集胞藻Synechocystis sp.PCC 6803脂质组的分析

以集胞藻Synechocystis sp.PCC 6803为研究对象,研究建立了基于超高效液相色谱耦合串联质谱技术脂质组学分析方法.鸟枪法脂质组学通过电喷雾离子化有效分离油脂粗提物中所含单个脂质分子,在三重四极杆扫描碎片离子,能够利用特征片段离子鉴定光合甘油酯的种类和酰基组成,具有高效、灵敏度高和质量准确度高等优点.对...     

蓝细菌Synechocystis sp.PCC6803中叶绿素合成调控类囊体膜重建的研究

利用ＤＮＡ体外重组技术构建了蓝细菌Ｓｙｎｅｃｈｏｃｙｓｔｉｓｓｐ．ＰＣＣ６８０３突变种ＯＲＦ４６９,它的染色体ＤＮＡ缺失ＯＲＦ４６９片段,该突变种在加入５ｍｍｏｌ／Ｌ葡萄糖的ＢＧ－１１培养基中经遮光培养２周后叶绿素全部消失,细胞甲醇提取液光谱中６６５ｎｍ处叶绿互峰消失,６２９ｎｍ处出现原叶绿素酸酯峰,完整细胞光谱仅存在６２０ｎｍ的藻胆蛋白肩峰,细胞的类囊体膜消失,但藻胆体颗粒并未减少;细胞培养物重     

硫代硫酸钠和葡萄糖对Synechocystis sp.PCC 6803细胞甘油酯及其脂肪酸组成的影响

对生长在添加有不同浓度的葡萄糖、硫代硫酸钠培养基中的蓝细菌Synechocystis sp.PCC 6803中的甘油酯及其脂肪酸组成进行比较.结果表明:硫代硫酸钠能有效地增加膜脂中硫代异鼠李糖二酰基甘油(SQDG)和磷脂酰甘油(PG)的百分含量,培养基中同时添加葡萄糖时能抵消硫代硫酸钠的这一效应.此外,硫代硫酸钠能显著增加单半乳糖甘油二酯(MGDG)、双半乳糖甘油二酯(DGDG)中十六碳酸(C16:0)的百分含量,这一效应也能为葡萄糖消除.硫代硫酸钠不能显著地改变SQDG中C16:0的百分含量,加入葡萄糖时能降低C16:0的百分含量.这些结果说明硫代硫酸钠可能充当一种还原剂使膜脂处于一种低的不饱和状态,同时加入葡萄糖时能降低硫代硫酸钠的还原力.此外,硫代硫酸钠还可作为SQDG合成中的硫供体.     

质体醌库和细胞色素b6f参与调控蓝细菌 Synechocystis sp. PCC 6803的状态转换

用调制叶绿素荧光研究了对苯醌(1,4-benzoquinone,BQ)和二溴百里香醌(2,5-dibromo-3-methyl-6-isopropyl-1,4-benzoquinone,DBMIB)对蓝细菌Synechocystissp.PCC6803状态转换的作用。BQ和DBMIB是质体醌(PQ)的类似物,两者均可充当PQ的电子受体。其中,DBMIB能够和细胞色素b6f的Qo位点特异结合。在没有作用光的情况下,BQ诱导暗适应的蓝细菌进入状态Ⅰ;相反,DBMIB诱导Syne鄄chocystis6803向状态Ⅱ转换。据此提出,在生理状态下蓝细菌根据PQ库的氧化还原状态调节状态转换;细胞色素b6f参与此调控过程。     

叶绿素缺失和异养生长对蓝藻Synechocystis sp.PCC 6803藻胆蛋白含量的影响

通过遮黑培养缺失ｆｒｘＣ基因的蓝藻Ｓｙｎｅｃｈｏｃｙｓｔｉｓｓｐ．ＰＣＣ６８０３突变工程株,获得了叶绿素缺失的藻细胞,吸收光谱测定及数学计算表明,藻细胞中叶绿素缺失后藻胆蛋白含量增加,藻蓝蛋白和别藻蓝蛋白含量分别为相同条件下野生株对照组的４倍和６倍。野生株遮黑培养时,细胞进行异养生长,藻胆蛋白含量下降,藻蓝蛋白和别藻蓝蛋白含量分别为光照培养条件下自养生长的野生株细胞的３４．５％和２５３％。另外,缺失ａｐｃＥ基因的突变工程株细胞的藻胆蛋白含量也少于对照野生株,表明ａｐｃＥ基因的编码蛋白ＬＣＭ与藻胆蛋白的含量相关。     

