Evidence from action and fluorescence spectra that UV-induced violet-blue-green fluorescence enhances leaf photosynthesis

We assessed the contribution of UV-induced violet-blue-green leaf fluorescence to photosynthesis in Poa annua, Sorghum halepense and Nerium oleander by measuring UV-induced fluorescence spectra (280-380 nm excitation, 400-550 nm emission) from leaf surfaces and determining the monochromatic UV action spectra for leaf photosynthetic O2-evolution. Peak fluorescence emission wavelengths from leaf surfaces ranged from violet (408 nm) to blue (448 nm), while excitation peaks for these maxima ranged from 333 to 344 nm. Action spectra were developed by supplementing monochromatic radiation from 280 to 440 nm, in 20 nm increments, to a visible nonsaturating background of 500 mumol m-2 s-1 photosynthetically active radiation and measuring photosynthetic O2-evolution rates. Photosynthetic rates tended to be higher with the 340 nm supplement than with higher or lower wavelength UV supplements. Comparing photosynthetic rates with the 340 nm supplement to those with the 400 nm supplement, the percentage enhancement in photosynthetic rates at 340 nm ranged from 7.8 to 9.8%. We suspect that 340 nm UV improves photosynthetic rates via fluorescence that provides violet-blue-green photons for photosynthetic energy conversion because (1) the peak excitation wavelength (340 nm) for violet-blue-green fluorescence from leaves was also the most effective UV wavelength at enhancing photosynthetic rates, and (2) the magnitude of photosynthetic enhancements attributable to supplemental 340 nm UV was well correlated (R2 = 0.90) with the apparent intensity of 340 nm UV-induced violet-blue-green fluorescence emission from leaves.     

两种不同光谱类型的R-藻红蛋白的荧光性质研究

红藻中的R-藻红蛋白(R-PE)依照其吸收光谱可分为两种不同的光谱类型,即“双峰型”和“三峰型”。本文通过对不同pH条件下的R-PE的荧光光谱及荧光寿命的研究,发现“三峰型”R-PE的pH稳定范围较“双峰型”R-PE大。在R-PE浓度对荧光光谱的影响实验中,随着蛋白浓度的增加,荧光峰位置逐渐红移。荧光寿命逐渐增大,荧光强度先行增加而后减弱。用碘离子对其荧光进行猝灭,随着碘离子浓度的增大,荧光强度逐渐降低,荧光寿命逐渐缩短,并服从Stem-Volmer规则。     

Remote Raman and fluorescence studies of mineral samples

In the present study, we investigated remote laser-induced fluorescence (LIF), at a distance of 4.8 m, of a variety of natural minerals and rocks, and Hawaiian Ti (Cordyline terminalis) plant leaves. These minerals included calcite cleavage, calcite onex and calcite travertine, gypsum, fluorapatite, Dover flint and chalk, chalcedony and nephelene syenite, and rubies containing rock. Pulsed laser excitation of the samples at 355 and 266 nm often resulted in strong fluorescence. The LIF bands in the violet-blue region at approximately 413 and approximately 437 nm were observed only in the spectrum of calcite cleavage. The green LIF bands with band maxima in the narrow range of approximately 501-504 nm were observed in the spectra of all the minerals with the exception of the nephelene syenite and ruby rocks. The LIF red bands were observed in the range approximately 685-711 nm in all samples. Excitation with 532 nm wavelength laser gave broad but relatively low fluorescence background in the low-frequency region of the Raman spectra of these minerals. One microsecond signal gating was effective in removing nearly all background fluorescence (with peak at approximately 610 nm) from calcite cleavage Raman spectra, indicating that the fluorescence was probably from long-lifetime inorganic phosphorescence.     

Flavonoid distribution in tissues of Phillyrea latifolia L. leaves as estimated by microspectrofluorometry and multispectral fluorescence microimaging

