铜绿微囊藻光合活性对LED光短期暴露的响应

为探究LED光对蓝藻光合活性的影响,以铜绿微囊藻Microcystis aeruginosa PCC 7806为对象, 25μmol photons/(m²·s)白色荧光灯为对照,检测了不同光质光强LED处理2h的光合活性。结果表明,与对照相比,25—50μmol photons/(m²·s) LED红光和蓝光、25—100μmol photons/(m²·s) LED白光和绿光处理下,细胞光合活性(F_v/F_m)显著提高。大于100μmol photons/(m²·s)的LED红光和蓝光、大于200μmol photons/(m²·s)的LED白光及大于500μmol photons/(m²·s)的LED绿光处理对光合活性有显著抑制作用,光系统Ⅱ(PSⅡ)最大光化学效率F_v/F_m、电子传递速率ETR(Ⅱ)、光量子产量Y(Ⅱ)、光系统Ⅰ(PSⅠ)电子传递速率ETR(Ⅰ)、...     

从种群竞争的角度初步研究微囊藻的产毒机理

采用将微囊藻和栅藻混合培养的方法,从种群竞争的角度初步探讨了微囊藻毒素的产毒机理,结果显示：当起始接种浓度相同时,混合培养组比纯微囊藻培养组产生更多的毒素,由于其它培养条件完全一致,所以推论是由于栅藻的存在,增加了微囊藻的生存压力。当起始接种浓度微囊藻：栅藻为10：1时,此混合培养组比纯微囊藻产生的毒素少,并且毒素降解也更快,推论原因是微囊藻在种群数量上远远超过栅藻,竞争压力较小,同时由于栅藻的存在,增加了培养液中色素的含量,加快了光降解的速度。     

金藻吞噬微囊藻产生的无毒变异株与产毒原始株的比较

分别从喂食三株原始产毒铜绿微囊藻Microcystis aeruginosa(AC、DS和PCC 7820)的金藻Poterioochromonassp.培养物中获得三株藻,以Nest PCR方法(引物对CC/CG和CH/CI)确定此三株藻均为微囊藻属藻株.HPLC测试结果显示这三株藻均不产生微囊藻毒素.显示Poterioochromonas sp.具有将产毒微囊藻转化为尤毒微囊藻的能力.比较产毒原始株与无毒变异株的生理特性发现,变异株的类胡萝卜素/叶绿素比值高于原始株;而光反应曲线结果表明,变异株的PSⅡ的量子产率和光合作用活力高于原始产毒株,并且变异株在较低光强下就可达到最大的光合作用活力.显示喂食后产生的变异株比原始株有较高的光合作用效率.变异株的藻蓝蛋白/叶绿素比值则低于原始株,光合作用最适光强低于变异株,并且显示产毒原始株通过增加藻蓝蛋白的相对含量来提高对光照的吸收.变异株具有较高的光合作用效率和藻蓝蛋白含量可能是其能够在微囊藻和金藻混合培养的群体中占优势的原因之一.     

光强对微囊藻群体形态的影响及其生理机制研究简

为了探讨光照对微囊藻形态的影响,研究了6株不同种的群体微囊藻在不同光强下群体形态的变化及其响应机制。研究发现,随着光强的增加,6株群体微囊藻的群体尺寸变大。当光强为80—200μmol/(m2·s)时,群体微囊藻DH-M1和DC-M2的比生长速率显著增大,而另4株在高光强下比生长速率无显著性差异;对多糖含量分析发现,高光强对群体微囊藻TH-M2、DC-M1、FACHB1174和FACHB1027胞外及胶被多糖的分泌与释放有显著的促进效果,而DH-M1和DC-M2多糖含量增加不明显。对于不同的微囊藻株,高光强促进群体形态变化的作用机理不同:光饱和点低的微囊藻是通过分泌大量的胞外及胶被多糖使群体尺寸变大,而光饱和点高的微囊藻是通过生长来促进群体尺寸的增大。此外,对产毒藻株在不同光强下的毒素基因表达及胞内毒素测定发现,高光强组的群体微囊藻mcyB和mcyD表达量升高,且胞内微囊藻毒素含量增加显著,推测微囊藻毒素也可能是影响微囊藻群体形态及大小的作用因子之一。     