硫代硫酸钠和葡萄糖对Synechocystis sp．PCC6803细胞甘油酯及其脂肪酸组成的影响

对生长在添加有不同浓度的葡萄糖、硫代硫酸钠培养基中的蓝细菌Synechocystis sp.PCC 6803中的甘油酯及其脂肪酸组成进行比较。结果表明：硫代硫酸钠能有效地增加膜脂中硫代异鼠李糖二酰基甘油(SQDG)和磷脂酰甘油(PG)的百分含量,培养基中同时添加葡萄糖时能抵消硫代硫酸钠的这一效应。此外,硫代硫酸钠能显著增加单半乳糖甘油二酯(MGDG)、双半乳糖甘油二酯(DGDG)中十六碳酸(C16：0)的百分含量,这一效应也能为葡萄糖消除。硫代硫酸钠不能显著地改变SQDG中C16：0的百分含量,加入葡萄糖时能降低C16：0的百分含量。这些结果说明硫代硫酸钠可能充当一种还原剂使膜脂处于一种低的不饱和状态,同时加入葡萄糖时能降低硫代硫酸钠的还原力。此外,硫代硫酸钠还可作为SQDG合成中的硫供体。     

硫代硫酸钠对蓝细菌Synechocystis sp. PCC 6803生长在含葡萄糖培养基中所产生的一种新糖脂的影响

当蓝细菌Synechocystis sp. PCC 6803在添加葡萄糖的BG-11培养基中培养时,细胞出现了一种新脂.这种脂经浓硫酸/α-萘酚染色反应证实为糖脂,记为糖脂-x.这一糖脂的出现伴随着其他脂、尤其是双半乳糖甘油二酯含量的下降.此外,在添加果糖、麦芽糖、乳糖等其他碳源的培养基中生长的细胞中也检测到这一糖脂.活性氧猝灭剂硫代硫酸钠加入到培养基中能有效地抑制糖脂x的出现.当在BG-11培养基中加入0.3%硫代硫酸钠后,糖脂x仅能在培养基中添加高浓度(100 mmol/L)的葡萄糖且细胞生长处于后指数期时检测到.这些结果表明蓝细菌Synechocystis sp. PCC 6803细胞在含葡萄糖的培养基中生长出现的一种新糖脂可能与活性氧有关.     

Expression of the gene encoding Δ12 acyl-lipid desaturase from Synechocystis sp. PCC 6803 improves potato plant resistance to late blight infection

Transgenic (DesA-LicBM3) potato (Solanum tuberosum L., cv. Desnitsa) plants expressing gene encoding Δ12 acyl-lipid desaturase from Synechosystis sp. PCC 6803 were obtained. A significant increase in the relative content of polyunsaturated (linoleic and linolenic) fatty acids in transformants as compared with original genotype was demonstrated. The improved resistance of transgenic plants to late blight causal agent (Phytophthora infestans) as compared with original cultivar was observed.     

硫代硫酸钠对蓝细菌Synechocystis sp．PCC 6803生长在含葡萄糖培养基中所产生的一种新糖脂的影响

当蓝细菌Synechocystis sp.PCC 6803在添加葡萄糖的BG—11培养基中培养时,细胞出现了一种新脂。这种脂经浓硫酸／α—萘酚染色反应证实为糖脂,记为糖脂—x。这一糖脂的出现伴随着其他脂、尤其是双半乳糖甘油二酯含量的下降。此外,在添加果糖、麦芽糖、乳糖等其他碳源的培养基中生长的细胞中也检测到这一糖脂。活性氧猝灭剂硫代硫酸钠加入到培养基中能有效地抑制糖脂x的出现。当在BG—11培养基中加入0．3％硫代硫酸钠后,糖脂x仅能在培养基中添加高浓度(100mmol／L)的葡萄糖且细胞生长处于后指数期时检测到。这些结果表明蓝细菌Synechocystis sp．PCC 6803细胞在含葡萄糖的培养基中生长出现的一种新糖脂可能与活性氧有关。     

