卤化银感光乳剂的光致电子顺磁共振信号强度与成熟时间的关系

本文发现含染料的溴化银模型乳剂在g=2.0023下的光致ESR信号强度随化学成熟时间的增长而增强,与光敏度的变化呈平行关系。这一现象与文献中报道的^[1]在实用乳剂上得出的结果恰恰相反。假设化学敏化产物在潜影形成过程中既能作为电子陷阱,又能作为空穴陷阱,可以解释这种差异。     

WAVELENGTH DEPENDENCE OF DNA INCISION BY A HUMAN ULTRAVIOLET ENDONUCLEASE

The wavelength dependence of an ultraviolet irradiation of the DNA substrate for a human endonuclease was determined. Sites of DNA incision for all UVB and UVC wavelengths examined were at cytosines which were neither cyclobutane pyrimidine dimers nor 6-4'-(pyrimidin-2-one)pyrimidines. The optimal wavelengths for formation of these cytosine photoproducts were between 270 and 295 nm. This human endonuclease therefore has a similar ultraviolet substrate specificity to endonuclease III.     

荧光素在明胶片中的光吸收及稳定性

由于对非线性光学材料的需求,近年来已有很多工作对荧光素的光学及光化学性质进行研究,研究对象既有溶液也有聚合物薄膜。本工作使用明胶片研究荧光素在明胶片中的光吸收、荧光及光稳定性。     

PHOTOBLEACHING OF A CYANINE DYE IN SOLUTION AND IN MEMBRANES

Abstract— N,N'-bis(2-ethyl-1,3-dioxolane)-kryptocyanine (EDKC), a lipophilic dye with a delocalized positive charge, photosensitizes cells to visible irradiation. In phosphate-buffered saline (PBS), EDKC absorbs maximally at 700 nm (ε= 1.2 × 10⁵ M⁻¹ cm⁻¹) and in methanol, the absorption maximum is at 706 nm (ε= 2.3 × 10⁵ M⁻¹ cm⁻¹). EDKC partitions from PBS into small unilamellar liposomes prepared from saturated phospholipids and into membranes prepared from red blood cells (RBC) and binds to human serum albumin (HSA). The EDKC fluorescence maximum red shifts from 713 nm in PBS to 720–725 nm in liposomes and RBC membranes and the fluorescence intensity is enhanced by factors of 14–35 compared to PBS (φ= 0.0046). EDKC is thermally unstable in PBS (T_1/2= 2 h at 1.3 × 10⁻⁵ M EDKC), but stable in methanol. In liposomes and RBC membranes, EDKC is 10 times more stable than in PBS, indicating that it is only partially exposed to the aqueous phase. Quenching of EDKC fluorescence in liposomes and RBC membranes by trinitrobenzene sulfonate also indicates that EDKC is not buried within the membranes. Photodecomposition of EDKC was oxygen-dependent and occurred with a low quantum yield (6.4 × 10⁻⁴ in PBS). Singlet oxygen was not detected upon irradiation of EDKC in membranes or with HSA since the self-sensitized oxidation of EDKC occurred at the same rate in D₂O as in H₂O and was not quenched by sodium azide or histidine.     

QUENCHING AND PHOTOBLEACHING OF EXCITED POLYCYCLIC AROMATIC HYDROCARBONS BY CARBON TETRACHLORIDE AND CHLOROFORM IN MICELLAR SYSTEMS

—Aromatic hydrocarbons incorporated into cetyltrimethylammonium chloride (CTACl) or sodium dodecylsulphate (SDS) micelles are efficiently quenched and photobleached by carbon tetrachloride. Similar results were obtained employing chloroform, but the efficiency of this compound as a quencher is nearly 10³ times smaller than that of carbon tetrachloride.
Bimolecular quenching constants, with the quencher concentration given in moles per liter of micellar pseudophase, have been evaluated and compared with those obtained in homogeneous solutions. For slow processes, the values obtained would indicate that the polarity sensed by the probe depends both upon the probe and the surfactant. For diffusionally controlled processes (i.e. quenching of biphenyl), bimolecular quenching constants are considerably smaller in the micellar pseudophase. For these processes the pseudo-first-order quenching rate constants are larger in SDS than in CTACl micelles. This effect is partly due to the smaller size of the SDS micelle but also is a consequence of a lower "microviscosity" of these micelles.     

