Zn~(2+)浓度对固氮鱼腥藻(Anabaena azotica Ley)光能转化特性的影响

本实验对在不同Zn2+浓度条件下培养的固氮鱼腥藻(Anabaena azoticaLey)的生长、光合放氧速率和叶绿素荧光参数Fv/Fm进行了测定.结果表明,当Zn2+浓度为1.0μmol/L时,其比生长速率(Specific growth rate)最大,光合放氧速率和Fv/Fm值最高.当Zn2+浓度大于等于5.0μmol/L时会抑制A.azotica Ley的生长和光合作用.对在0μmol/L和5.0μmol/L Zn2+浓度下生长的藻细胞藻胆体-类囊体膜复合物吸收光谱的比较和对与5.0μmol/L

鱼腥藻Anabaena PCC7120原生质球和液泡的同步诱导

国家自然科学基金资助项目( 39870 0 83)

蓝藻Anabaena sp.PCC7120 羧体碳酸酐酶的鉴定

在丝状蓝藻Anabaena sp.PCC7120细胞粗提液的碳酸酐酶(CA)分析中,发现了两种形式的CA活性.高CO_2下生长的细胞,在35μmol/L EZ(Ethoxyzolamide,碳酸酐酶的抑制剂)存在的情况下,CA总活性的85％左右被抑制,其半抑制浓度I_(50)为7.4μmol/L;随着EZ浓度的继续增加,CA活性在EZ浓度达到约150μmol/L处出现了第二个抑制峰,在250μmol/L处抑制程度达到最大,使CA总活性的15％被抑制,其半抑制浓度I_(50)为190μmol/L。在空气条件

鱼腥藻（Anabaena sp．）营养成分分析

研究分析了混合鱼腥藻粉的营养成分，结果表明混合鱼腥藻粉蛋白质含量为４０．５％；氨基酸组成符合联合国粮农卫生组织（ＦＡＯ／ＷＨＯ）规定的标准；并含有较丰富的糖类、脂肪酸、无机元素和色素。证实了鱼腥藻可以作为蛋白饲料资源开发和利用。

固氮蓝藻Anabaena sp.7120的叶绿素蛋白复合体的分离和光谱特性的研究

用光合膜片增溶和SDS-聚丙烯酰胺凝胶电泳方法,从固氮蓝藻Anabaena sp.7120分离到7条色素带。迁移率较慢的五条叶绿素蛋白复合体带,具有相同的吸收光谱和室温荧光光谱特性。它们的红区最大吸收峰在676nm;蓝区最大吸收峰在438nm。它们的室温荧光发射最高峰在672—673nm;在710,732和740nm都有小峰。这些是CPⅠ叶绿素所特有的。我们认为这5条带都是属于光系统Ⅰ的叶绿素蛋白复合体。另一条迁移率稍快的叶绿素蛋白复合体带为CPⅡ。它的红区最大吸收峰在672nm;蓝区最大吸收峰在436n

纯化柱胞鱼腥藻(Anabaena cylindrca)固氮酶组份(铁蛋白)的厌氧制备电泳法

<正> 各种固氮生物的固氮酶对氧都很敏感,无论是制备固氮酶的组份Ⅰ(钼铁蛋白)或组份Ⅱ(铁蛋白),也无论采取什么方法(如DEAE-纤维素层析法、硫酸鱼精朊沉淀法、胶滤、制备凝胶电泳等等)都必需在严格厌氧条件下进行,铁蛋白对氧更加敏感,因此要获得较纯而又具活力的铁蛋白,其分离、纯化过程既要严格厌氧又要迅速。到目前为止,仅红螺菌(Rhodospirillum rubrum)和棕色

鱼腥藻(Anabaena 7120)DNA的转化作用

用化学方法从固氮蓝藻鱼腥藻(Anabaena 7120)细胞中有效地提取了DNA,以此为供体DNA,用它的氧敏感固氮突变种鱼腥藻一1(Anabaena-l)为受体进行转化实验。在大量的转化实验中,仅有两次获得转化后的突变种在空气中、在无氮培养基上能生长,其转化频率为10~(-6)—10~(-5)。转化子在有氧条件下的乙炔还原活力相当于野生种。它表明突变种的除氧系统通过转化而得到恢复。推测鱼腥藻7120突变种可能具有吸收和整合外源DNA的能力。对丝状蓝藻转化困难的原因进行了探讨,结果表明受体藻胞外DNA酶活

鱼腥藻(Anabaena)对氧敏感的固氮突变种

用紫外线和亚硝基胍,诱变筛选出两株具异形胞而不能在空气中固定分子氮的鱼腥藻Anabaena)突变种。突变表型是稳定的。在微氧条件下,能固定分子氮而生长,但固氮酶活很弱。酶活的高低与藻蓝素含量和光照强度成反相关。突变种细胞的固氮酶对氧非常敏感,反应气相中加入1%的氧对乙炔还原活力已有明显抑制,20%的氧完全阻抑固氮作用。除去氧后固氮酶重新合成,其过程受 NH_4~+和氯霉素阻遏。通过氮饥饿使藻蓝素含量降低,或降低光照强度,或加入二氯苯基甲基脲抑制光合放氧时,均可显著地提高突变种的固氮酶活力。突变种细胞还原氯

