevalence of cyanobacterium Microcystis sp., which was detected in 87 % samples, followed by Dolichospermum (Anabaena) sp. observed in 33 % samples. CYN was detected by ELISA only in one sample at a concentration of 1.2 μg/L. STXs presence was indicated for the first time in Czech water reservoirs when the toxins were found at low concentrations (0.03–0.04 μg/L) in two samples (7 %) collected from two different reservoirs, where STXs co-occurred with MCs and eventually also with CYN. In both STX-positive samples, the phytoplankton community was dominated by Microcystis sp., but Dolichospermum sp. and/or Aphanizomenon sp. were also present as putative producers of STX and/or CYN. Cyanotoxins commonly occurred in Czech water reservoirs, and MCs frequently at concentrations possibly associated with human health risks. MCs were the most prevalent and abundant cyanotoxins, but also other cyanotoxins were detected, though sporadically. Further research and regulatory monitoring of cyanotoxins other than MCs is therefore required.     

Removal of Microcystins by Phototrophic Biofilms. A Microcosm Study (6 pp)

Background, Aims and Scope Microcystins (MCs) are a family of natural toxins produced by cyanobacteria (blue-green algae). As a result of eutrophication, massive cyanobacterial blooms occur more frequently and MCs represent important contaminants of freshwater ecosystems. Bacterial biodegradation is considered a main mechanism for MC breakdown in environmental conditions. While existing studies were mostly focused on MC biodegradation by planktonic bacteria, our experiments examined the fate and kinetics of MC degradation in river-originated phototrophic biofilms and investigated factors influencing the rate of MC removal. Methods The fate of dissolved MCs was studied in laboratory microcosms with different composition (containing water only, water with phytoplankton and/or phototrophic biofilms). Biofilms originated from river ecosystem were pre-incubated under various conditions (with/without presence of cyanobacterial biomass or model organic substrates: glucose and protein - casein). Changes in MC concentration (0-14 days) in water columns were measured by HPLC DAD after external additions of purified MCs (160 μg L-1, MC-LR and MC YR), and halftimes (t1/2) of MC removal were estimated. Results and Discussion The slow degradation of MC was revealed in tap water (t1/2 ~ 14 days) and river water without cyanobacteria (t1/2 ~ 8 days). Enhanced removal occurred in the presence of natural planktonic cyanobacteria (t1/2 ~ 44 h), most probably due to microorganisms associated with the biomass of cyanobacterial bloom. More rapid MC elimination occurred in the variants containing phototrophic biofilms, and was particularly pronounced at those biofilms pre-cultivated in the presence of cyanobacterial blooms (t1/2 ~ 20 h). Much slower removal was observed in the variants simulating possible substrate-dependent induction of microorganism metabolism (biofilms pre-incubated with glucose: t1/2 ~ 35 h, and casein: t1/2 ~ 80 h). After termination of experiments, total amounts of MCs accumulated in the biofilms were below 5% of the initial toxin level revealing significant biodegradation processes. Conclusion The microcosm studies contributed to understanding of the environmental fate of MCs and revealed a rapid biodegradation by phototrophic biofilms. The rate of MC elimination depends on history of biofilm community, previous contact with cyanobacteria seems to be a selective factor improving the biodegradation potential. Recommendation and Outlook Our results experimentally showed a positive role of biofilms in MC elimination during water treatment processes such as bank filtration or slow sand filtration, and could eventually serve for further research of biofilm-based technological applications for MCs removal in small-scale drinking water treatment facilities.