碳氮源对转基因鱼腥藻Anabaena sp.PCC7120培养的影响

对碳源、氮源种类和用量对转rhTNF-α基因鱼腥藻7120（Anabaena sp.PCC7120）培养的影响进行了研究,发现最适碳源为蔗糖,最适氮源为NaNO3,最佳用量分别为9g/L和2．25g/L,此时生物量远高于自养方式,达2．52g/L,比相同条件下在BG－11培养基培养高71．66％,ATNF－α表达量为16％－22％,生物活性为10^5U/mg。     

蓝细菌PCC6803染色体上的毒素蛋白Slr0664与抗毒素蛋白Ssr1114的相互作用

【目的】证明蓝细菌PCC6803染色体上的毒素-抗毒素系统(TA,toxin-antitoxin system)ssr1114/slr0664中毒素蛋白Slr0664与抗毒素蛋白Ssr1114之的相互作用。【方法】构建在大肠杆菌(Escherichia coli)BL21(DE3)中诱导表达H6-Ssr1114或共表达H6-Ssr1114和Slr0664的重组质粒,诱导表达后借助亲和捕捉技术在不同的条件下纯化H6-Ssr1114或共纯化重组蛋白H6-Ssr1114和Slr0664,并通过肽谱分析共纯化的重组蛋白,证明H6-Ssr1114与Slr0664之间存在相互作用。【结果】诱导Slr0664表达对细胞产生毒性作用导致生长抑制或细胞死亡,诱导H6-Ssr1114和Slr0664共表达时细胞能能正常生长,在非变性条件下可纯化共表达的重组蛋白H6-Ssr1114和Slr0664,在变性条件下仅H6-Ssr1114被纯化,肽谱分析结果表明共纯化的的重组蛋白为H6-Ssr1114和Slr0664。【结论】ssr1114/slr0664TA系统中抗毒素蛋白Ssr1114与毒素蛋白Slr0664之间存在相互作用。     

集胞藻PCC 6803类铁氧还蛋白Slr1205的功能研究

类铁氧还蛋白 (ferredoxin-like, Fd-like) 在高等植物中具有调控叶绿体发育等多种重要的生理功能,但在蓝藻中的生物功能尚未被发现。通过比较集胞藻PCC 6083编码Fd-like蛋白基因的敲除突变株Δslr1205与野生型 (WT) 在不同碳源和光周期条件下的生理生化表型,分析Slr1205在集胞藻中的功能。结果显示,在高CO2浓度自养、混合营养和光异养时,Δslr1205的生长速率低于WT,而在空气中自养条件下并无差异。与此相对应,混合营养和光异养时Δslr1205比WT的呼吸速率低,与呼吸作用密切相关的NDH-1L复合体的含量少。Δslr1205在所有测试的条件下有较高的类胡萝卜素以及偏黄的表型。这些数据表明,Fd-like蛋白Slr1205的缺失造成在碳源充足条件下的生长速率下降,这可能是由于呼吸作用下调导致供能不足。研究结果为今后深入研究蓝藻Fd-like蛋白奠定了基础,为开展光合作用和呼吸作用的调节机制研究探索了新方向。     

蓝细菌PCC6803染色体上的一对毒素-抗毒素基因的鉴定

大肠杆菌细胞染色体上毒素－抗毒素系统(TA, toxin-antitoxin system)基因参与环境胁迫诱导的细胞死亡或生长抑制。在蓝细菌PCC6803染色体上开放阅读框ssr1114和slr0664具有与TA系统相同的遗传结构, slr0664编码产物与RelBE毒素－抗毒素系统中的毒素蛋白RelE同源, 但没有发现有与ssr1114编码产物同源的蛋白。为证明slr0664和ssr1114表达产物的毒性和抗毒性作用, 构建了含有乳糖诱导调控的启动子和阿拉伯糖诱导调控的启动子的表达调控系统, 将slr0664基因编码序列置于Plac启动子控制下, ssr1114编码序列置于PBAD启动子控制下, slr0664诱导表达产物对细胞具有毒性作用, ssr1114诱导表达产物具有抗slr0664表达产物的毒性作用。提示slr0664为毒素基因, ssr1114为抗毒素基因, 二者组成一个TA系统, 但其有关特性和功能尚待进一步证明。     

