嗜热藻BP-1中几个蓝细菌光敏色素结构域体内重组及光化学性质研究北大核心CSCD

通过蛋白质序列同源性比对分析,在嗜热藻(Thermosynechococcus elongatus BP-1)里面找到了与已知的Pb/Pg型蓝细菌光敏色素TePixJ和TeTlr0924同源的3个基因tlr0911、tlr1215和tlr1999。通过分子克隆技术把它们的GAF结构域分别构建在pET30a(+)表达载体上,与可生成藻蓝胆素(PCB)的质粒pACYCDuet-ho1-pcyA在大肠杆菌BL21(DE3)体内重组,生成重组蛋白,利用亲和层析柱分离纯化,纯化后的蛋白质经过锌荧光和蛋白质酸性尿素变性以及荧光光谱和吸收光谱等实验分析鉴定,结果表明,Tlr0911-GAF存在蓝光吸收态Pb406 nm和绿光吸收态Pg527 nm之间的可逆光转换,它可共价结合两种藻胆色素,即藻紫胆素(PVB)和藻蓝胆素(PCB),Tlr1999-GAF则存在蓝光吸收态Pb417 nm和青光吸收态Pt496 nm之间的可逆光转换,它同样共价结合PVB和PCB,而Tlr1215-GAF1和Tlr1215-GAF2不能自发结合藻胆色素,不具有光活性。     

蓝细菌光敏色素Alr1966GAF2及其突变体的表达与光化学性质研究

采用PCR技术从鱼腥藻（Anabaena sp.PCC7120）中扩增蓝细菌光敏色素基因片段alr1966gaf2,将alr1966gaf2插入到pET-30a（+）载体中,构建表达质粒pET-alr1966gaf2。最后将Alr1966GAF2与HO1、PcyA在E.coli BL21（DE3）中共表达获得色素蛋白Alr1966GAF2,并对该蛋白的光化学性质进行分析。结果显示,色素蛋白Alr1966GAF2结合色素为藻蓝胆素（phycoerythrobilin,PCB）或藻紫胆素（phycoviolobilin,PVB）,在3种不同吸收态15Z-P_{428 nm}、中间态和15E-P_{514 nm}之间具有顺序可逆光效应。通过定点突变技术将DXCF基序中的保守性Cys突变为Ala,获得了突变体Alr1966GAF2（C72A）。将Alr1966GAF2（C72A）与HO1、PcyA共表达,获得色素蛋白Alr1966GAF2（C72A）。研究结果表明Alr1966GAF2（C72A）结合色素为PCB,Alr1966GAF2（C72A）-PCB具有较强的荧光活性,其荧光量子的产率高达0.11。Alr1966GAF2（C72A）不仅能够共价结合PCB,还可以结合胆绿素（Biliverdin,BV）,均具有较强的红色荧光活性。     

蓝细菌光敏色素的分子结构、生物合成和可逆光致变色效应

蓝细菌光敏色素(CBCRs)是蓝细菌中感受光的重要光受体,能够响应从紫外光到红外光范围内的光信号,进而影响蓝细菌的光化学行为。蓝细菌光敏色素通过N-末端GAF(cGMP phosphodiesterase,adenylyl cyclase and FhlA domain)结构域中保守性半胱氨酸共价结合藻胆色素,形成具有感光生理功能的色素蛋白质。本文重点在分子水平上综述了蓝细菌光敏色素的分子结构、生物合成和可逆光致变色效应机理,并基于最新的研究进展,就蓝细菌光敏色素今后的研究方向进行了展望。     