A new method for detecting the tissue-specific distribution of flavonoids has been developed by coupling microspectrofluorometry and multispectral fluorescence microimaging techniques. Fluorescence responses of cross sections taken from 1 year old Phillyrea latifolia leaves exposed to full (sun leaves) or 15% (shade leaves) solar radiation in a coastal area of Southern Tuscany were analyzed. Fluorescence spectra of different tissue layers, each normalized at its fluorescence maximum, that were stained or not stained with Naturstoff reagent A (in ethanol), under excitation with UV light (lambdaexc = 365 nm) or blue light (lambdaexc = 436 nm) were recorded. The shape of the fluorescence spectra of tissue layers from shade and sun leaves differed only under UV excitation. The fluorescence of stained cross sections from sun and shade leaves as well as from different layers of sun leaves received a markedly different contribution from the blue (470 nm) and the yellow-red (580 nm) wavebands. Such changes in tissue fluorescence signatures were related to light-induced changes of extractable caffeic acid derivatives and flavonoid glycosides, namely quercetin 3-O-rutinoside and luteolin 7-O-glucoside. Wall-bound phenolics, i.e. hydroxycinnamic acids (p-coumaric, ferulic and caffeic acid) and flavonoids (apigenin and luteolin derivatives), did not substantially differ between sun and shade leaves. A Gaussian deconvolution analysis of fluorescence spectra was subsequently performed to estimate the contribution of flavonoids (emitting at 600 nm, F600 [red fluorescence contribution = signal integrated over a Gaussian band centered at about 600 nm]) relative to the tissue fluorescence (Ftot [total fluorescence = signal integrated over the whole fluorescence spectrum]). The F600/ Ftot ratios sharply differed between analogous tissues of sun and shade leaves, as well as among tissue layers within each leaf type. A highly resolved picture of the tissue flavonoid distribution was finally provided through a fluorescence microimaging technique by acquiring fluorescence images at the blue (fluorescence at about 470 nm [F470]) and yellow-red (fluorescence at about 580 nm [F580]) wavelengths and correcting the F580 image for the contribution of nonflavonoids to the fluorescence at 580 nm. Monochrome images were elaborated by adequate computing functions to visualize the exclusive accumulation of flavonoids in different layers of P. latifolia leaves. Our data show that in shade leaves flavonoids almost exclusively occurred in the adaxial epidermal layer. In sun leaves flavonoids largely accumulated in the adaxial epidermal and subepidermal cells and followed a steep gradient passing from the adaxial epidermis to the inner spongy layers. Flavonoids also largely occurred in the abaxial epidermal cells and constituted the exclusive class of phenylpropanoids synthesized by the cells of glandular trichomes. The proposed method also allowed for the discrimination of the relative abundance of hydroxycinnamic derivatives and flavonoids in different layers of the P. latifolia leaves.     

Boltwoodite [K(UO2)(SiO3OH)(H2O)1.5] and compreignacite K2[(UO2)3O2(OH)3]2.7H2O characterized by laser fluorescence spectroscopy

Synthetically prepared boltwoodite and compreignacite were characterized with time-resolved laser-induced fluorescence spectroscopy (TRLFS). The obtained TRLFS emission spectra of both synthesized uranium minerals differ from each other in their positions of the vibronic peak maxima and in their fluorescence lifetimes. Also, the shapes of the spectra and their respective intensities are different. The TRLFS-spectrum of boltwoodite showed well-resolved sharp vibronic peaks at 485.1, 501.5, 521.2, 543.0, 567.4, and 591.4nm with deep notches between them and compreignacite is characterized by two broad peaks with various shoulders. Here five emission bands were identified at 500.7, 516.1, 532.4, 554.3, and 579.6nm. The shape of the TRLFS spectra of compreignacite is typical for uranium in a hydroxide coordination environment. For both minerals two fluorescence lifetimes were extracted. The two species of boltwoodite and compreignacite, respectively, showed the same positions of the peak maxima showing that the coordination environments are similar, but differ in the chemistry and number of possible quenchers, e.g. water molecules and hydroxide groups. For boltwoodite fluorescence lifetimes of 382 and 2130ns, and for compreignacite shorter ones of 202 and 914ns, respectively, were determined. The spectroscopic signatures of the two uranyl minerals reported here could be useful for identifying uranyl(VI) mineral species as colloids, as thin coatings on minerals, as minor component in soils, or as alteration products of nuclear waste.     