THE WAVELENGTH DEPENDENCE OF HERPES SIMPLEX VIRUS INACTIVATION BY ULTRAVIOLET RADIATION

The effect of different wavelengths of ultraviolet (UV) radiation on Herpes simplex virus when assayed on mammalian cells (measured by plaque forming ability) was investigated. The wavelength dependence of viral inactivation was obtained for 11 different wavelengths over the region 238–297 nm. The resulting action spectrum does not closely follow the absorption spectrum of either nucleic acid or protein. The most effective wavelengths for viral inactivation are over the region 260–280 nm.     

HOMOGENEOUS PHOTOBLEACHING OF CHLOROPHYLL HOLOCHROMES IN A PHOTOSYSTEM I REACTION CENTER COMPLEX

Chlorophyll (Chl) photobleaching and P700 photodegradation were followed simultaneously in a P700 Chi a-protein complex (Chl a /P700 < 35). During strong illumination, the photobleaching kinetics of the bulk Chl corresponded with that of P700 photodegradation. The absence of a blue shift of the absorption maximum at 678 nm after photobleaching indicated the simultaneous degradation of all Chl holochromes and the absence of long wavelength-absorbing energy traps that would protect P700 against excess light energy. It was deduced that in the P700 reaction center core complex, the excitons are uniformly distributed amongst the Chl holochromes, which decreases the deleterious effects of excess light energy on P700 and protects the photosystem against photoinhibition.     

FREE ENERGY DEPENDENCE OF THE QUENCHING OF CHLOROPHYLL a FLUORESCENCE BY SUBSTITUTED QUINONES*

The quenching of chlorophyll a (Chl a) fluorescence hy a series of substituted benzoquinones. naphthoquinones and anthraquinones has been examined employing ethanol and acetonitrile as solvents. All quinones are good quenchers of fluorescence. There is an excellent linear relation between the Stern-Volmer quenching constants, K, and the polarographic half wave potentials (E₁₂) of the quinones, with more oxidizing quinones being better quenchers. The quenching data are consistent with the excited state half wave potential of ?1.31 eV predicted theoretically, demonstrating that the kinetically estimated value of the Chl a excited state reduction potential agrees with that expected on spectroscopic grounds. The results of quenching are not in agreement with the conventional Marcus theory of electron-transfer reactions, as there is no evidence of quenching constant. K_q. decrease vsΔG⁰ even for free energy changes nearly twice that expected for the onset of the Marcus inverted region. However, the kinetically estimated K_q values are in good agreement with the ones calculated by using the Rehm and Weller equation for fluorescence quenching by electron transfer. Our experimental results support the electron transfer mechanism of quenching proposed by Seely.     

TEMPERATURE AND VISCOSITY DEPENDENCE OF FLUORESCENCE QUENCHING BY OXYGEN IN MODEL SYSTEMS

Abstract— The bimolecular rate constant, k _q, for the quenching of the fluorescence of pyrenebutyric acid and naphthaleneacetic acid by molecular oxygen has been studied as a function of temperature and viscosity, η. Fluorescence lifetime measurements were used to monitor the degree of quenching. Glycerol-water and sucrose-water mixtures were used to increase the bulk viscosity. Plots of log k _q vs log η show deviations from Stokes-Einstein behavior, but the data are consistent with the patterns that have been observed for other diffusion limited reactions. This work provides background information, regarding the viscosity dependence of oxygen quenching reactions, which is essential for the correct interpretation of oxygen quenching/viscosity dependence studies with more complex systems (i.e. quenching of tryptophan residues in proteins).     

A LOW INTENSITY PERMANENT LIQUID LIGHT STANDARD ACTIVATED BY RADIOACTIVITY

Abstract— The total radiant flux from a solution containing a radioactive compound, hexadecme-l-¹⁴C, plus an appropriate scintillator, has been determined. The procedure used involves comparison of its luminescent emission with the light scattered by glycogen illuminated with a monochromatic homogeneous light beam of known photon flux. These standards are particularly convenient for use with chemiluminescent and bioluminescent reactions, since the geometry of the emission may be duplicated exactly.     

TEMPERATURE DEPENDENCE OF INDUCTION OF CYCLOBUTANE-TYPE PYRIMIDINE PHOTODIMERS IN HUMAN FIBROBLASTS BY 313 nm LIGHT

The rate of cyclobutane-type pyrimidine photodimerization with 313 nm light was determined in confluent cultures of xeroderma pigmentosum cells of group A. A new method was developed for the determination of sodium borohydride reduced thymine-thymine (TT) and cytosine-thymine (CT) dirners by high pressure liquid chromatography. It was found that the yield of dimerization andtheratioof CT/TT depended on the irradiation temperature in the physiological fluence range of 2.25 to 15 kJ m⁻². Both were significantly higher at 37 than at 0°C.     