鱼腥藻PCC7120细菌光敏色素缺失突变体的自催化重组研究

采用聚合酶链式反应（PCR）从鱼腥藻PCC7120 DNA中扩增出细菌光敏色素缺失突变体基因aphA（26-320）、aphA（27-320）、aphA（28-320）、aphA（29-320）和aphA（32-320）。利用表达载体pET30a进行高效表达,获得的AphA缺失突变体脱辅基蛋白在一定的反应体系下与藻蓝胆素进行了体外重组的研究。研究表明：AphA（26-320）体外重组获得的色素蛋白具有与植物光敏色素相似的可逆光致变色效应,同时酸性尿素变性实验和Zn^2＋荧光电泳实验显示藻蓝胆素和以上蛋白质发生共价连接。AphA（26-320）与藻蓝胆素重组产物的Pr／Pfr吸收峰处于660／610nm。其他4个缺失突变体,AphA（27-320）、AphA（28-320）、AphA（29-320）、AphA（32-320）和藻蓝胆素的重组产物中则没有发现可逆光致变色信号,表明这些缺失突变体不能和藻蓝胆素发生自催化重组。维系细菌光敏色素AphA与色素自催化连接的裂合酶结构域位于AphA（26-320）包含的肽链之中。     

藻蓝蛋白裂合酶CpeS色氨酸定点诱变及体内重组功能研究

为了研究藻蓝蛋白β亚基Cys-84裂合酶CpeS结构与功能的关系以及色氨酸残基对于该酶功能的影响,构建了藻蓝蛋白β亚基Cys-84裂合酶CpeS的两个色氨酸突变体,分别为CpeS（W14I）和CpeS（W75S）。通过体内重组检测酶活性的变化,研究色氨酸残基的突变对裂合酶催化活性的影响。重组结果显示：突变体CpeS（W14I）的催化活性几乎完全丧失,为野生型的8％;突变体CpeS（W75S）的催化活性为野生型的76％。由此推测,第14位色氨酸可能是CpeS酶活性的必需氨基酸,其所处的位置可能是裂合酶CpeS的活性位点。     

藻胆体核亚基ApcD定点突变及体内重组功能研究

在对Anabaena sp.PCC7120藻胆体核亚基ApcD结合色素PCB的体内重组中,发现色素蛋白在提纯前后最大吸收峰和荧光峰发生了红移,从提纯前的605nm及633nm变为提纯后的650nm及665nm.为了研究该现象的原因,构建了ApcD的8个突变体,重组结果显示:突变体ApcD(Y88I)色素蛋白在提纯后的吸收光谱和荧光光谱较提纯前均多出一个峰,分别为668nm,690nm;ApcD(W59Q)、ApcD(Y73A)、ApcD(W87E)色素蛋白在提纯前后的吸收光谱和荧光光谱一致;ApcD(M126S)、ApcD(Y116S)、ApcD(M160T)色素蛋白在提纯前后的吸收光谱一致,而提纯后的荧光峰位置较提纯前分别红移了5nm、7nm和10nm;ApcD(M115I)色素蛋白在提纯前后的吸收光谱和荧光光谱均发生了红移,从提纯前的605nm和633nm变为提纯后的638nm和655nm.这些色素蛋白在酸性尿素溶液变性条件下的最大吸收峰始终在662nm,表明辅基色素仍然是藻蓝胆素;在对PCB-ApcD、PCB-ApcD(Y116S)及PCB-ApcD(M160T)的圆二色谱分析发现,该两个氨基酸的突变均...     

光系统Ⅱ反应中心CP47/D1/D2/Cyt b-559复合物中色素分子空间取向的线二色光谱研究(英文)

线二色光谱(LD)是研究色素分子在光合膜上空间取向和排布的重要手段。采用低温(1 0 0K)吸收光谱和线二色光谱技术研究光系统Ⅱ核心复合物CP47/D1/D2/Cytb_5 5 9中色素分子的空间取向。结果表明,在光系统Ⅱ核心复合物CP47/D1/D2/Cytb_5 5 9中 6 80nm处有吸收的叶绿素分子Qy 跃迁与光合膜平面平行。β_胡萝卜素分子有两种不同的空间取向,其中在 470和 5 0 5nm处有吸收的 β_胡萝卜素分子(Ⅰ)与光合膜平面近似平行,而在 46 0和 490nm处有吸收的 β_胡萝卜素分子(Ⅱ)与光合膜垂直。光破坏实验显示垂直取向的 β_胡萝卜素分子对强光敏感。6 80nm处吸收的叶绿素分子成分复杂,可能包含有P6 80和核心天线CP47蛋白上的色素分子。     