Photophysical properties of carborane-containing derivatives of 5,10,15,20-tetra(p-aminophenyl)porphyrin

Absorption, fluorescence emission, fluorescence excitation spectra and fluorescence decay kinetics of carborane derivatives of 5,10,15,20-tetra(p-aminophenyl)porphyrin have been investigated. Carborane derivatives are prepared by acylation of the amino groups of 5,10,15,20-tetra(p-aminophenyl)porphyrin by 9-carboranyl acetyl chloride. From the analysis of the absorption and fluorescence spectra, it is concluded that covalent linking of carborane molecules to the tetraphenylporphyrin molecule significantly changes the self-conjugated pi-system of the porphyrin macrocycle: positions of maxima of absorption and fluorescence spectra shift to the red region by 3-8 nm; the halfwidths of these bands are broadened by 2.5-5.0 nm; the relative intensity of the bands I-IV also changes. The fluorescence decay kinetics of the carborane derivatives are biexponential. According to the experimental data and model simulation, it is concluded that the intramolecular electron transfer proceeds from the porphyrin excited part of the molecule to carboranyls with a rate constant of 415 ps(-1) and efficiency of 0.16-0.8. Recombination of separated charges occurs within 1.4 ns.     

利用激光腔内共振衰减技术研究CH2 CHO自由基的近紫外吸收光谱

Near-ultraviolet absorption spectrum of the B 2A" 0 ← X 2A" band of the vinoxy radical（CH2CHO）is recorded by cavity ringdown spectroscopy（CRDS）. The absorption spectrum shows a series of vibronic bands starting from 28786 cm - 1 and an increasing broad background towards higher photon energy. The CRDS absorption spectrum is similar to an early low-resolution absorption spectrum;and the vibronic peak positions match well with those in the laser-induced fluorescence and photofragment yield spectra.     

LIF technique offers the potential for the detection of cadmium-induced alteration in photosynthetic activities of Zea Mays L.

The laser-induced fluorescence spectra of leaves of Zea mays L. plants treated with different concentrations (0.01, 0.10 and 1.00 mM) of cadmium were recorded in region 650–800 nm using 488 nm line of Argon Ion laser as excitation source and PMT as detector. Besides this, blue-green fluorescence and Chl fluorescence were also measured using third harmonic (355 nm) of Nd:YAG laser as excitation source and 320 M monochromator with intensified charge coupled device as a detector in the region 400–800 nm. These spectra have been used to analyse the effect of several doses of cadmium on the photosynthetic activities of Z. mays L. plants. The fluorescence intensity ratios (FIR) of control as well as treated Z. mays L. were calculated by evaluating curve-fitted parameters using Gaussian spectral function. In addition, growth parameters like photosynthetic pigments content were also estimated. The chlorophyll fluorescence intensity ratio F685/F735 excited by both 488 and 355 nm lines are strongly correlated with photosynthetic pigments content (total chlorophyll and carotenoids) and their ratios. Consequently, there also existed a correlation between the blue-green fluorescence intensity ratio F470/F540 and photosynthetic pigments content.     

基于羟苯基苯并咪唑的Zn2+比率荧光探针

通过羰基将两分子2-(4-氨基-2-羟苯基)苯并咪唑(4-AHBI)连接,合成了结构高度对称的新化合物N,N′-二-[3-羟基-4-(2-苯并咪唑)苯基]脲(C27H20N6O3,1),测试了不同溶剂条件下1的紫外吸收和荧光发射光谱,研究了1对Zn2+的选择性识别作用。结果表明,随着溶剂极性的增大,1的紫外吸收峰发生蓝移,激发态分子内质子转移(ESIPT)荧光发射峰明显增强。与4-AHBI相比,1在乙腈溶液中的紫外吸收强度增强约3.5倍,最大吸收峰红移8 nm,荧光发射增强8倍多。1在乙腈溶液中的Zn2+荧光响应行为表明1与Zn2+的结合将导致1在445 nm处的荧光强度不断降低,而在395 nm处出现的新峰的荧光强度不断增强,具有比率荧光探针的特点,而且检测范围较宽,可达1×10-6-1×10-2 mol.L-1。     

Detection of Vibrational Spectroscopic Biomarkers of the Effect of Gold Nanoparticles on Wheat Seedlings Using Attenuated Total Reflectance Fourier Transform Infrared Spectroscopy