荧光原位杂交技术和流式细胞仪用于环境样品中产毒及非产毒微囊藻的定量监测

全球范围内,高频次、大范围暴发的蓝藻水华对淡水水体环境造成严重影响.微囊藻因其在生长特别是衰亡过程中向水体释放微囊藻毒素而威胁人类健康.因此,分析其产毒株及非产毒株在环境样品中的组成,建立产毒蓝藻的预报及评价体系显得极为重要.本文采用荧光原位杂交技术结合流式细胞技术实现对环境样品中产毒藻株的鉴别与定量.针对目标基因mcyA设计的、以地高辛标记的双链DNA探针可有效应用于产毒微囊藻FACHB905和PCC7806的鉴别.分别对来自滇池、太湖和关桥的11个样品进行分析显示,该方法与传统的形态学鉴定及PCR方法有较好的匹配.荧光原位杂交技术与流式细胞相结合可有效鉴别产毒与非产毒微囊藻,尤其可以对野外样品中产毒与非产毒藻株进行简便、可视化地鉴别,从而达到对产毒微囊藻水华早期预警的目的.     

阴离子表面活性剂LAS对产毒和无毒微囊藻生长及产毒特性的影响

文章研究了低浓度范围内不同浓度梯度的阴离子表面活性剂直链烷基苯磺酸盐(LAS)对产毒微囊藻(Microcystis aeruginosa, FACHB905)和无毒微囊藻(Microcystis wesenbergii, FACHB908)生长、光合特性、种间竞争及毒素合成的影响。结果表明,在0.05—5.0 mg/L LAS浓度梯度处理下,产毒微囊藻的生物量、产毒基因mcyD表达量和每细胞MCs含量均在培养12d后显著增加。产毒微囊藻胞内和胞外MCs含量在各LAS浓度处理后分别为0.069、0.052、0.061、0.038和0.037 fg/fg Chl.a及107.1、103.7、127.1、99.6和113.7 ng/L。即使在0.5 mg/L低浓度LAS处理条件下,上述3个参数也分别比对照组显著增加了24.2%、12.4倍和10.4%。浓度为0—0.2 mg/L LAS对无毒微囊藻的生物量无明显影响,而较高浓度的LAS(0.5—5.0 mg/L)明显抑制了无毒微囊藻的生长。在两株微囊藻混合培养时, 0.2—1.0 mg/L LAS处理组的产毒铜绿微囊藻mcy D的表达对LAS...     

微囊藻对柔细束丝藻生长及土臭素合成与释放的影响

文章选择两种特征不同的微囊藻——产毒的铜绿微囊藻(Microcystis aeruginosa)和无毒的惠氏微囊藻(Microcystis wesenbergii),分别以不同的接种比例(1﹕2、1﹕1和2﹕1)与产土臭素(Geosmin)的柔细束丝藻(Aphanizomenon gracile)混合培养,以探索种间相互作用对藻类生长和束丝藻土臭素合成与释放的影响。结果表明,在共培养条件下,两种微囊藻均抑制了柔细束丝藻的生长,而柔细束丝藻却促进了两种微囊藻的生长。惠氏微囊藻促进了柔细束丝藻土臭素的释放(接种比例为1﹕1时,束丝藻胞外土臭素的细胞份额达到269.43 fg/cell),仅在生长早期与生长受到抑制阶段促进了土臭素的合成;铜绿微囊藻在共培养早期促进了束丝藻土臭素的合成,但共培养却抑制了土臭素的释放,而且在共培养的中后期已检测不到土臭素。研究结果表明,在自然水体中束丝藻与微囊藻的季节演替过程中,微囊藻在与束丝藻的竞争中处于优势,且微囊藻对束丝藻的竞争压力促使后者合成异味物质,随着束丝藻的消亡可能伴随大量异味物质的释放,增加异味事件发生风险。     

