嗜热蓝藻层理鞭枝藻（Mastigocladus laminosus）藻胆体在解离过程中荧光发射光谱和光能传递的研究

研究了层理鞭枝藻胆体在不同浓度磷酸冲溶液中解离过程中荧光发射光谱的变化和光能传递,完整藻胆体的７７Ｋ荧光光谱中只有一个峰,位于６８５ｎｍ,它是末端发射体（核心－膜连接多肽和别蓝蛋白－Ｂ）的荧光峰,部分解离藻胆体的荧光光谱的主峰位移至６５２ｎｍ,次峰位于６８５ｎｍ;６６０ｎｍ为一弱荧光发射肩,它们依次为Ｃ－藻蓝蛋白,末端发射体和别藻蓝蛋白的荧光。严重解离藻胆体的荧光主峰移至６４４ｎｍ;次峰由６８５ｎ     

螺旋藻（Spirulina platensis）藻胆体在解离过程中荧光发射光谱和光能传递的研究

对螺旋藻（Ｓｐｉｒｕｌｉｎａｐｌａｔｅｎｓｉｓ）藻胆体在室温和７７Ｋ处于不同浓度磷缓冲溶液和不同解离时间的荧光发射光谱进行了研究。藻胆体在０．９ｍｏｌ／Ｌ磷酸缓冲溶液中,由于没有发生解离,光能传递效率高,在７７Ｋ荧光发射光谱中只有一个峰,位于６８７ｎｍ,属于别藻蓝蛋白－Ｂ。当藻胆体悬浮在０．３ｍｏｌ／Ｌ磷酸缓冲溶液中１分钟,７７Ｋ荧光光谱的主峰出现在６８４ｎｍ．又出现６５５ｎｍ和６６６ｎｍ荧光峰,它们依次属子Ｃ－藻蓝蛋白和别藻蓝蛋白。在２小时;６５５ｎｍ荧先峰成为主峰,６８４ｎｍ荧光峰为次峰,６６６ｎｍ荧光肩消失。这表明Ｃ－藻蓝蛋白所捕获的先能已不能传递给别藻蓝蛋白,但能传给别藻蓝蛋白－Ｂ。我们提出在螺旋藻藻胆体中存在两类Ｃ－藻蓝蛋白,一是与别藻蓝蛋白相连接,另一是与别藻蓝蛋白－Ｂ相连接。     

螺旋藻（Spirulina platensis）藻胆体在解离过程中荧光发射光谱和光能传递的研究

对螺旋藻（Ｓｐｉｒｕｌｉｎａｐｌａｔｅｎｓｉｓ）藻胆体在室温和７７Ｋ处于不同浓度磷缓冲溶液和不同解离时间的荧光发射光谱进行了研究。藻胆体在０．９ｍｏｌ／Ｌ磷酸缓冲溶液中,由于没有发生解离,光能传递效率高,在７７Ｋ荧光发射光谱中只有一个峰,位于６８７ｎｍ,属于别藻蓝蛋白－Ｂ。当藻胆体悬浮在０．３ｍｏｌ／Ｌ磷酸缓冲溶液中１分钟,７７Ｋ荧光光谱的主峰出现在６８４ｎｍ．又出现６５５ｎｍ和６６６ｎｍ荧光峰,它们依次属子Ｃ－藻蓝蛋白和别藻蓝蛋白。在２小时;６５５ｎｍ荧先峰成为主峰,６８４ｎｍ荧光峰为次峰,６６６ｎｍ荧光肩消失。这表明Ｃ－藻蓝蛋白所捕获的先能已不能传递给别藻蓝蛋白,但能传给别藻蓝蛋白－Ｂ。我们提出在螺旋藻藻胆体中存在两类Ｃ－藻蓝蛋白,一是与别藻蓝蛋白相连接,另一是与别藻蓝蛋白－Ｂ相连接。     