The aim of this study is to evaluate the biochemical changes in the leaves of wheat seedlings exposed to gold nanoparticles (AuNPs) nondestructively and rapidly using attenuated total reflectance Fourier transform infrared spectroscopy and laser-induced fluorescence. The 18?nm size gold nanoparticles are synthesized by citrate reduction. For analyzing the effect of gold nanoparticles on wheat seedlings, the treatment of gold nanoparticles was applied to the seedlings through roots and following the spectroscopic measurement of biochemical signatures. The laser-induced fluorescence measurement has been performed to access the effect of gold nanoparticles on the chlorophyll concentration of wheat seedlings. The decrease in the fluorescence intensity and the fluorescence intensity ratio on the treatment of gold nanoparticles indicates increase in the concentration of chlorophyll in the leaves of wheat seedlings. The attenuated total reflectance Fourier transform infrarred spectroscopy in combination with principal component analysis has been used to visualize the biochemical changes in the cellulose, hemicellulose, pectin, lignin, amino acids, proteins, and lipid of the leaves of wheat seedlings by recording infrared spectra in the region from 4000 to 400?cm^?1. Principal component analysis applied to the preprocessed infrared data clearly distinguishes the spectral variability between control and gold nanoparticle treated seedlings. The study shows that exposure of gold nanoparticles increases the concentrations of cellulose, hemicelluloses, pectin, and lignin in the leaves of wheat seedlings. The increase in these chemicals indicates the modulation of cell walls of the wheat seedlings by the gold nanoparticle treatment. The exposure to gold nanoparticles also enhances the expression of lipid and proteins in the leaves of wheat seedlings.     

对微环境敏感的系列双亲卟啉的光谱研究

研究了系列双亲卟啉(四苯酚基卟啉P₀及其烷氧基衍生物P₁,P₂,P₃)在不同微环境下的电子吸收光谱和荧光发射及荧光激发光谱.研究发现,卟啉在THF溶液中以单体形式存在,并且其侧链取代基对卟啉电子态的影响很小;然而卟啉在CTAB胶束溶液中的光谱特性却表现出很大差异,由此分析了不同侧链取代基对卟啉分子聚集行为和定位性质的影响,初步解释了卟啉在CTAB胶束溶液中随体系pH值改变而发生的荧光猝灭现象.     

Raman Spectrum of Er-Y-codoped ZrO2 and Fluorescence Properties of Er3+

Er-Y-codoped ZrO2 mixed oxides with monoclinic, tetragonal and cubic structures were prepared by a sol-gel method. The crystal structure of ZrO2 matrix and the effect of the ZrO2 phases on the fluorescence properties of Er3+ were studied using Raman spectroscopy. The results indicated that the fluorescence properties of Er3+ depend on its local ZrO2 crystal structures. As ZrO2 matrix transferred from monoclinic to tetragonal and cubic phase, the Raman and fluorescence bands of Er3+ decreased in intensities and tended to form a single peak. With 632.8 nm excitation, the bands between 640 and 680 nm were attributed to the fluorescence of Er3+ in the ZrO2 environment. However, only the fluorescence was observed and no Raman spectra were seen under 514.5 nm excitation, while only Raman spectra were observed under 325 nm excitation. UV Raman spectroscopy was found to be more sensitive in the surface region while the information provided by XRD mainly came from the bulk. The phase with lower symmetry forms more easily on the surface than in the bulk.     

Biological variability in the ratios of protochlorophyllide forms in leaves and epicotyls of dark-grown pea (Pisum sativum L.) seedlings (a statistical method to resolve complex spectra)

Low-temperature (77K) fluorescence emission spectra of 100 dark-grown pea (Pisum sativum L.) seedlings of various ages were measured. The spectra of the 100 leaf samples were collected into a separate data group and those of epicotyls formed another one. This group was divided into three sub-groups as spectra of uppermost, middle and lowermost 3 cm sections. Further sub-groups were formed on the basis of the ages of the plants. The spectra were normalized to their total integral values (within the 580-780 nm region) then the AVERAGE (arithmetic mean function) and AVEDEV (average of the absolute deviations of data points of their mean function) spectra were calculated. Very sharp bands were found in the AVEDEV spectra. Even the strongly overlapped 629 and 636 nm emission bands appeared as separate peaks, due to the decrease of their half-bandwidth values in the AVEDEV function. Both types of spectra were resolved into Gaussian components. The results showed that the variabilities of the 633 and 655 nm protochlorophyllide forms were similar in the leaves. In epicotyls, the protochlorophyllide forms had different variabilities, especially in the middle sections. The most variable was the amplitude of the 636 nm band and the variabilities of the 629 and 655 nm bands were smaller but still remarkable. The calculation of AVEDEV spectra is an effective method to study the biological variability and spectral resolution of biological samples containing chromophores with multiple spectral properties.     