光强对微囊藻群体形态的影响及其生理机制研究

为了探讨光照对微囊藻形态的影响,研究了6株不同种的群体微囊藻在不同光强下群体形态的变化及其响应机制。研究发现,随着光强的增加,6株群体微囊藻的群体尺寸变大。当光强为80200 mol/（m2s）时,群体微囊藻DH-M1和DC-M2的比生长速率显著增大,而另4株在高光强下比生长速率无显著性差异;对多糖含量分析发现,高光强对群体微囊藻TH-M2、DC-M1、FACHB1174和FACHB1027胞外及胶被多糖的分泌与释放有显著的促进效果,而DH-M1和DC-M2多糖含量增加不明显。对于不同的微囊藻株,高光强促进群体形态变化的作用机理不同:光饱和点低的微囊藻是通过分泌大量的胞外及胶被多糖使群体尺寸变大,而光饱和点高的微囊藻是通过生长来促进群体尺寸的增大。此外,对产毒藻株在不同光强下的毒素基因表达及胞内毒素测定发现,高光强组的群体微囊藻mcyB和mcyD表达量升高,且胞内微囊藻毒素含量增加显著,推测微囊藻毒素也可能是影响微囊藻群体形态及大小的作用因子之一。       

温、光、盐对硅藻STR01生长、总脂、脂肪酸的影响

为了优化新分离STR01的生态培养条件, 采用单因子试验和正交试验研究了不同温度、光照强度、盐度和温、光、盐三因素三水平对该藻的生长、总脂和脂肪酸组成影响。结果表明: 温、光、盐对STR01的生长、总脂和脂肪酸组成影响显著(P<0.05)。生长的适宜温度为15—35℃, 最适25—30℃(K值达0.679—0.682), 总脂含量积累的最适温度是25℃(总脂可达17.23%), 温度20℃时有利于该藻PUFA的积累, 可达34.23%。STR01生长的适宜光照强度为40—120 μmol/(m2·s), 最适光强为60 μmol/(m2·s), 光照强度40 μmol/(m2·s)有利于该藻的PUFA积累, 可达34.29%。STR01生长的适宜盐度为10—35, 最适盐度25, 盐度25时PUFA含量较高(43.42%)。正交试验结果表明温度对STR01的平均相对生长速率和总脂含量影响显著, 生长的最优组合: 温度30℃、光照强度60 μmol/(m2·s)、盐度25, 该组合下的生长速率达0.756; 总脂含量积累的最优组合: 温度30℃、光照强度60 μmol/(m2·s)、盐度20, 该组合下的总脂含量为20.00%。PUFA的最优组合: 温度25℃、光照强度60 μmol/(m2·s)、盐度20, 该组合下PUFA的含量为35.37%。综上所述: 该藻生长迅速, 总脂含量较高, PUFA丰富, 是一种可开发利用的耐高温浮游硅藻。     

滇池水华蓝藻铜锈微囊藻和绿色微囊藻的生长生理特性及毒素分析

从滇池分离纯化了两种常见水华微囊藻即铜锈微囊藻和绿色微囊藻。在常规培养条件下,两种藻类在对数生长期的生长速率μ值分别为0.61和0.63;早期生长的抑制光强不大于100μmol m~(-2)s~(-1)。铜锈微囊藻主要产生3种微囊藻毒素:MYCST-RR,MYCST-YR和MYCST-LR,绿色微囊藻产生的主要微囊藻毒素为[Dha~7]-MYCST-RR,和[Dha~7]-MYCST-LR,另含有少量的[Dha~7]-MYCST-YR。在低光强15μE m~(-2)s~(-1)时,毒素含量每毫克干重细胞达到3.127μg微囊藻毒素,当光强达到100μE m~(-2)s~(-1)时,毒素含量降低到每毫克干重细胞1.971μg;光强对毒素形成的影响受到温度的调节,而温度对毒素形成的影响不大。探讨了两种微囊藻细胞在不同光照强度下叶绿素荧光比值Fv/Fm的变化,此比值的变化可以间接反映细胞受外界光照强度抑制程度。     