集胞藻PCC 6803中脂肪酸激活酶Slr1609互作蛋白的鉴定

集胞藻中slr1609是编码脂肪酸激活酶的基因,对与其相关的重要功能伴侣蛋白进行研究,可以完善对脂肪酸合成模块的认识,为进一步通过合成生物学技术改造蓝细菌提供理论支持。本研究在集胞藻PCC 6803中建立了蛋白质复合体分析及鉴定技术:利用氯霉素抗性基因筛选,构建带有3×FLAG标签的Slr1609突变株,通过RT-PCR优化重组蛋白表达条件;同时对突变株进行了Western blotting鉴定,以及利用Native-PAGE验证了蛋白质复合体的存在。最后,LC-MS/MS质谱鉴定获得了Slr1609蛋白复合体中的可能伴侣蛋白。     

Proteomic characterization of acid stress response in Synechocystis sp. PCC 6803

A comparative proteomic analysis using 2-DE coupled with MALDI-MS and LC-MS/MS was performed in Synechocystis sp. PCC 6803 to identify protein candidates involved in acid stress response in cyanobacteria. Comparison of soluble proteins from the cytoplasmic fraction of cells grown on media set at pH 7.5 and 5.5 using 2-DE identified four proteins, which showed significant changes in the abundance. Surprisingly, several general stress proteins, either the heat shock family proteins or chaperonins, did not show perceptible fold changes in response to acidity. Compared to the cytoplasmic proteome, the periplasmic proteome showed remarkable changes as a function of external pH. Protein expression profiling at different external pH, i.e., 9.0, 7.5, 6.0 and 5.5, allowed classifying the periplasmic proteins depending on their preferential expression patterns towards acidity or alkalinity. Among the acid- and base-induced proteins, oxalate decarboxylase and carbonic anhydrase were already known for their role in pH homeostasis. Several unknown proteins from the periplasm, that showed significant changes in response to pH, provide ideal targets for further studies in understanding pH stress response in cyanobacteria. This study also identified 14 novel proteins, hitherto unknown from the periplasmic space of Synechocystis.     

A large-scale protein protein interaction analysis in Synechocystis sp. PCC6803.

Protein-protein interactions (PPIs) play crucial roles in protein function for a variety of biological processes. Data from large-scale PPI screening has contributed to understanding the function of a large number of predicted genes from fully sequenced genomes. Here, we report the systematic identification of protein interactions for the unicellular cyanobacterium Synechocystis sp. strain PCC6803. Using a modified high-throughput yeast two-hybrid assay, we screened 1825 genes selected primarily from (i) genes of two-component signal transducers of Synechocystis, (ii) Synechocystis genes whose homologues are conserved in the genome of Arabidopsis thaliana, and (iii) genes of unknown function on the Synechocystis chromosome. A total of 3236 independent two-hybrid interactions involving 1920 proteins (52% of the total protein coding genes) were identified and each interaction was evaluated using an interaction generality (IG) measure, as well as the general features of interacting partners. The interaction data obtained in this study should provide new insights and novel strategies for functional analyses of genes in Synechocystis, and, additionally, genes in other cyanobacteria and plant genes of cyanobacterial origin.     

Proteomic analysis of heterotrophy in Synechocystis sp. PCC 6803

To provide an insight into the heterotrophic metabolism of cyanobacteria, a proteomic approach has been employed with the model organism Synechocystis sp. PCC 6803. The soluble proteins from Synechocystis grown under photoautotrophic and light-activated heterotrophic conditions were separated by 2-DE and identified by MALDI-MS or LC-MS/MS analysis. 2-DE gels made using narrow- and micro-range IPG strips allowed quantitative comparison of more than 900 spots. Out of 67 abundant protein spots identified, 13 spots were increased and 9 decreased under heterotrophy, representing all the major fold changes. Proteomic alterations and activity levels of selected enzymes indicate a shift in the central carbon metabolism in response to trophic change. The significant reduction in light-saturated rate of photosynthesis as well as in the expression levels of rubisco and CO(2)-concentrating mechanism proteins under heterotrophy indicates the down-regulation of the photosynthetic machinery. Alterations in the expression level of proteins involved in carbon utilization pathways refer to enhanced glycolysis, oxidative pentose phosphate pathway as well as tricarboxylic acid cycle under heterotrophy. Proteomic evidences also suggest an enhanced biosynthesis of amino acids such as histidine and serine during heterotrophic growth.     

