Kinetic resolution of different recovery phases of photoinhibited photosystem II in cold-acclimated and non-acclimated spinach leaves

Leaf discs from spinach were exposed to a photon flux density of 1250 μmol m⁻²s⁻¹ at 5°C for 2 or 3 h in ambient air. Photoinhibition of photosystem II (PS II) was measured by means of chlorophyll fluorescence. Recovery of photosystem II was followed at 6°C and 20°C in low light or darkness for periods up to 12 h.
The experimental setup allowed kinetic resolution of different phases of recovery. The experiments revealed a temperature dependent dark recovery phase and two distinct light- and temperature dependent phases: (1) A relatively fast, light dependent recovery phase occurred in parallel with partial recovery of basic fluorescence at 6°C and 20°C. A population of PS II centers with very slow fluorescence induction kinetics, which had accumulated during photoinhibition treatment, disappeared during this phase. This fast recovery phase is proposed to represent reactivation of photoinhibited PS II, without dissassembly or incorporation of new D₁-protein. (2) A relatively slow light-dependent recovery phase took place at 20°C, but not at 6°C. In the presence of the chloroplast translation inhibitor streptomycin, part of the 2nd phase was inhibited. This phase is proposed to involve assembly of new Photosystem II centers, which is partly dependent on de novo synthesis of D₁-reaction center protein, but presumably is also using a preexisting pool of D₁-protein. Cold acclimation of the leaves resulted in a decreased sensitivity for photoinhibition of photosystem II. Recovery of photoinhibited photosystem II at 6°C of the cold-acclimated leaves was faster than in non-acclimated leaves, but this effect can be ascribed to diminished photoinhibitory damage.     

Effect of some environmental factors on cyanophage AS-1 development in Anacystis nidulans

The development cycle of the cyanophage AS-1 was studied in the host blue-green alga, Anacystis nidulans, under conditions that impair photosynthesis and under various light/dark regimes. Under standard conditions of incubation the 16-h development cycle consisted of a 5-h eclipse period and an 8-h latent period. Burst size was decreased by dark incubation to 2% of that observed in the light. An inhibitor of photosystem II, 3-(3,4-dichlorophenyl)-1,1-dimethyl urea (DCMU), reduced the burst size to 27% of that of the uninhibited control, whereas cyanophage production was completely abolished by carbonyl-cyanide m-chlorophenyl hydrazone (CCCP), an inhibitor of photosynthetic electron transport. Dark incubation of infected cells decreased the latent period by 1–2 h and the eclipse period by 1 h, once the cultures were illuminated. This suggests that adsorption took place in the dark. Intracellular growth curves indicated that light is necessary for viral development. Infected cells must be illuminated at least 13 h to produce a complete burst at the same rate as the continuously illuminated control. Low light intensities retarded the development cycle, and at lowest light intensities no phage yield was obtained. AS-1 is highly dependent on host cell photophosphorylation for its development.List of Abbreviations CCCP Carbonyl-cyanide m-chlorophenyl hydrazone - DCMU 3-(3,4-dichlorophenyl)-1,1-dimethyl urea - m.o.i. multiplicity of infection - O.D. optical density - PFU plaque-forming unit Dedicated to Prof. Roger Y. Stanier on the occasion of his 60th birthday     

Formation in the dark, of virus-induced deoxyribonuclease activity in Anacystis nidulans, an obligate photoautotroph.