Competition between a toxic and a non-toxic <Emphasis Type="Italic">Microcystis</Emphasis> strain under constant and pulsed nitrogen and phosphorus supply

The toxicity of a harmful algal bloom is strongly determined by the relative abundance of non-toxic and toxic genotypes and might therefore be regulated by competition for growth-limiting resources. Here, we studied how the toxic Microcystis aeruginosa strain PCC 7806 and a non-toxic mutant compete for nitrogen and phosphorus under constant and pulsed nutrient supply. Our monoculture and competition experiments show that these closely related genotypes have distinct nutrient physiologies and that they differ in their ability to compete for nitrogen and phosphorus. The toxic wild type won the competition under nitrogen limitation, while the non-toxic mutant dominated under phosphorus limitation. Pulses of both nitrogen and phosphorus increased the dominance of the toxic genotype, which lead to an even faster competitive exclusion of the non-toxic genotype under nitrogen pulses and to coexistence of both genotypes under phosphorus pulses. Our findings indicate that the genotype level dynamics driven by resource competition can be an important factor in determining cyanobacterial bloom toxicity.     

Reversal in competitive dominance of a toxic versus non-toxic cyanobacterium in response to rising CO2

Climate change scenarios predict a doubling of the atmospheric CO₂ concentration by the end of this century. Yet, how rising CO₂ will affect the species composition of aquatic microbial communities is still largely an open question. In this study, we develop a resource competition model to investigate competition for dissolved inorganic carbon in dense algal blooms. The model predicts how dynamic changes in carbon chemistry, pH and light conditions during bloom development feed back on competing phytoplankton species. We test the model predictions in chemostat experiments with monocultures and mixtures of a toxic and non-toxic strain of the freshwater cyanobacterium Microcystis aeruginosa. The toxic strain was able to reduce dissolved CO₂ to lower concentrations than the non-toxic strain, and became dominant in competition at low CO₂ levels. Conversely, the non-toxic strain could grow at lower light levels, and became dominant in competition at high CO₂ levels but low light availability. The model captured the observed reversal in competitive dominance, and was quantitatively in good agreement with the results of the competition experiments. To assess whether microcystins might have a role in this reversal of competitive dominance, we performed further competition experiments with the wild-type strain M. aeruginosa PCC 7806 and its mcyB mutant impaired in microcystin production. The microcystin-producing wild type had a strong selective advantage at low CO₂ levels but not at high CO₂ levels. Our results thus demonstrate both in theory and experiment that rising CO₂ levels can alter the community composition and toxicity of harmful algal blooms.     

Iron uptake by toxic and nontoxic strains of Microcystis aeruginosa

Iron uptake by microcystin-producing and non-microcystin-producing strains of Microcystis aeruginosa was investigated through short-term uptake assays. Although strain-specific differences were observed, the siderophore-independent Fe uptake kinetics were essentially similar (e.g., maximum uptake rates of 2.0 to 3.3 amol·cell(-1)·h(-1)) for the wild-type toxic strain PCC7806 and a genetically engineered mutant unable to produce microcystin.     