嗜热蓝藻优雅粘囊藻藻胆体的特性和别藻蓝蛋白的亚基组成

研究了优雅粘囊藻藻胆体的特性。从聚丙烯酰胺凝胶电泳、吸收光谱和二阶导数图谱可证明,它的ＰＢＳ含有一种红色藻胆蛋,两种Ｃ－藻蓝蛋白和三种别藻蓝蛋白。但是,用ＰＡＧＥ和羟基磷灰石柱层析分离和纯化所得藻胆蛋白,一般仅得到一种Ｃ－ＰＣ和一种亚基组成特殊的别藻蓝蛋白ＡＰＣ。这种ＡＰＣ吸收光谱和荧光发射相同于已报告的ＡＰＣ６６０ｎｍ。但是它的亚基组成是（αα＇ββ＇）２而不是（α＇α２β２β＇）Ｌｃ＾１０或α     

螺旋藻(Spirulina Platensis)藻胆体的光谱特性和能量传递的研究

研究了螺旋藻藻胆体的吸收光谱,室温和液氮温度荧光发射光谱和激发光谱.完整藻胆体的室温荧光峰位于678nm,不完整藻胆体位于672nm.在完整藻胆体的液氮温度荧光光谱中只有一个发射峰,不完整藻胆作有两个峰.研究结果表明C-藻蓝蛋白与别藻蓝蛋白之间的连接和别藻蓝蛋白与别藻蓝蛋白-B之间的连接具有不同的稳定性;前者稳定性较差,易解离.对藻胆体内藻胆蛋白之间的光能传递进行了讨论.     

嗜热蓝藻优雅粘囊藻藻胆体的特性和别藻蓝蛋白的亚基组成

研究了优雅粘囊藻藻胆体（ＰＢＳ）的特性。从聚丙烯酰胺凝胶电泳（ＰＡＧＥ）、吸收光谱和二阶导数图谱可证明,它的ＰＢＳ含有一种红色藻胆蛋白,两种Ｃ－藻蓝蛋白和三种别藻蓝蛋白。但是,用ＰＡＧＥ和羟基磷灰石柱层析分离和纯化所得藻胆蛋白,一般仅得到一种Ｃ－ＰＣ和一种亚基组成特殊的别藻蓝蛋白ＡＰＣ。这种ＡＰＣ吸收光谱和荧光发射相同于已报告的ＡＦＣ６６０ｎｍ。但是它的亚基组成是（αα′ββ′）２而不是（α′α２β２β′）Ｌｃ１０或（αβ）３。     

蓝藻藻胆体与类囊体膜之间光能传递的研究

从嗜热蓝藻优雅粘囊藻（Ｍｙｘｏｓａｒｃｉｎａ ｃｏｎｃｉｎｎａ Ｐｒｉｎｔｚ．）中分离到具有放氧活性的藻胆体－类囊体膜复合物。它的吸收峰位于６８０、６２８、４９０、４３８和４２０ ｎｍ ,在低离子强度（０．１～０．４ ｍ ｏｌ／Ｌ）磷酸缓冲液中的６６４ ｎｍ 荧光发射峰随离子强度的降低而升高,７１８ ｎｍ 荧光发射峰与此相反（７７ 。Ｋ,Ｅｘ＝ ５８０ ｎｍ ）。当把游离的藻胆体和已解离去藻胆体的类囊体膜在蔗糖磷酸缓冲液中重组时,随时间延长（０～６０ ｍ ｉｎ）,７１８ ｎｍ 荧光发射峰逐渐升高,６８５ ｎｍ 荧光发射峰逐渐下降（７７ 。Ｋ,Ｅｘ ＝ ５８０ ｎｍ ）,表明藻胆体与类囊体之间的解离和结合对光能传递的影响     

发菜藻胆体的分离和光谱特性的研究

完整藻胆体和不完整藻胆体的吸收峰都在618nm。完整藻胆体的室温荧光峰位于670nm以上,而不完整藻胆体则在670nm以下。完整藻胆体的77K荧光发射光谱中只有648nm一个荧光发射带;而在不完整藻胆体,则有2个或3个发射带,它们位于684nm,666nm和648nm,依次属于别藻蓝蛋白-B,别藻蓝蛋白和C-藻蓝蛋白的荧光。     