光系统Ⅱ反应中心CP47/D1/D2/Cyt b-559复合物中色素分子空间取向的线二色光谱研究

线二色光谱(LD)是研究色素分子在光合膜上空间取向和排布的重要手段.采用低温(100K)吸收光谱和线二色光谱技术研究光系统Ⅱ核心复合物CP47/D1/D2/Cyt b-559中色素分子的空间取向.结果表明,在光系统Ⅱ核心复合物CP47/D1/D2/Cyt b-559中680 nm处有吸收的叶绿素分子Qy跃迁与光合膜平面平行.β-胡萝卜素分子有两种不同的空间取向,其中在470和505nm处有吸收的β-胡萝卜素分子(Ⅰ)与光合膜平面近似平行,而在460和490nm处有吸收的β-胡萝卜素分子(Ⅱ)与光合膜垂直.光破坏实验显示垂直取向的β-胡萝卜素分子对强光敏感.680nm处吸收的叶绿素分子成分复杂,可能包含有P680和核心天线CP47蛋白上的色素分子.     

Cyanobacteriochrome TePixJ of Thermosynechococcus elongatus harbors phycoviolobilin as a chromophore

Cyanobacteria have several putative photoreceptors (designated cyanobacteriochromes) that are related to but distinct from the established phytochromes. The GAF domain of the phototaxis regulator, PixJ, from a thermophilic cyanobacterium Thermosynechococcus elongatus BP-1 (TePixJ_GAF) is a cyanobacteriochrome which exhibits reversible photoconversion between a blue light-absorbing form (max = 433 nm) and a green light-absorbing form (max = 531 nm). To study the chromophore, we prepared TePixJ_GAF chromoprotein from heterologously expressed Synechocystis and performed spectral analysis after denaturation by comparing it with the cyanobacterial phytochrome Cph1 which harbors phycocyanobilin (PCB) as a chromophore. The results indicated that the chromophore of TePixJ is not PCB, but its isomer, phycoviolobilin (PVB). It is suggested that the GAF domain of TePixJ has auto-lyase and auto-isomerase activities.     

Characterization of cyanobacteriochrome TePixJ from a thermophilic cyanobacterium Thermosynechococcus elongatus strain BP-1

A putative photoreceptor gene, TepixJ, of a thermophilic cyanobacterium is homologous to SypixJ1 that mediates positive phototaxis in the unicellular motile cyanobacterium Synechocystis sp. PCC 6803. The putative chromophore-binding GAF domain of TePixJ protein was overexpressed as a fusion with a polyhistidine tag (His-TePixJ_GAF) in Synechocystis cells and isolated to homogeneity. The photoreversible conversion of His-TePixJ_GAF showed peaks at 531, 341 and 266 nm for the green light-absorbing form (Pg form), and peaks at 433 and 287 nm for the blue light-absorbing form (Pb form). At 77K, the Pg form fluoresced at 580 nm, while the Pb form did not emit any fluorescence. Mass spectrometry of the tryptic chromopeptide demonstrated that a phycocyanobilin isomer binds to the conserved cysteine at ring A via a thioether bond. It is established that TePixJ and SyPixJ1 are novel photoreceptors in cyanobacteria ('cyanobacteriochromes') that are similar, but distinct from the phytochromes and bacteriophytochromes.     