Immunogold localisation of microcystins in cryosectioned cells of Microcystis

Insights into the origins, function(s), and fates of cyanobacterial toxins may be obtained by an understanding of their location within cyanobacterial cells. Here, we have localised microcystins in laboratory cultures of Microcystis PCC 7806 and PCC 7820 by immunogold labelling. Cryosectioning was used for immunoelectron microscopy since microcystins were extracted during the ethanol-based dehydration steps routinely used for sample preparation. Microcystins were specifically localised in the nucleoplasm and were associated with all major inclusions of the microcystin-producing strains Microcystis PCC 7806 (MC(+)) and Microcystis PCC 7820, and labelling was preferentially associated with the thylakoids and around polyphosphate bodies. A mutant strain of Microcystis PCC 7806 (MC(-)) which does not produce microcystins was used as a control. Distribution of total gold label within each cell region or associated with inclusions indicated that most of the cells' microcystin pool was associated with the thylakoids (69%, PCC 7806 (MC(+)); 78%, PCC 7820), followed by the nucleoplasmic region (19%, PCC 7806 (MC(+)); 12%, PCC 7820). Cryosectioning is a useful technique since it reduces the extraction of microcystins during sample preparation for electron microscopy.     

Effects of light on the microcystin content of Microcystis strain PCC 7806

Many cyanobacteria produce microcystins, hepatotoxic cyclic heptapeptides that can affect animals and humans. The effects of photosynthetically active radiation (PAR) on microcystin production by Microcystis strain PCC 7806 were studied in continuous cultures. Microcystis strain PCC 7806 was grown under PAR intensities between 10 and 403 micro mol of photons m(-2) s(-1) on a light-dark rhythm of 12 h -12 h. The microcystin concentration per cell, per unit biovolume and protein, was estimated under steady-state and transient-state conditions and on a diurnal timescale. The cellular microcystin content varied between 34.5 and 81.4 fg cell(-1) and was significantly positively correlated with growth rate under PAR-limited growth but not under PAR-saturated growth. Microcystin production and PAR showed a significant positive correlation under PAR-limited growth and a significant negative correlation under PAR-saturated growth. The microcystin concentration, as a ratio with respect to biovolume and protein, correlated neither with growth rate nor with PAR. Adaptation of microcystin production to a higher irradiance during transient states lasted for 5 days. During the period of illumination at a PAR of 10 and 40 micro mol of photons m(-2) s(-1), the intracellular microcystin content increased to values 10 to 20% higher than those at the end of the dark period. Extracellular (dissolved) microcystin concentrations were 20 times higher at 40 micro mol of photons m(-2) s(-1) than at 10 micro mol of photons m(-2) s(-1) and did not change significantly during the light-dark cycles at both irradiances. In summary, our results showed a positive effect of PAR on microcystin production and content of Microcystis strain PCC 7806 up to the point where the maximum growth rate is reached, while at higher irradiances the microcystin production is inhibited.     

Competition between toxic Microcystis aeruginosa and nontoxic Microcystis wesenbergii with Anabaena PCC7120

To elucidate the changes in the proportions of microcystin (MC)-producing Microcystis, non-MC-producing Microcystis and Anabaena strains during cyanobacteria blooms, we compared their fitness under different initial biomass ratios. Culture experiments were carried out with three cyanobacterial strains: single-celled toxic Microcystis aeruginosa PCC7806 (Ma7806), single-celled nontoxic Microcystis wesenbergii FACHB-929 (Mw929) and filamentous Anabaena PCC7120 (An7120). Growth curves expressed as biovolume, Ma7806 microcystin-LR (MC-LR) content (detected with HPLC and ELISA), and the culture medium dissolved total nitrogen and dissolved total phosphorous (DTP) were measured to monitor nutrient uptake. Results suggest that the dominant strain in competition experiments between Ma7806 and An7120 was mainly controlled by the initial biomass ratio of the two strains, but there was also evidence for allelopathic interactions, where MC-LR produced by Ma7806 played an important role in the competition process. However, Mw929 was always less competitive when co-cultured with An7120 regardless of initial biomass ratio. Culture medium DTP showed significant differences between competition experiments in all sets, suggesting that Mw929 could be more suited to low phosphorus environments than Ma7806 and An7120. Overall, the competitive ability of Ma7806 was stronger than Mw929 when co-cultured with An7120 in the case of excess nutrients and the results could well unravel the seasonal succession process of cyanobacteria blooms.     