In Anacystis nidulans, upon infection with cyanophage AS-1, after a lag period of 1 h the level of deoxyribonuclease (DNase) activity increaded rapidly up to 15- to 20-fold in 4 to 5 h in the light. In contrast, the ribonuclease and phosphomonoesterase activities increased significantly only 4 to 5 h after infection, i.e. as late as 1 h prior to lysis. In complete darkness, the nuclease levels remained unaltered. However, when the infected cells were exposed to light for 1 or 2 h after infection, the DNase level increased essentially to the same extent in the dark as in continuous light, although the complete replication cycle of the virus was impaired in the dark and cells lysed only in the continuously illuminated cultures. Inhibition of photosystem II with 3-(3,4-dichlorophenyl)-1-dimethylurea during the early illumination period strongly decreased the subsequent, infection-dependent increase in DNase activity in the dark. The virus-induced increase in DNase activity was also inhibited by chloramphenicol. The data suggest that, in spite of the obligate photoautotrophic nature of A. nidulans, dark metabolism is able to support fully the formation of some specific proteins if the triggering of their synthesis takes place in light.     

Adsorption of cyanophage AS-1 to unicellular cyanobacteria and isolation of receptor material from Anacystis nidulans.

Cells of unicellular cyanobacteria of typological group Ia, containing approximately 50 mol% guanine + cytosine (G+C) in their DNA (R. Y. Stanier, R. Kunisawa, M. Mandel, and G. Cohen-Bazire, Bacteriol. Rev. 35:171-205, 1971), were susceptible to infection by the cyanophage AS-1. Cyanobacteria of the same typological group, containing approximately 65 mol% G+C in their DNA, did not adsorb the cyanophage AS-1 or adsorbed it at a low rate. AS-1 was not propagated by any of the investigated strains with a high G+C content in their DNA. However, cells of strains 6907 and 6911 were lysed by cyanophage AS-1. A comparison of the host range of this phage with the lipopolysaccharide composition of host and non-host cell walls suggests that lipopolysaccharides are involved in the adsorption process. About 8 microgram of lipopolysaccharide per ml from host strains inactivated 50% of the particles of a solution containing 100 PFU/ml after 60 min of incubation at 30 degrees C. Material with receptor activity was extracted from the host strain Anacystis nidulans KM. The extract was purified of glycolipids and pigments, and a fraction showing receptor activity was isolated. This fraction contained three polypeptides of molecular weights between 54,000 and 64,000. Heat and protease treatment of whole cells and of isolated receptor material decreased the receptor activity. The fluorescence intensity of A. nidulans cells labeled with 1-anilino-8-naphthalene sulfonate was increased when AS-1 was adsorbed to these cells. The participation of lipopolysaccharides and proteins in the formation of the receptor complex is discussed.     

AS-1L - a newly discovered strain of Cyanophage AS-1 in GDR

In samples, taken from waters in the surroundings of Leipzig (GDR) in 1978, we found cyanophages in Central Europe for the first time. Among other cyanophages we isolated the new strain AS-1L. Out of 20 tested cultures of unicellular cyanobacteria seven strains belonging to the genus Synechococcus proved to be susceptible for this cyanophage. In morphology AS-1L corresponds to the cyanophage AS-1 found in the U.S.A., to which it is related serologically, too. AS-1L differs from the other strains of AS-1 by a shorter growth cycle, especially a shorter latent period, by the kinetics of inactivation by antiserum, and by a somewhat narrower pH scope of stability. Consequently the isolated cyanophage is to be looked at as a new strain of the cyanophage AS-1.     

Ultraviolet Light Inactivation and Photoreactivation of AS-1 Cyanophage in Anacystis nidulans

Black light effected photorecovery of AS-1 cyanophage and wild-type cells. However, only partial photoreactivation of AS-1 was observed in a partially photoreactivable mutant of Anacystis nidulans.     

Bacteriophage infection interferes with guanosine 3''-diphosphate-5''-diphosphate accumulation induced by energy and nitrogen starvation in the cyanobacterium Anacystis nidulans