Proteomic studies of the thylakoid membrane of Synechocystis sp. PCC 6803

Purified thylakoid membranes from the cyanobacterium Synechocystis sp. PCC 6803 were used for the first time in proteomic studies. The membranes were prepared by a combination of sucrose density centrifugation and aqueous polymer two-phase partitioning. In total, 76 different proteins were identified from 2- and 1-D gels by MALDI-TOF MS analysis. Twelve of the identified proteins have a predicted Sec/Tat signal peptide. Fourteen of the proteins were known, or predicted to be, integral membrane proteins. Among the proteins identified were subunits of the well-characterized thylakoid membrane constituents Photosystem I and II, ATP synthase, cytochrome b6f-complex, NADH dehydrogenase, and phycobilisome complex. In addition, novel thylakoid membrane proteins, both integral and peripheral were found, including enzymes involved in protein folding and pigment biosynthesis. The latter were the chlorophyll biosynthesis enzymes, light-dependent protochlorophyllide reductase and geranylgeranyl reductase as well as phytoene desaturase involved in carotenoid biosynthesis and a water-soluble carotenoid-binding protein. Interestingly, in view of the protein sorting mechanism in cyanobacteria, one of the two signal peptidases type I of Synechocystis was found in the thylakoid membrane, whereas the second one has been identified previously in the plasma membrane. Sixteen proteins are hypothetical proteins with unknown function.     

启动子PpetE与Pcpc560对集胞藻PCC 6803生物合成乙醇的影响

为了增加工程集胞藻PCC 6803的乙醇合成产量,通过选用强启动子Pcpc560 驱动并提高外源乙醇合成基因(pdc,yqhD)的表达,从而促进乙醇的生产。具体方法利用同源双交换引入来源于运动型发酵单胞菌的丙酮酸脱羧酶基因(pdc)与来源于大肠杆菌的NADPH依赖型醛还原酶基因(yqhD)并选用不同的启动子来驱动其表达。通过逆转录定量PCR分析,比较在不同启动子驱动的情况下,外源乙醇合成基因(pdc,yqhD)的表达情况并检测相应突变株的乙醇产量。结果显示相较于中等启动子,铜离子诱导启动子PpetE,来源于集胞藻PCC 6803的光强启动子Pcpc560显著促进了外源乙醇合成基因(pdc,yqhD)的表达,并增加了工程菌株乙醇合成的产量。超强启动子Pcpc560搭配pdc,yqhD的组合表达,显著提高了工程菌株的乙醇合成产量。     

集胞藻PCC6803 中relA/spoT 同源基因syn-rsh (slr1325)的鉴定

[目的]四磷酸或五磷酸鸟苷(Guanosine 3′,5′-bispyrophosphate,(p)ppGpp)是细菌在遭遇环境胁迫时细胞产生应激反应的信号分子,(p)ppGpp由其合成酶RelA或具有合成酶或水解酶双重催化功能的RelA/SpoT合成.本文证明了集胞藻PCC6803(Synechocystis sp.)中唯一编码RelA/SpoT同源蛋白(命名为Syn-RSH)的基因slr1325(syn-rsh)的功能.[方法]通过互补试验证明syn-rsh表达产物的生物学功能;以纤维素薄层层析检测不同条件下Escherichia coli(p)ppGpp合成缺陷突变株及集胞藻PCC6803细胞中的(p)ppGpp.[结果]诱导Syn-RSH表达可使(p)ppGpp合成酶和水解酶基因缺失的E.coli突变株回复野生型表型,并在细胞中积累一定水平的ppGpp;在实验室培养条件下,集胞藻PCC6803细胞中可检测到低水平的ppGpp,氨基酸饥饿可诱导ppGpp水平升高并维持在相应水平.[结论]Syn-RSH具有(p)ppGpp合成酶和水解酶的双重功能,(p)ppGpp是集胞藻PCC6803在实验室生长条件下细胞生长所必需的.