Toxicity and extrachromosomal DNA in strains of the cyanobacterium Microcystis aeruginosa

Abstract Correlations were sought between toxicity and the presence of plasmids in toxic and non-toxic strains of Microcystis aeruginosa . Plasmids were present in toxic and non-toxic cultures. Cultivation of the toxic Microcystis PCC7820 in the presence of novobiocin did not influence toxicity, although extrachromosomal DNA was no longer detected after novobiocin treatment. The data indicate that it is unlikely that plasmids are involved in the toxicity of Microcystis PCC7820.     

黑暗限气条件下铜绿微囊藻细胞死亡的形态结构和生理生化变化

【目的】研究铜绿微囊藻细胞死亡过程中形态和生理生化变化,探讨蓝藻细胞死亡机制。【方法】通过黑暗限气处理模拟水华爆发后期水体环境,在处理后不同时间取样,对藻液的OD值,溶氧含量和pH值进行监测,使用透射电镜对细胞形态结构变化进行观察,通过胱天蛋白酶(Cysteine-dependent aspartate specificprotease,Caspase)活性检测、活性氧含量测定、末端脱氧核糖核酸转移酶介导的dUTP缺口末端标记(Terminal deoxynucleotidyl transferase-mediated dUTP nick end-labeling,TUNEL)染色和琼脂糖凝胶电泳对处理后藻细胞的死亡生理进行研究。【结果】黑暗限气处理后,藻培养液pH值和溶解氧含量下降,处理12 h后藻液开始变黄,48 h后藻细胞全部死亡。电镜观察结果表明,藻细胞在黑暗限气处理所导致的死亡过程中出现空泡和类囊体、核糖体等内部结构解体但细胞壁仍保持完整等现象。活性氧含量和caspase活性检测表明,在藻细胞死亡过程中活性氧含量和caspase活性上升。TUNEL染色和琼脂糖凝胶电泳分析发现,藻细胞在死亡过程中DNA发生断裂和降解。【结论】铜绿微囊藻细胞在黑暗和限气处理中表现出和真核生物细胞程序性死亡相类似的死亡特征,这说明细胞死亡机制是保守的,原核细胞和真核细胞一样具有程序性死亡机制。     

Functional analysis of PilT from the toxic cyanobacterium Microcystis aeruginosa PCC 7806

The evolution of the microcystin toxin gene cluster in phylogenetically distant cyanobacteria has been attributed to recombination, inactivation, and deletion events, although gene transfer may also be involved. Since the microcystin-producing Microcystis aeruginosa PCC 7806 is naturally transformable, we have initiated the characterization of its type IV pilus system, involved in DNA uptake in many bacteria, to provide a physiological focus for the influence of gene transfer in microcystin evolution. The type IV pilus genes pilA, pilB, pilC, and pilT were shown to be expressed in M. aeruginosa PCC 7806. The purified PilT protein yielded a maximal ATPase activity of 37.5 +/- 1.8 nmol P(i) min(-1) mg protein(-1), with a requirement for Mg(2+). Heterologous expression indicated that it could complement the pilT mutant of Pseudomonas aeruginosa, but not that of the cyanobacterium Synechocystis sp. strain PCC 6803, which was unexpected. Differences in two critical residues between the M. aeruginosa PCC 7806 PilT (7806 PilT) and the Synechocystis sp. strain PCC 6803 PilT proteins affected their theoretical structural models, which may explain the nonfunctionality of 7806 PilT in its cyanobacterial counterpart. Screening of the pilT gene in toxic and nontoxic strains of Microcystis was also performed.