Application of light emitting diodes as a light source to a photosynthetic culture of Chlorobium thiosulfatophilum

Summary Economical light energy supply plays a key role in determining the success of industrial application of photosynthetic microorganisms. The bacteriochlorophyll a of C. thiosulfatophilum harvests the light at 760 nm, which oxidizes toxic H₂S by photosynthesis. Light emitting diode(LED), which emits a maximum intensity at 710 nm and 60% of its maximum at 760 nm, was adopted as an alternative light source to inefficient incandescent light. With the array of the LEDs adjustable to the reactor wall 95% of the light energy was saved over the incandescent light source in comparable conditions.     

Effects of light intensity distribution on growth of Rhodobacter capsulatus

For cultivation of photosynthetic cells under defined light intensity distributions, the repeated batch culture, in which a part of culture broth containing grown cells was repeatedly replaced at predetermined time intervals with a fresh medium to keep the cell concentration constant at an initial value, was employed. By use of this method the effects of the light intensity distribution on the growth characteristics of Rhodobacter capsulatus were studied. Unexpected decreases in the specific growth rate were observed in culture of R. capsulatus at high cell concentrations and a long light path length. Big differences in the light intensities of lightly and darkly illuminated portions in photobioreactors, which reflects the light intensity distribution, seemed to cause this phenomenon, which must be taken into consideration for stable growth of photosynthetic cells.     

Effect of light source on the microbiological desulfurization in a photobioreactor

Removal rates of a toxic pollutant-hydrogen sulfide were investigated using several light sources in photosynthetic desulfurization. An incandescent bulb has a broad spectrum starting from about 400?nm but emits most of its light energy beyond 800?nm as heat. LED₇₁₀ among those sources saved energy considerably comparing with the incandescent light, but the scattering and absorption was a problem in light transmission within the deep region of a bioreactor due to its own weak light intensity. Fluorescent light was inefficient in desulfurization in comparison with light sources illuminating with wide wavelength range, because of the weak transmittance at the peak wavelength of 460?nm. A combination of LED₇₁₀ and fluorescent lamp was estimated as an optimal light source in this study.     

The nature of floral signals in Arabidopsis. I. Photosynthesis and a far-red photoresponse independently regulate flowering by increasing expression of FLOWERING LOCUS T (FT)

Arabidopsis flowers in long day (LD) in response to signals transported from the photoinduced leaf to the shoot apex. These LD signals may include protein of the gene FLOWERING LOCUS T (FT) while in short day (SD) with its slower flowering, signalling may involve sucrose and gibberellin. Here, it is shown that after 5 weeks growth in SD, a single LD up-regulated leaf blade expression of FT and CONSTANS (CO) within 4-8 h, and flowers were visible within 2-3 weeks. Plants kept in SDs were still vegetative 7 weeks later. This LD response was blocked in ft-1 and a co mutant. Exposure to different LD light intensities and spectral qualities showed that two LD photoresponses are important for up-regulation of FT and for flowering. Phytochrome is effective at a low intensity from far-red (FR)-rich incandescent lamps. Independently, photosynthesis is active in an LD at a high intensity from red (R)-rich fluorescent lamps. The photosynthetic role of a single high light LD is demonstrated here by the blocking of the flowering and FT increase on removal of atmospheric CO(2) or by decreasing the LD light intensity by 10-fold. These conditions also reduced leaf blade sucrose content and photosynthetic gene expression. An SD light integral matching that in a single LD was not effective for flowering, although there was reasonable FT-independent flowering after 12 SD at high light. While a single photosynthetic LD strongly amplified FT expression, the ability to respond to the LD required an additional but unidentified photoresponse. The implications of these findings for studies with mutants and for flowering in natural conditions are discussed.     