Anacystis nidulans accumulates large amounts of guanosine 3'-diphosphate-5'-diphosphate (ppGpp) upon nutritional or energy starvation induced by light-to-dark shift, treatment with carbonylcyanide-m-chlorophenylhydrazone (an uncoupler), or treatment with L-methionine-DL-sulfoximine (an inducer of nitrogen starvation). In contrast to healthy A. nidulans cells, those infected by AS-1 cyanophage do not respond with ppGpp accumulation when starved after about one-third of the complete infection cycle, except, to some extent, under extreme conditions when both nitrogen deprivation and energy deprivation are induced simultaneously (darkening plus L-methionine-DL-sulfoximine treatment). In contrast to cyanophage infection in Anacystis, infection with T4 phage of Escherichia coli CP 78 cells does not affect their accumulation of ppGpp under treatments identical with or similar to those applied in the experiments with Anacystis. This difference in response of phage-infected heterotrophic and photoautotrophic cells to starvation seems to reflect differences in control of nutritional or energy metabolism rather than differences in ability to synthesize ppGpp.     

Induction of temperate cyanophage AS-1 by heavy metal - copper

Background  

It has been reported that some marine cyanophage are temperate and can be induced from a lysogenic phase to a lytic phase by different agents such as heavy metals. However, to date no significant reports have focused on the temperate nature of freshwater cyanophage/cyanobacteria. Previous experiments with cyanophage AS-1 and cyanobacteria Anacystis nidulans have provided some evidence that AS-1 may have a lysogenic life cycle in addition to the characterized lytic cycle.     

Signalling via rat dopamine D2-receptors expressed in mouse fibroblasts is not influenced by compounds binding to the sigma sites of these cells

The mouse fibroblast cell line LZR-1 is a well-established test system used to characterize the intrinsic activity of dopamine D₂-receptor ligands (Neve et al., Mol. Pharmac., 1989). This cell line is transfected with a eucaryotic expression vector containing the gene of the rat dopamine D_2B-receptor (short isoform of the D₂-receptor) (Bunzow et al., Nature, 1988). In addition to the expression of high levels of the rat dopamine D₂-receptor, these mouse cells also express sigma binding sites. Binding affinities of BMY 14,802, DTG, haloperidol, ( + )-pentazocine, ( + )-3-PPP, and ( + )-SKF 10,047 for the sigma binding sites as well as for the D₂-dopamine receptor in membranes of LZR-1 cells were determined. Using intact LZR-1 cells, it was found that the influence of sigma ligands on signalling via the dopamine D₂-receptor can be explained by their affinity for the latter receptor. Specific sigma ligands did not influence dopaminergic signal transduction in LZR-1 cells. It is therefore concluded that the LZR-1 cell is a suitable test model for determination of the intrinsic activity of dopamine D₂-receptor ligands even if these compounds have affinity for sigma binding sites.     

Evidence for photosynthetic independence of viral multiplication in cyanophage LPP-1 infected cyanobacterium Phormidium uncinatum

Abstract Pigment decomposition, oxygen evolution and CO₂ fixation were measured in the cyanobacterium Phormidium uncinatum after infection with cyanophage LPP-1, under light and dark conditions. A gradual decrease in para benzoquinone supported O₂ evolution, chlorophyll a and phycocyanin level were noticed after 6 h of infection. These results demonstrated decreased photosynthetic activity of the host P. uncinatum prior to the start of LPP-1 multiplication. Metabolic inhibitor investigations confirmed that the cyanophage LPP-1 multiplication was independent of host photosynthesis.     

Evidence for a restriction/modification-like system in Anacystis nidulans infected by cyanophage AS-1

Anacystis nidulans infected by AS-1 cyanophage contains an endonuclease (AS-1 endonuclease) which splits host DNA but not AS-1 phage DNA [Szekeres, M. (1981) Virology, 111, 1-10]. AS-1 phage DNA proved to be resistant not only to AS-1 endonuclease but also to a number of restriction endonucleases the recognition sites of which contain a central dG-dC dinucleotide. Since an unmodified 5'dG-dC dinucleotide was shown to be present at the sites at which DNA is cleaved by AS-1 endonuclease, the results suggest that the sites attacked preferentially by the AS-1 endonuclease are specifically protected on the AS-1 DNA molecule. The modification of AS-1 DNA was shown to occur specifically in infected Anacystis because AS-1 DNA fragments which are normally resistant to AS-1 endonuclease became susceptible to this enzyme if inserted into pBR322 plasmid and cloned in Escherichia coli. AS-1 DNA was shown to contain about 5% of a modified nucleotide which was not 5-methyldeoxycytidylic acid. Results presented and our earlier data suggest that in Anacystis infected by AS-1 phage, a restriction/modification-like system operates which is able to eliminate 'unwanted' (host) DNA selectively.     