发菜藻胆体分离和光谱特性的研究

完整藻胆体和不完整藻胆体的吸收峰都在618nm。完整藻胆体的室温荧光峰位于670nm 以上,而不完整藻胆体则在670nm以下。完整藻胆体的77K荧光发射光谱中只有648nm一个荧光发射带;而在不完整藻胆体,则有2个或3个发射带,它们位于684nm,666nm和648nm, 依次属于别藻蓝蛋白 — B,别藻蓝蛋白和C — 藻蓝蛋白的荧光。     

蓝藻(Cyanobacteria)藻胆体内核结构与功能的研究I.变藻蓝蛋白六聚体(αβ)5APβ16.3LCM42分离及其表征

利用藻胆体温和解离的方法和超速离心分离技术首次得到了变藻蓝蛋白六聚体,并通过光谱技术,凝胶柱过滤柱色谱方法,和ＳＤＳ－ＰＡＧＥ电泳方法以及蔗糖密度超速离心方法对其进行表征。结果表明：该变落蓝蛋白六聚体的最大吸收峰（λ＾Ａｍａｘ＝６５２ｎｍ）,荧光发射峰位于６６６ｎｍ,并且在６８０ｎｍ处有一明显肩峰;其分子量大约为２４０ＫＤ左右;其分子组成为（αβ）５＾ＡＰβ＾１６．３ＬＣＭ＾４２;离心沉降系数为１     

Effects of proteinase K on the energy transfer between phycobiliproteins in phycobilisomes

Spectral changes in fluorescence of phycobilisomes (PBS) of A. variabilis treated with proteinase K were studied at room and liquid nitrogen temperature. In control PBS, the relative yield of 77 K fluorescence of F686 was very high, and those of F655 and F666 were low. In PBS treated with proteinase K for less than 1 h, F686 decreased, and F655 and F666 increased. In PBS treated with proteinase K for 2 h, F655 was the main peak of fluorescence emission, F686 was the second peak, the fluorescence emission peak of F666 disappeared. In PBS treated with proteinase K for more than 8 h, F655 showed only one fluorescence emission peak.We suggested that phycobiliporteins in the PBS of A. variabilis constitute an energy transfer chain, shown as follows:{fx91-1}The linkages between APC and APC-B, C-PC and APC, and C-PC and APC-B had different sensitivity towards proteinase K.     

三种藻胆蛋白在复合累积LB膜中的能量传递

制备了R-藻红蛋白(R-PE)、C-藻蓝蛋白(C-PC)及变藻蓝蛋白(APC)的单组分累积LB膜及三组分复合累积LB膜. 吸收及荧光光谱测定表明三种蛋白的LB膜的光谱重叠性质与他们在水溶液中的性质相同. 结构测定表明, 三种蛋白在其LB膜中排列有序, 且由它们组装的复合累积LB膜结构类似于藻类植物中的藻胆体结构. 通过稳态荧光光谱及其光谱解叠, 观察到了三种蛋白在复合累积LB膜中的激发能量传递现象. 根据给体荧光峰的猝灭, 计算出在复合累积LB膜中从给体R-PE经C-PC到受体APC的能量传递效率为51%.     

Comparison of main emissions at--196?C from phycobilisomes of two blue-green algae Anabaena cylindrica and Anacystis nidulans

Main emissions at—196?C from phycobilisomes of two blue-greenalgae Anabaena cylindrica and Anacystis nidulans were studiedwith special reference to allophycocyanin (APC) B content. Supplementaryexperiments were done with Anabaena variabilis (M-2 and M-3).The main emission from phycobilisome of Anacystis nidulans richin APC B was located at 681 nm. The location was identical tothat of the main emission from APC B but at a shorter wavelengththan that of in vivo emission (685 nm). Results indicate thatAPC B acts as the energy output of phycobilisomes, but thatthe in vivo 685 nm emission is not attributed to APC B. The main emission of the phycobilisome of Anabaena cylindricawas always located at 685 nm irrespective of the preparationmethod; 0.75 M phosphate buffer [Plant Physiol., 63: 615–620(1979)] or 30% polyethylene glycol [Special Issue of Plant &Cell Physiol., No. 3, p. 23–31 (1977)]. This alga alsocontained a special form of APC, but its content was very low.The location of its emission band (681 nm) was identical tothat of APC B, but shorter than that of the main band of phycobilisomes(685 nm). The 685 nm emitter in phycobilisomes showed a charactersimilar to chlorophyll a but not phycobiliproteins in treatmentsfor aqueous extraction or methanol extraction. Results indicatethat the pigment is probably chlorophyll a as we assumed previously.The 685 nm emission from phycobilisomes of Anabaena variabilis(M-2 and M-3) showed the same character. Results were interpreted as indicating that (i) the contentof the special form of APC varies with the species or strainof blue-green algae and (ii) the energy at the phycobilin levelis transferred directly from APC to pigment system II chlorophylla when the amount of the special form of APC is low. (Received October 24, 1979; )     