Controlling light-use by Rhodobacter capsulatus continuous cultures in a flat-panel photobioreactor

The main bottleneck in scale-up of phototrophic fermentation is the low efficiency of light energy conversion to the desired product, which is caused by an excessive dissipation of light energy to heat. The photoheterotrophic formation of hydrogen from acetate and light energy by the microorganism Rhodobacter capsulatus NCIMB 11773 was chosen as a case study in this work. A light energy balance was set up, in which the total bacterial light energy absorption is split up and attributed to its destinations. These are biomass growth and maintenance, generation of hydrogen and photosynthetic heat dissipation. The constants defined in the light energy balance were determined experimentally using a flat-panel photobioreactor with a 3-cm optical path. An experimental method called D-stat was applied. Continuous cultures were kept in a so-called pseudo steady state, while the dilution rate was reduced slowly and smoothly. The biomass yield and maintenance coefficients of Rhodobacter capsulatus biomass on light energy were determined at 12.4 W/m(2) (400-950 nm) and amounted to 2.58 x 10(-8) +/- 0.04 x 10(-8) kg/J and 102 +/- 3.5 W/kg, respectively. The fraction of the absorbed light energy that was dissipated to heat at 473 W/m(2) depended on the biomass concentration in the reactor and varied between 0.80 and 0.88, as the biomass concentration was increased from 2.0 to 8.0 kg/m(3). The process conditions were estimated at which a 3.7% conversion efficiency of absorbed light energy to produced hydrogen energy should be attainable at 473 W/m(2).     

The Effect of an Incandescent Supplement on the Growth of Tomato Plants in Low Light

Young tomato plants were grown at low light flux densities (21W m^-2 for 8 h days) in growth cabinets under three types offluorescent lamps or under a fluorescent/incandescent mixedsource. Whilst net assimilation rates under the fluorescentlamps were in agreement with those calculated from the lampcharacteristics and the photosynthetic action spectrum, therate under the mixed source was about 20 per cent higher thanexpected. Relative growth rates and relative leaf area growthrates were also higher and leaf area ratios lower under thefluorescent/incandescent lamp combination than under the purefluorescent sources. Small differences in stem elongation, leaftemperature and dry weight distribution which were associatedwith the addition of incandescent radiation were not consideredto be responsible for these increases. When the light flux densityfrom the mixed source was reduced by 20 per cent, the plantgrowth parameters were then similar to those in fluorescentlight alone.     

Physiological predetermination of germination responses in Arabidopsis thaliana (L.) HEYNH.

Seed of Arabidopsis thaliana (L.) HEYNH., race Estland, producedunder temperature controlled axenic conditions and continuousexposure to white light containing markedly different proportionsof red and far-red radiant energy, were tested for photoinducedand dark-germination patterns. Dark germination percentagesfor after-ripened seed grown under cool white fluorescent lampsaveraged 45%, under cool white plus incandescent lamps 12%,and under incandescent lamps alone 0%. Since incandescent lampsprovide a larger proportion of energy of wavelengths greaterthan 700 nm, it is concluded that subsequent dark germinationis altered by the spectral quality to which the parent plantis exposed. The sensitivity of light germinating seed for photoinductionby red energy also was altered by changing the spectral qualityunder which they were grown. Light energy rich in wavelengthsgreater than 700 nm produced seed most sensitive to subsequentred induction. This sensitivity changed during storage and isprobably related to changes in after-ripening time. ¹Research was carried out in partial fulfillment of the Ph.D.requirements, the George Washington University. Research waspartially supported by Atomic Energy Commission Contract No.AT (30–1)2373. Published with approval of Secretary ofSmithsonian Institution (Received September 18, 1969; )     

Growth response of cotton to CO2 enrichment in differing light environments

Experiments were conducted to examine the growth responses of cotton (Gossypium hirsutum L. cv. Coker 315) to CO₂ enrichment under different light regimes. Plants were exposed to 350 or 700 μl l^?1 CO₂ and six light treatments differing in photosynthetic period length (8 or 16 h) and in photosynthetic photon flux density (PPFD) for 32 days of vegetative growth. Higher PPFD (1 100 μmol m^?2 s^?1) was provided by a combination of high intensity discharge and incandescent lamps (HID), and lower PPFD (550 μmol m^?2 s^?1) was provided by fluorescent and incandescent lamps (F) or HID and incandescent lamps with shade cloth (HID_s). Growth was generally much slower with the 8-h photosynthetic periods, but the growth stimulation by CO₂ enrichment was larger than with 16-h photosynthetic periods. After 28 to 32 days of treatment, the growth enhancement with CO₂ enrichment was 152 and 78% for 8- and 16-h photosynthetic periods, respectively, under HID; 100 and 77% in F, and 77 and 56% in HID_s. The higher PPFD of HID positively influenced the CO₂ effect only at the slower growth rate in the 8-h light period. The stimulation of leaf area expansion by CO₂ enrichment was also greater with the 8-h photosynthetic period for all light sources. These results, and others on net assimilation rate, shoot to root dry weight ratios and specific leaf weights, suggest that the growth response to CO₂ enrichment with the longer photosynthetic period was depressed by limiting factors, perhaps nutritional, in the growth environment. The results also show that extensive variability in CO₂ response can occur under light intensities which are often used in growth chamber experiments.     