Outer membrane proteins induced by iron deficiency in Anabaena sp PCC 7120

Iron deficiency can induce cyanobacteria to synthesize siderophore receptor proteins on the outer membrane to enhance the uptake of iron. In this study, an outer membrane of high purity was prepared from Anabaena sp. PCC 7120 based on aqueous polymer two-phase partitioning and discontinuous sucrose density ultra-centrifugation, and the induction of outer membrane proteins by iron deficiency was investigated using 2-D gel electrophoresis. At least. five outer membrane proteins were newly synthesized or significantly up-regulated in cells transferred to iron-deficient conditions, which were all identified to be siderophore receptor proteins according to MALDI-TOF-MS analyses. Bacterial luciferase reporter genes luxAB were employed to monitor the transcription of the encoding genes. The genes were induced by iron deficiency at the transcriptional level in different responsive modes. Luciferase activity expressed from an iron-regulated promoter may be used as a bioreporter for utilizable iron in natural water samples. (C) 2009 National Natural Science Foundation of China and Chinese Academy of Sciences. Published by Elsevier Limited and Science in China Press. All rights reserved.

Mouse Toxicity of Anabaena flos-aquae from Lake Dianchi, China

Some species of the genera Anabaena can produce various kinds of cyanotoxins, which may pose risks to environment and human health. Anabaena has frequently been observed in eutrophic freshwater of China in recent years, but its toxicity has been reported only in a few studies. In the present study, the toxicity of an Anabaena flos-aquae strain isolated from Lake Dianchi was investigated. Acute toxicity testing was performed by mouse bioassay using crude extracts from the lyophilized cultures. The mice exposed to crude extracts showed visible symptoms of toxicity and died within 10-24 h of the injection. Serum biochemical parameters were evaluated by the use of commercial diagnostic kits. Significant alterations were found in the serum biochemical parameters: alkaline phosphatase (AKP), gamma-glutamyl transpepticlase (gamma-GT), aspartate amino transferase (AST), alanine amino transferase (ALT), AST/ALT ratio, total protein content, albumin content, albumin/globulin (A/G) ratio, blood urea nitrogen (BUN), serum creatinine (Ssr), and total antioxidative capacity (T-AOC). Histopathological observations were carried out with hematoxylin and eosin (HE) stain under light microscope. Severe lesions were seen in the livers, kidneys, and lungs of the mice injected with crude extracts. The alterations of biochemical parameters were in a dose-dependent manner, and the severities of histological lesions were in the same manner. Based on biochemical and histological studies, this research firstly shows the presence of toxin-producing Anabaena species in Lake Dianchi and the toxic effects of its crude extracts on mammals. (C) 2008 Wiley Periodicals, Inc. Environ Toxicol 24: 10-18, 2009.

Morphological characteristics and phylogenetic relationship of Anabaena species from Lakes Dianchi and Erhai, China

Although Anabaena is one of the most prevalent planktonic freshwater genus in China, there are few taxonomic reports of Anabaena strains by morphology and genetics. In this study, morphological characteristics and phylogenetic relationships of seven Anabaena strains isolated from two plateau lakes, Lakes Dianchi and Erhai, were investigated. Morphological characteristics such as morphology of filament, cellular shapes and sizes, relative position of heterocytes and akinetes, and presence or absence of aerotopes, were described for these seven strains. Phylogenetic relationships were determined by constructing 16S rRNA gene tree using the neighbor-joining algorithm. The seven strains were morphologically identified as three groups, and phylogenetic analysis based on 16S rRNA gene sequences also showed that these seven strains were in three groups. Strains EH-2, EH-3, and EH-4 were in group A belonging to the Anabaena circinalis and A. crassa group, and strains DC-1, DC-2, and EH-1 were in group B and identified as A. flos-aquae. Strain DC-3 without aerotopes was significantly different from the other isolated strains and was determined as A. cylindrica.

A gene cluster that regulates both heterocyst differentiation and pattern formation in Anabaena sp strain PCC 7120

Wild-type Anabaena sp. strain PCC 7120, a filamentous nitrogen-fixing cyanobacterium, produces single heterocysts at semi-regular intervals. asr0100 (patU5) and alr0101 (patU3) are homologous to the 5' and 3' portions of patU of Nostoc punctiforme. alr0099 (hetZ) overlaps the 5' end of patU5. hetZ, patU5 and patU3 were all upregulated, or expressed specifically, in proheterocysts and heterocysts. Mutants of hetZ showed delayed or no heterocyst differentiation. In contrast, a patU3 mutation produced a multiple contiguous heterocyst (Mch) phenotype and restored the formation of otherwise lost intercalary heterocysts in a patA background. Decreasing the expression of patU3 greatly increased the frequency of heterocysts in a mini-patS strain. Two promoter regions and two principal, corresponding transcripts were detected in the hetZ-patU5-patU3 region. Transcription of hetZ was upregulated in a hetZ mutant and downregulated in a patU3 mutant. When mutants hetZ::C.K2 and hetZ::Tn5-1087b were nitrogen-deprived, P-hetC-gfp was very weakly expressed, and in hetZ::Tn5-1087b, P-hetR-gfp was relatively strongly expressed in cells that had neither a regular pattern nor altered morphology. We conclude that the hetZ-patU5-patU3 cluster plays an important role in co-ordination of heterocyst differentiation and pattern formation. The presence of homologous clusters in filamentous genera without heterocysts is suggestive of a more general role.