The postmaturational cleavage of 23 S ribosomal RNA in Anacystis nidulans is inhibited by infection with cyanophage AS-1

The 23S (1.1×10⁶ mol.wt.) rRNA of Anacystis nidulans undergoes postmaturational cleavage to produce 0.9×10⁶ and 0.2×10⁶ molecular species. We have provided evidence in double labelling experiments, in which we could distinguish between the fate of molecules synthesized before and after infection, respectively, that infection with cyanophage AS-1 abruptly and completely inhibits the cleavage of 23S rRNA in Anacystis cells.     

感染丝状蓝藻的噬藻体的裂解周期和释放量的测定

近年来 ,随着浮游病毒的认识的深入 ,人们认识到浮游病毒对水体中初级生产力的影响是巨大的[1] ,其主要证据就是发现噬藻体在海洋蓝藻的种群控制上发挥着重要作用[2 ] 。噬藻体的释放量和裂解周期是衡量噬藻体感染力的重要指标 ,很多重要的生态指标如病毒在生态系统中对宿主的致死率、病毒种群得以维持的阈浓度等都需要使用病毒的释放量和裂解周期来加以推算[3,4 ] ,因此准确地测定这两个基本参数是十分重要的。在自然界 ,很多丝状蓝藻 ,如颤藻、鱼腥藻、螺旋藻、席藻等是能够形成水华的 ,其中有些还具有产毒的功能[5] 。丝状蓝藻的形态特征…     

Acid and alkaline phosphatase activity in the cyanobacteriumAnacystis nidulans under copper stress

The effect of lethal concentration of copper ions on the activities of acid and alkaline phosphatases was investigated in the cyanobacteriumAnacystis nidulans and the cyanophage AS-1 resistant mutant. When the level of phosphate declined in the medium, the cells were induced to form alkaline phosphatase (periplasmic protein) and acid phosphatase (cytoplasmic protein). In the presence of copper, the level of enzymes was low, suggesting that synthesis and activity were not completely abolished by copper. This may be related to the permeability of cell membrane.     

Inhibitory effect of heavy water on mutability of chemically injured Escherichia coli cells

After E. coli cells (WP2 and WP2uvrA) were treated with chemical mutagens (methyl methanesulfonate, MMS; N-methyl-N-nitrosourea, MNU; 4-nitroquinoline 1-oxide, 4NQO) in 1/15 M phosphate buffer, the mutability of the treated cells plated on a D₂O-agar plate was compared with that plated on an ordinary H₂O-agar plate. The mutation frequency decreased more or less on the D₂O-agar plate. The D₂O-substitution effects, as termed by the relative mutation frequencies (MF_D2O/MF_H2O), are 0.92 for MMS, 0.29 for MNU, and 0.42 for 4NQO in WP2, and 0.68 for MMS, 0.49 for MNU, and 0.16 for 4NQO in WP2uvrA. The D₂O effect seemed to be partly related to the function of the uvrA gene-associated products. The pH dependence of mutability was discussed in connection with the D₂O-substitution effect.     