Single-molecule spectroscopy selectively probes donor and acceptor chromophores in the phycobiliprotein allophycocyanin

We report on single-molecule fluorescence measurements performed on the phycobiliprotein allophycocyanin (APC). Our data support the presence of a unidirectional F?rster-type energy transfer process involving spectrally different chromophores, alpha84 (donor) and beta84 (acceptor), as well as of energy hopping amongst beta84 chromophores. Single-molecule fluorescence spectra recorded from individual immobilized APC proteins indicate the presence of a red-emitting chromophore with emission peaking at 660 nm, which we connect with beta84, and a species with the emission peak blue shifted at 630 nm, which we attribute to alpha84. Polarization data from single APC trimers point to the presence of three consecutive red emitters, suggesting energy hopping amongst beta84 chromophores. Based on the single-molecule fluorescence spectra and assuming that emission at the ensemble level in solution comes mainly from the acceptor chromophore, we were able to resolve the individual absorption and emission spectra of the alpha84 and beta84 chromophores in APC.     

Photosynthetic vesicles with bound phycobilisomes from Anabaena variabilis.

Photosynthetically active vesicles with attached phycobilisomes from Anabaena variabilis, were isolated and shown to transfer excitation energy from phycobiliproteins to F696 chlorophyll (Photosystem II). The best results were obtained when cells were disrupted in a sucrose/phosphate/citrate mixture (0.3 : 0.5 : 0.3 M, respectively) containing 1.5% serum albumin. The vesicles showed a phycocyanin/chlorophyll ratio essentially identical to that of whole cells, and oxygen evolution rates of 250 mumol O2/h per mg chlorophyll (with 4 mM ferricyanide added as oxidant), whereas whole cells had rates of up to 450. Excitation of the vesicles by 600 nm light produced fluorescence peaks (-196 degrees C) at 644, 662, 685, 695, and 730 nm. On aging of the vesicles, or upon dilution, the fluorescence yield of the 695 nm emission peak gradually decreased with an accompanying increase and final predominant peak at 685 nm. This shift was accompanied by a decrease in the quantum efficiency of Photosystem II activity from an initial 0.05 to as low as 0.01 mol O2/einstein (605 nm), with a lesser change in the Vmax values. The decrease in the quantum efficiency is mainly attributed to excitation uncoupling between phycobilisomes and Photosystem II. It is concluded that the F685 nm emission peak, often exclusively attributed to Photosystem II chlorophyll, arises from more than one component with phycobilisome emission being a major contributor. Vesicles from which phycobilisomes had been removed, as verified by electron microscopy and spectroscopy, had an almost negligible emission at 685 nm.     

PHYCOBILIPROTEIN COMPOSITION AND CHLOROPLAST STRUCTURE IN THE FRESHWATER RED ALGA COMPSOPOGON COERULEUS (RHODOPHYTA)1

Serial sections of uncorticated axial cells of Compsopogon coeruleus revealed a single interconnected parietal chloroplast. Phycobilisomes in such chloroplasts were hemidiscoidal in shape with a broad-face diameter of ca. 25–30 nm. The molar ratio of phycobiliproteins in whole cell extracts was IPE:3PC:1APC, similar to isolated phycobilisomes. Two spectrally distinct C-phycocyanin forms (A618 nm, F648 nm and A630 nm, F652 nm) were resolved in dissociated phycobilisomes along with B-phycoerythrin and allophycocyanin.