Non-destructive Phenotyping of Chili Pepper Ripening Using Spectroscopic Probes: A Potential Approach for Shelf-Life Measurement

This study explores the application of spectroscopic techniques (laser induced fluorescence, Raman and attenuated total reflectance Fourier transform infrared) coupled with principal component analysis for the nondestructive, extraction free and rapid evaluation of biochemical changes associated with ripening of chili peppers at four stages (mature, pre-ripe, ripe and post-ripe). The analysis of the fluorescence spectra of the exocarp of chili pepper shows a decrease in the intensity of chlorophyll bands at 685 and 735?nm and an increase in the intensity of carotenoid fluorescence bands at 490–500?nm and 565–580?nm with progress in the ripening stages. These changes are regarded to be significant phenotypic markers for the ripening of chili peppers. The observed changes in the position of carotenoid bands in Raman spectra at 1004, 1156, 1188, and 1524?cm^?1 with increase in their intensity indicating the accumulation of carotenoids and change in the carotenoid composition from β-carotene in the mature chilis to capsanthin in the ripe chilis. In addition, the infrared spectra show changes in the carbohydrates, amide II, amide I and cutin at various stages of ripening. Also, the variation in the position of pectin bands indicates change in its molecular mass with decreasing content. The determined spectral signatures can be used as biomolecular index for effective monitoring of the ripening of chili peppers. The commercial application of noninvasive spectroscopic probes will be advantageous for the phenotyping of economically important plant parts, screening, grading, shelf life estimation and quality standardization.     

不同环境介质中芘的三维荧光光谱研究

本文首次运用三维荧光光谱研究芘在不同环境介质中的荧光特性, 揭示芘的F3/F4反映的是环境有序性介质的形成, 而不是所处环境极性大小的一个量度,F1/F3才是其所处环境极性大小的一个量度, 结果显示芘的三维荧光光谱可以更好地对环境性质进行研究, 将进一步扩大芘的应用范围。     

Fluorescence resonance energy transfer between polyphenolic compounds and riboflavin indicates a possible accessory photoreceptor function for some polyphenolic compounds

The photoreceptive extreme tip of the wheat coleoptile exhibits intense green-yellow fluorescence under UV light, suggesting the presence of UV-absorbing materials. Fluorescence spectra of the intact coleoptile tip and tip homogenate showed the presence of the known photoreceptor pigments flavin and carotene, and a preponderance of phenolic compounds. Absorption spectra and fluorescence spectra of various phenolic compounds showed close overlap with the absorption and fluorescence spectra of the wheat coleoptile tip homogenate. Fluorescence spectra of several phenolic compounds showed close overlap with the absorption bands of flavin, carotene and pterine, suggesting possible energy transduction from phenols to these photoreceptors. Excitation of gentisic acid and ferulic acid with 340 nm light in the presence of flavin showed enhancement of flavin fluorescence in a concentration- and viscosity-dependent fashion, indicating fluorescence resonance energy transfer between them and riboflavin. Furthermore, several phenolic compounds tested generated superoxide anion on excitation at 340 nm, suggesting that superoxide-dependent signal cascades could operate in a polyphenol-mediated pathway. Phenolic compounds thus may act as accessory photoreceptors bringing about excitation energy transfer to the reactive photoreceptor molecules, or they may take over the function of the normal photoreceptor in genetic mutations lacking the system, or both processes may occur. The responses of plants to UV-B and UV-A light in mutants may be explained in terms of various phenolics acting as energy transducers in photoreceptor functioning.     

EXCITATION ENERGY TRANSFER IN THE CRYPTOPHYTES. FLUORESCENCE EXCITATION SPECTRA AND PICOSECOND TIME-RESOLVED EMISSION SPECTRA OF INTACT ALGAE AT 77 K

Excitation spectra of chlorophyll- a (Chl- a ) fluorescence in intact cells of Cryptomonas ovata, Chroomonas pauciplastida and Chroomonas salina were determined at 77 K. For all species the excitation spectra for emission from Chl- a associated with photosystem II (PSII) showed increased contributions by a carotenoid (493 nm) and phycobiliproteins, and decreased contributions by carotenoid (417 nm, 505 nm) and Chl- a (445 nm) as compared to excitation spectra for emission from Chl- a associated with photosystem I (PSI). Excitation spectra of C. salina and C. ovata showed an increased contribution by Chl- c ² to PSII Chl- a fluorescence emission. In all three species the absorbance band positions of Chl- a , as determined from the excitation spectra, were similar to those previously described in green plants. green algae and phycobilisome-containing organisms. Time-resolved 77 K fluorescence emission spectra of C. ovata and C. salina showed successive emission from both phycoerythrin and Chl- c ², PSII Chl- a , and PSI Chl- a. C. pauciplastida showed successive emission from phycocyanin, PSII Chl- a , and PSI Chl- a. Spectral red-shifts with time were observed for the phycobiliprotein peaks in all three species. The fluorescence decay of phycoerythrin in C. ovata and C. salina was faster than that of phycocyanin in C. pauciplastida. The results are discussed in relation to the organization of the antenna pigments of PSII and PSI in the cryptophyte algae.     