The cytochrome bc1 complex of Rhodobacter sphaeroides can restore cytochrome c2-independent photosynthetic growth to a Rhodobacter capsulatus mutant lacking cytochrome bc1.

Plasmids encoding the structural genes for the Rhodobacter capsulatus and Rhodobacter sphaeroides cytochrome (cyt) bc1 complexes were introduced into strains of R. capsulatus lacking the cyt bc1 complex, with and without cyt c2. The R. capsulatus merodiploids contained higher than wild-type levels of cyt bc1 complex, as evidenced by immunological and spectroscopic analyses. On the other hand, the R. sphaeroides-R. capsulatus hybrid merodiploids produced only barely detectable amounts of R. sphaeroides cyt bc1 complex in R. capsulatus. Nonetheless, when they contained cyt c2, they were capable of photosynthetic growth, as judged by the sensitivity of this growth to specific inhibitors of the photochemical reaction center and the cyt bc1 complex, such as atrazine, myxothiazol, and stigmatellin. Interestingly, in the absence of cyt c2, although the R. sphaeroides cyt bc1 complex was able to support the photosynthetic growth of a cyt bc1-less mutant of R. capsulatus in rich medium, it was unable to do so when C4 dicarboxylic acids, such as malate and succinate, were used as the sole carbon source. Even this conditional ability of R. sphaeroides cyt bc1 complex to replace that of R. capsulatus for photosynthetic growth suggests that in the latter species the cyt c2-independent rereduction of the reaction center is not due to a structural property unique to the R. capsulatus cyt bc1 complex. Similarly, the inability of R. sphaeroides to exhibit a similar pathway is not due to some inherent property of its cyt bc1 complex.     

Photocatabolism of acetone by nonsulfur purple bacteria

Abstract Tests for the capacity of nonsulfur purple bacteria to photocatabolize acetone revealed that certain strains of Rhodobacter (Rb.) capsulatus and Rhodomicribium (Rm.) vannielii could grow on this organic compound. Phototrophic growth of R. capsulatus strain B10 on acetone was CO₂ dependent. Dark anaerobic or dark aerobic growth of R. capsulatus on acetone was not observed, although microaerobic growth in the dark did occur. Of a total of 13 species of nonsulfur purple bacteria examined, only strains of Rb. capsulatus and Rm. vannielii were found capable of photoheterotrophic growth on acetone.     

High-Intensity Vapor Lamp for Biological Research

A vapor arc light source has been adapted to the study of the lethal action on bacteria of near-ultraviolet (UV) and visible light. Its use makes possible much shorter exposure times than could be obtained from previously available sources. The output of radiant energy is sufficient to provide a fairly detailed action spectrum for lethality in the long-UV and visible region without the addition of exogenous sensitizers. Populations of cells of Escherichia coli WP2 were inactivated through five log(10) cycles with light at 460 nm. Significant inactivation also was obtained with light at 550 and 650 nm.     

Cloning and characterization of senC, a gene involved in both aerobic respiration and photosynthesis gene expression in Rhodobacter capsulatus.

The purple nonsulfur photosynthetic eubacterium Rhodobacter capsulatus is a versatile organism that can obtain cellular energy by several means, including the capture of light energy for photosynthesis as well as the use of light-independent respiration, in which molecular oxygen serves as a terminal electron acceptor. In this study, we have identified and characterized a novel gene, senC, mutations in which affect respiration as well as the induction of photosynthesis gene expression. The protein coded by senC exhibits 33% sequence identity to the yeast nucleus-encoded protein SCO1, which is thought to be a mitochondrion-associated cytochrome c oxidase assembly factor. Like yeast SCO1, SenC is required for optimal cytochrome c oxidase activity in aerobically grown R. capsulatus cells. We further show that senC is required for maximal induction from the puf and puh operons, which encode the structural polypeptides of the light-harvesting and reaction center complexes.     