Distribution of plasmids in cyanobacteria of the LPP group

Abstract The distribution of plasmid DNA has been studied in 23 strains and variants of non-heterocystous filamentous cyanobacteria that are susceptible to infection by the LPP-1 cyanophage (archetype). 21 have identical plasmid profiles and contain 3 plasmids of M _rs 0.9, 10 and approx. 12 · 10⁶ respectively. In one strain, Plectonema FS180, the plasmids have been designated pMP1, pMP2, and pMP3, respectively. pMP1 shows sequence homology with pMP2 and pMP3 but not with DNA from an LPP-type cyanophage. Plectonema UTEX 598 lacks the small plasmid only, while Plectonema UTEX 1541 is distinct amongst all these strains with 3 plasmids of M _rs 3, 10, and > 30 · 10⁶, respectively. The findings support the view that the majority of these strains may be independent isolates of a single species.     

维生素D3对黄颡鱼头肾极化分型的巨噬细胞影响

研究以黄颡鱼(Pelteobagrus fulvidraco)头肾巨噬细胞为研究对象,通过细菌脂多糖(LPS)和环磷酸腺苷(cAMP)分别诱导M1型和M2型极化,200 pmol/L维生素D₃孵育后对其形态学特征、生物学功能及极化相关基因的表达进行分析鉴定来确定维生素D₃在巨噬细胞极化中的调节作用。结果表明,维生素D₃能降低诱导后M1型和M2型巨噬细胞的死亡率,并增强巨噬细胞的吞噬活性。在M1型巨噬细胞中维生素D₃能够抑制活性氧(ROS)和炎症介质一氧化氮(NO)的产生,降低超氧阴离子自由基的活力,白介素1β(IL-1β)和肿瘤坏死因子-α(TNF-α)的表达水平显著降低(P<0.05);在M2型细胞中能够增加精氨酸酶的活性,显著增加白介素10(IL-10)和转化生长因子(TGF-β)的表达水平(P<0.05),最终抑制巨噬细胞向M1表型极化,促进巨噬细胞向M2表型极化,发挥抗炎作用;黄颡鱼头肾巨噬细胞中Nos-2和Arg-2分别是M1和M2巨噬细胞的生物标记基因。研究结果为进一步研究鱼...     

The effect of pH on the reduction kinetics of P-680 in tris-treated chloroplasts

The primary donor of Photosystem II (PS II), P-680, was photo-oxidized by a short flash and its rate of reduction was measured at different pH values by following the recovery of the absorption change at 820 nm in chloroplasts pretreated with a high concentration of Tris. The re-reduction is biphasic with a fast phase (dominant after the first flash) attributed to the donation by a donor, D₁, and a slow phase (usually dominant after the second flash) attributed to a back-reaction with the primary acceptor.

It is found that pH has a strong influence on the donation from D₁ (τ = 2 μs at pH 9, 44 μs at pH 4), but no influence on the back reaction (τ ≈ 200 μs). pH also influences the stability of the charge separation since the contribution of donation from D₁ at the second flash increases at lower pH, getting close to 100% at pH 4.     

The location of the chloride binding sites in the oxygen-evolving complex of spinach Photosystem II

³⁵Cl-NMR studies are presented here for spinach Photosystem II membranes inhibited by hydroxylamine (to remove Mn), Tris (to remove Mn and 18, 24 and 33 kDa polypeptides), and salt-washing (to remove 18 and 24 kDa; and 33 kDa polypeptides). Removal of Mn affects the ³⁵Cl-NMR binding curve only slightly, indicating that not all of the bound Mn is directly required for Cl-binding. Removal of both Mn and extrinsic polypeptides eliminates almost all of the Cl⁻-specific binding observable by NMR. Removal of the extrinsic 18 and 24 kDa polypeptides drastically changes the ³⁵Cl-NMR binding pattern; this effect is partially restored by the addition of 2 mM CaSO₄, and, to a lesser extent, by the partial rebinding of the polypeptides. Existence of Cl⁻ binding to the intrinsic polypeptides (e.g., D₁/D₂), with a peak at 0.5 mM Cl⁻, is shown in samples lacking 18, 24 and 33 kDa polypeptides. Thus, both intrinsic (i.e., on the D₁/D₂ membrane protein) and extrinsic (i.e., on the 33 kDa protein) binding sites for Cl⁻ are suggested to exist.