Spectroscopic properties of protochlorophyllide analyzed in situ in the course of etiolation and in illuminated leaves

The spectroscopic properties of photoactive (i.e. flash-transformable) and nonphotoactive protochlorophyll(ide)s (Pchl(ide)) were reinvestigated during the development of bean leaves in darkness. Two phases in the process of Pchl(ide) accumulation were apparent from quantitative measurements of pigment content: a lag phase (first week) during which photoactive Pchl(ide) accumulated faster than nonphotoactive Pchl(ide); and a fast phase (second week), showing parallel accumulation of both types of Pchl(ide). 'Flashed-minus-dark' absorbance difference spectra recorded in situ at 77 K showed that P650-655 was the predominant form of photoactive protochlorophyllide regardless of developmental stage. Quantitative analysis of energy migration processes between the Pchl(ide) forms showed the existence of energy transfer units containing a 1:8 ratio of nonphotoactive and photoactive Pchl(ide)s during development. Gaussian deconvolution of in situ 77 K fluorescence spectra indicated that the 633 nm band of nonphotoactive Pchl(ide) was made of four bands, at 625, 631, 637 and 643 nm, whose relative amplitudes only slightly changed during development. The emission band of photoactive Pchlide was also analyzed using the same method. Three components were found at 644, 652 and 657 nm. The emission band of P650-655 included the last two components, which become predominant only in fully etiolated plants. Photoactive Pchlide with an emission maximum at 653 nm was detected in the light during development of leaves of photoperiodically grown plants.     

BINDING OF HEMATOPORPHYRIN DERIVATIVE TO BRAIN TUMOR CELLS—A FLUORESCENCE SPECTROSCOPIC STUDY

The binding of hematoporphyrin derivative (HpD) to brain tumor cells and their photosensitivity was studied as a function of HpD concentration, time of incubation and growth phase of cells. Upon binding to cells, HpD showed three fluorescence bands at 616, 636 and 678 nm. In plateau phase cells a fluorescence band at 636 nm was predominant, which was further enhanced by increasing HpD concentration and/or increasing incubation time. In exponential phase cells the maximum fluorescence was exhibited at 616 nm. After 1 h incubation of exponential phase cells with increasing HpD concentration an overall intensity enhancement occurred with no change in the distribution of bands, whereas longer incubation time caused an increase in relative intensity of the 636 nm band similar to that observed in plateau phase cells. After 1 h incubation with HpD plateau phase cells were more photosensitive than exponential phase cells, although cell bound HpD was much less in the former case. Incubation of cells for 24 h drastically enhanced the photosensitivity irrespective of the growth phase. Our results suggest a relationship between the fluorescence emission band of HpD at 636 nm and photosensitivity of cells.     

Synthesis and optical properties of fluorene‐based polymers incorporating organosilicon unit

The synthesis and optical properties of polymers bearing the repeating unit of terfluorene and various organosilicon groups were investigated. Polymers with high molecular weight and good solubility could be obtained by Suzuki coupling polymerization from silylene‐containing fluorene‐based dibromo monomers and 9,9‐dihexylfluorene‐2,7‐bis(trimethyleneborate). From UV spectra of polymers bearing acyclic silylene bridge, the organosilicon units not only interrupted a π‐conjugation but also contributed to an electronic communication between connected fluorenes. The emission maximum wavelengths (ca. 400 nm) blue‐shifted when compared with that of polyfluorene (418 nm) and the fluorescence quantum yields were considerably high (>0.82) in the CHCl₃ solution. On the other hand, rather broad emission was observed at 480 nm and the fluorescence quantum yield was quite low (0.004) in the solution‐state PL spectrum of tetraphenylsilole‐containing polymer. The polymer emitted visible green light in the spin‐coated film. The fluorescence peak intensity at 486 nm gradually decreased when the film was illuminated with the UV light of 359 nm in air. © 2007 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem 45: 4786–4794, 2007