Influence of the degree and mode of light limitation on growth characteristics of the Rhodobacter capsulatus continuous cultures

The influence of the degree and mode of light limitation on growth characteristics of turbidostat cultures of Rhodobacter capsulatus was investigated using mass and energy balance regularities. Light limitation was achieved by increasing the steady-state biomass concentration at constant incident light intensity ( approximately 100 W/m(2)) or by decreasing the incident light intensity at constant steady-state biomass concentration ( approximately 500 mg of dry biomass/L). It was shown that under conditions of light limitation of Rh. capsulatus, the content of P and N in the biomass as well as the biomass degree of reduction were determined by the growth rate of the cultures. The energetic yield of biomass of Rh. capsulatus and total bacteriochlorophyll a content increased when light limitation increased. These parameters were higher in the cultures, in which light limitation was achieved by lowering the incident light intensity at low biomass concentration. This seems to be due to different distribution of light within the photobioreactor when dissimilar modes of light limitation were used.     

低强度532nm与633nm激光血管内照射生物效应比较

目的：研究同等照射条件的低强度532nm与633nm激光血管内照射对家兔白细胞计数与淋巴细胞凋亡的影响,比较两种激光生物效应的特点。方法：用532nm和633nm激光对健康日本大耳白家兔血管内照射,平均照射功率均设在5mW左右,照射总能量约12J。两组家兔均于照前及照后1d、4d、7d、11d进行外周血白细胞计数,于照前及照后1d、5d进行淋巴细胞凋亡分析。结果：532nm激光照射后,家兔外周血白细胞计数表现为先显著升高后趋向恢复,633nm激光照射后白细胞计数变化类似,但与照前相比升高不明显;与照前相比,两组家免外周血淋巴细胞凋亡比例于照后1d均明显降低,照后5d均显著升高;两组家兔相比,照射后白细胞计数差别明显,但淋巴细胞凋亡比例差异不显著。结论：同等照射条件下,低强度532nm与633nm激光照射血液的生物效应相似,都可以促进白细胞的代谢更新,只是532nm激光的效应略强一些。     

半导体激光对紫球藻生物学效应的影响

采用波长650nm,功率40mW,功率密度13W／cm^2的半导体激光,对紫球藻（Porphyridium cruentum)进行诱变,辐照时间分别为5min、10min、20min。通过对紫球藻每天细胞数、叶绿素a、第7d细胞干重和胞外多糖产量的测定可知：与对照组比较,3个处理对紫球藻生长及胞外多糖产生影响,5min、10min均有不同程度的促进作用,其中5min作用最明显,而20min则有抑制作用。     

A single flavoprotein,AppA, integrates both redox and light signals in Rhodobacter sphaeroides

Anoxygenic photosynthetic proteobacteria exhibit various light responses, including changing levels of expression of photosynthesis genes. However, the underlying mechanisms are largely unknown. We show that expression of the puf and puc operons encoding structural proteins of the photosynthetic complexes is strongly repressed by blue light under semi-aerobic growth in Rhodobacter sphaeroides but not in the related species Rhodobacter capsulatus. At very low oxygen tension, puf and puc expression is independent of blue light in both species. Photosynthetic electron transport does not mediate the blue light repression, implying the existence of specific photoreceptors. Here, we show that the flavoprotein AppA is likely to act as the photoreceptor for blue light-dependent repression during continuous illumination. The FAD cofactor of AppA is essential for the blue light-dependent sensory transduction of this response. AppA, which is present in R. sphaeroides but not in R. capsulatus, is known to participate in the redox-dependent control of photosynthesis gene expression. Thus, AppA is the first example of a protein with dual sensing capabilities that integrates both redox and light signals.     

The thermodynamic response of soft biological tissues to pulsed ultraviolet laser irradiation.