Cloning, solubilization, and characterization of squalene synthase from Thermosynechococcus elongatus BP-1

Squalene synthase (SQS) is a bifunctional enzyme that catalyzes the condensation of two molecules of farnesyl diphosphate (FPP) to give presqualene diphosphate (PSPP) and the subsequent rearrangement of PSPP to squalene. These reactions constitute the first pathway-specific steps in hopane biosynthesis in Bacteria and sterol biosynthesis in Eukarya. The genes encoding SQS were isolated from the hopane-producing bacteria Thermosynechococcus elongatus BP-1, Bradyrhizobium japonicum, and Zymomonas mobilis and cloned into an Escherichia coli expression system. The expressed proteins with a His(6) tag were found exclusively in inclusion bodies when no additives were used in the buffer. After extensive optimization, soluble recombinant T. elongatus BP-1 SQS was obtained when cells were disrupted and purified in buffers containing glycerol. The recombinant B. japonicum and Z. mobilis SQSs could not be solubilized under any of the expression and purification conditions used. Purified T. elongatus His(6)-SQS gave a single band at 42 kDa by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and molecular ion at m/z 41886 by electrospray mass spectrometry. Incubation with FPP and NADPH gave squalene as the sole product. Incubation of the enzyme with [(14)C]FPP in the absence of NADPH gave PSPP. The enzyme requires Mg(2+) for activity, has an optimum pH of 7.6, and is strongly stimulated by detergent. Under optimal conditions, the K(m) of FPP is 0.97 +/- 0.10 microM and the k(cat) is 1.74 +/- 0.04 s(-1). Zaragozic acid A, a potent inhibitor of mammalian, fungal, and Saccharomyces cerevisiae SQSs, also inhibited recombinant T. elongatus BP-1 SQS, with a 50% inhibitory concentration of 95.5 +/- 13.6 nM.     

Remarkable stability of the proton translocating F1FO-ATP synthase from the thermophilic cyanobacterium Thermosynechococcus elongatus BP-1

For functional characterization, we isolated the F1FO-ATP synthase of the thermophilic cyanobacterium Thermosynechococcus elongatus. Because of the high content of phycobilisomes, a combination of dye-ligand chromatography and anion exchange chromatography was necessary to yield highly pure ATP synthase. All nine single F1FO subunits were identified by mass spectrometry. Western blotting revealed the SDS stable oligomer of subunits c in T. elongatus. In contrast to the mass archived in the database (10,141 Da), MALDI-TOF-MS revealed a mass of the subunit c monomer of only 8238 Da. A notable feature of the ATP synthase was its ability to synthesize ATP in a wide temperature range and its stability against chaotropic reagents. After reconstitution of F1FO into liposomes, ATP synthesis energized by an applied electrochemical proton gradient demonstrated functional integrity. The highest ATP synthesis rate was determined at the natural growth temperature of 55 degrees C, but even at 95 degrees C ATP production occurred. In contrast to other prokaryotic and eukaryotic ATP synthases which can be disassembled with Coomassie dye into the membrane integral and the hydrophilic part, the F1FO-ATP synthase possessed a particular stability. Also with the chaotropic reagents sodium bromide and guanidine thiocyanate, significantly harsher conditions were required for disassembly of the thermophilic ATP synthase.     

Primary intermediate in the photocycle of a blue-light sensory BLUF FAD-protein, Tll0078, of Thermosynechococcus elongatus BP-1

Proteins with a BLUF (sensor of blue light using flavin adenine dinucleotide) domain represent a newly recognized class of photoreceptors that is widely distributed in the genomes of photosynthetic bacteria, cyanobacteria, and Euglena. Recently, Okajima et al. [Okajima, K., Yoshihara, S., Geng, X., Katayama, M. and Ikeuchi, M. (2003) Plant Cell Physiol. 44 (Suppl), 162] purified BLUF protein Tll0078 encoded in the genome of thermophilic cyanobacterium Thermosynechococcus elongatus BP-1 by expressing the protein in Escherichia coli. We investigated the photocycle of Tll0078 by measuring the picosecond fluorescence kinetics, transient absorption changes, and the UV-visible absorption spectra at 10 to 330 K. The absorption spectrum of the FAD moiety of Tll0078 showed a 10-nm red shift upon illumination at 278-330 K. The quantum efficiency of the formation of the red-shifted form was 29%. Illumination at 10 K, on the other hand, caused only a 5-nm red shift in about one-half of the protein population. The 5-nm-shifted form was stable at 10 K. The 5-nm red-shifted form was converted into the 10-nm red-shifted form at 50-240 K upon warming in the dark. At room temperature, the 10-nm red-shifted final product appeared within 10 ns after laser flash excitation. The lifetime of the fluorescence of FAD was found to be 120 ps at room temperature. These results reveal a fast and efficient photoconversion process from the singlet-excited state to the final product at room temperature. A photocycle of BLUF protein is proposed that includes the 5-nm red-shifted intermediate form as the precursor for the 10-nm red-shifted final product. The temperature dependence of each step of the photocycle is also discussed.     