The physical mechanisms that enable short pulses of high-intensity ultraviolet laser radiation to remove tissue, in a process known as laser ablation, remain obscure. The thermodynamic response of biological tissue to pulsed laser irradiation was investigated by measuring and subsequently analyzing the stress transients generated by pulsed argon fluorine (ArF, lambda = 193 nm) and krypton fluorine (KrF, lambda = 248 nm) excimer laser irradiation of porcine dermis using thin-film piezoelectric transducers. For radiant exposures that do not cause material removal, the stress transients are consistent with rapid thermal expansion of the tissue. At the threshold radiant exposure for ablation, the peak stress amplitude generated by 248 nm irradiation is more than an order of magnitude larger than that produced by 193 nm irradiation. For radiant exposures where material removal is achieved, the temporal structure of the stress transient indicates that the onset of material removal occurs during irradiation. In this regime, the variation of the peak compressive stress with radiant exposure is consistent with laser-induced rapid surface vaporization. For 193 nm irradiation, ionization of the ablated material occurs at even greater radiant exposures and is accompanied by a change in the variation of peak stress with radiant exposure consistent with a plasma-mediated ablation process. These results suggest that absorption of ultraviolet laser radiation by the extracellular matrix of tissue leads to decomposition of tissue on the time scale of the laser pulse. The difference in volumetric energy density at ablation threshold between the two wavelengths indicates that the larger stresses generated by 248 nm irradiation may facilitate the onset of material removal. However, once material removal is achieved, the stress measurements demonstrate that energy not directly responsible for target decomposition contributes to increasing the specific energy of the plume (and plasma, when present), which drives the gas dynamic expansion of ablated material. This provides direct evidence that ultraviolet laser ablation of soft biological tissues is a surface-mediated process and not explosive in nature.     

Characterization of the photoreduction of the secondary quinone QB in the photosynthetic reaction center from rhodobacter capsulatus with FTIR spectroscopy

The photoreduction of the secondary quinone acceptor QB in reaction centers (RCs) of the photosynthetic bacteria Rhodobacter (Rb.) capsulatus has been investigated by light-induced FTIR difference spectroscopy in 1H2O and 2H2O. The Q-B/QB FTIR spectra reflect reorganization of the protein upon electron transfer, changes of protonation state of carboxylic acid groups, and (semi)quinone-protein interactions. As expected from the conservation of most of the amino acids near QB in the RCs from Rb. capsulatus and Rb. sphaeroides, several protein and quinone IR bands are common to both spectra, e.g., the 1728 cm-1 band is assigned to proton uptake by a carboxylic acid residue, most probably Glu L212 as previously proposed for Rb. sphaeroides RCs. However, noticeable changes are observed at 1709 cm-1 (deprotonation of a Glu or Asp residue), 1674 and 1659 cm-1 (side chain and/or backbone), around 1540 cm-1 (amide II), and in the semiquinone absorption range. This FTIR study demonstrates that the environment of the secondary quinone in Rb. capsulatus is close but not identical to that in Rb. sphaeroides suggesting slight differences in the structural organization of side chains and/or ordered water molecules near QB.     

钝顶螺旋藻形态、生长及光合作用对不同波段太阳辐射的响应

为探讨中不同波段的光合有效辐射对钝顶螺旋藻(Arthrospira platensis)形态、生长及光合作用的影响,实验将钝顶螺旋藻D-0083藻液转入带塞的石英管中, 石英管水平置于阳光下并在其上覆盖不同的截止型和带通型滤光片, 以使藻丝接受不同波段的太阳辐射; 并检测其生长、形态与光合活动的变化。结果发现: 所有波段 (320500、395700、510700和610700 nm) 光合有效辐射下的藻丝均螺旋变紧且生物量增加。其中以包含少量紫外辐射A (Ultraviolet-A)的蓝光波段 (320500 nm)和红光波段(600700 nm) 对藻丝形态变化、生长及光合速率的诱发效率较高。在320500、395700、510700和 610700 nm波段上的单位能量光照引起钝顶螺旋藻螺距变化的效率分别为0.070、0.015、0.021、0.045 m/(Wm2)。 波段320500 nm虽然会轻微抑制钝顶螺旋藻D-0083的有效光化学效率(Fv'/Fm')、电子传递速率(ETR)和藻蓝蛋白的荧光发射, 但是却能够有效诱导其藻丝变紧促进生长。此外, 钝顶螺旋藻D-0083的藻丝变紧程度、比生长速率变化与不同波段太阳辐射下藻丝体的光合性能相一致。该研究表明任何波段的光合有效辐射都能使螺旋藻藻丝螺旋变紧并引发生长和光合作用, 其中以蓝光和红光的效率最高。