Structural response of Photosystem 2 to iron deficiency: characterization of a new photosystem 2-IdiA complex from the cyanobacterium Thermosynechococcus elongatus BP-1

Iron deficiency triggers various processes in cyanobacterial cells of which the synthesis of an additional antenna system (IsiA) around photosystem (PS) 1 is well documented [T.S. Bibby, J. Nield, J. Barber, Iron deficiency induces the formation of an antenna ring around trimeric photosystem I in cyanobacteria, Nature 412 (2001) 743-745, E.J. Boekema, A. Hifney, A.E. Yakushevska, M. Piotrowski, W. Keegstra, S. Berry, K.P. Michel, E.K. Pistorius, J. Kruip, A giant chlorophyll-protein complex induced by iron deficiency in cyanobacteria, Nature 412 (2001) 745-748]. Here we show that PS2 also undergoes prominent structural changes upon iron deficiency: Prerequisite is the isolation and purification of a PS2-IdiA complex which is exclusively synthesized under these conditions. Immunoblotting in combination with size exclusion chromatography shows that IdiA is only bound to dimeric PS2. Using single particle analysis of negatively stained specimens, IdiA can be localized in averaged electron micrographs on top of the CP43 subunit facing the cytoplasmic side in a model derived from the known 3D structure of PS2 [B. Loll, J. Kern, W. Saenger, A. Zouni, J. Biesiadka, Towards complete cofactor arrangement in the 3.0 A resolution structure of photosystem II, Nature 438 (2005) 1040-4]. The presence of IdiA as integral part of PS2 is the first example of a new PS2 protein being expressed under stress conditions, which is missing in highly purified PS2 complexes isolated from iron-sufficient cells.     

Functional analysis of psbV and a novel c-type cytochrome gene psbV2 of the thermophilic cyanobacterium Thermosynechococcus elongatus strain BP-1.

Cytochrome c-550 is an extrinsic protein associated with photosystem II (PSII) in cyanobacteria and lower eukaryotic algae and plays an important role in the water-splitting reaction. The gene (psbV) for cytochrome c-550 was cloned from the thermophilic cyanobacteria Thermosynechococcus (formerly Synechococcus) elongatus and T. (formerly Synechococcus) vulcanus. In both genomes, located downstream of psbV were a novel gene (designated psbV2) for a c-type cytochrome and petJ for cytochrome c-553. The deduced product of psbV2 showed composite similarities to psbV and petJ. Phenotype of psbV-disruptant in Thermosynechococcus was practically the same as that reported in Synechocystis sp. PCC 6803. Either psbV or psbV2 gene of T. elongatus was expressed in the psbV-disruptant of Synechocystis sp. PCC 6803, which resulted in recovery of the photoautotrophic growth. However, the enhanced requirement of Ca(2+) or Cl- ions in the psbV-disruptant of Synechocystis was suppressed by expression of psbV but not by expression of psbV2. Thus, it is concluded that psbV2 can partly replace the role of psbV in PSII. The close tandem arrangement of psbV/psbV2/petJ implies that psbV2 was created by gene duplication and intergenic recombination during evolution.