WAVELENGTH DEPENDENCE FOR THE INDUCTION OF BACTERIOPHAGE LAMBDA BY ANTITUMOR AGENT GILVOCARCIN V

The wavelength dependence for the induction of a lambda- lacZ fusion phage of E. coli by photo-activated gilvocarcin V was determined using a spot test or a quantitative assay for the lacZ gene product. Suspensions of bacteria and chemical were exposed to radiation of different wavelengths in the region 313-546 nm, using a double grating monochromator. The prophage induction profiles generated were similar to the absorption spectrum of gilvocarcin V in this region, with a peak near 400 nm. The radiation fluence and chemical concentration required for threshold levels of prophage induction exhibited a nearly reciprocal relationship. These results have implications for the therapeutic use of gilvocarcins as antitumor agents.     

光学解偏振法测定高聚物的结晶速度

制成了光学解偏振法测定高聚物结晶过程的仪器,测试了聚丙烯、尼龙6等几种试样。本方法的优点是:样品用量少,测试温度范围宽,可以测定较快的结晶过程。由于设计了透射光强度自动控制电路,实验结果可靠,重复性好,并能自动记录。     

ELEMENTAL SELENIUM GENERATED BY THE PHOTOBLEACHING OF SELENOMEROCYANINE PHOTOSENSITIZERS FORMS CONJUGATES WITH SERUM MACROMOLECULES THAT ARE TOXIC TO TUMOR CELLS

Elemental selenium generated by the photobleaching of selenomerocyanine dyes forms conjugates with serum albumin and serum lipoproteins that are toxic to leukemia and selected solid tumor cells but well tolerated by normal CD34-positive hematopoietic stem and progenitor cells. Serum albumin and lipoproteins act as Trojan horses that deliver the cytotoxic entity (elemental selenium) to tumor cells as part of a physiological process. They exploit the fact that many tumors have an increased demand for albumin and/or low-density lipoprotein. Se(0)-protein conjugates are more toxic than selenium dioxide, sodium selenite, selenomethionine, or selenocystine. They are only minimally affected by drug resistance mechanism, and they potentiate the cytotoxic effect of ionizing radiation and several standard chemotherapeutic agents. The cytotoxic mechanism of Se(0)-protein conjugates is not yet fully understood. Currently available data are consistent with the notion that Se(0)-protein conjugates act as air oxidation catalysts that cause a rapid depletion of intracellular glutathione and induce apoptosis. Drugs modeled after our Se(0)-protein conjugates may prove useful for the local and/or systemic therapy of cancer.     

PHOTOLYSIS OF PHOSPHODIESTER BONDS IN PLASMID DNA BY HIGH INTENSITY UV LASER IRRADIATION

Abstract— The cleavage of phosphodiester bonds in DNA exposed to high intensity UV laser pulses in aerated aqueous solution has been investigated using a krypton fluoride excimer laser (248 nm) and bacterial plasmid DNA. The dependence of strand breakage on fluence and intensity has been studied in detail and shows that the process is non-linear with respect to intensity. The relationship between the quantum yield for strand breakage and intensity shows that the strand breakage reaction involves two-photon excitation of DNA bases. The quantum yield rises with intensity from a lower value of 7 times 10^-5 until a maximum value of 4.5 times 10^-4 is attained at intensities of 10¹¹ W m^-2 and above. This value is approximately fifty-fold higher than the quantum yield for strand breakage induced by exposure to low density UV irradiation (254 nm, 12 W m^-2). DNA sequencing experiments have shown that strand breakage occurs by the specific cleavage of the phosphodiester bond which lies immediately 3' to guanine residues in the DNA, leaving some alkali-labile remnant attached to the terminal phosphate. A mechanism for DNA strand breakage which involves the generation of guanine radical cations is proposed.     

PHOTOBLEACHING OF PORPHYRINS USED IN PHOTODYNAMIC THERAPY AND IMPLICATIONS FOR THERAPY

Abstract— The development of an extraction procedure to quantitate dihematoporphyrin ether (DHE) concentration in tissues correlated to fluorescence measurements from instrumentation developed for in vivo fluorimetry was examined. In vivo fluorometric results from mouse mammary carcinoma (SMT-F) were calibrated against results of the chemical extraction assay quantitated spectrophotometrically. Fluorescence and drug extractable levels increase in a linear fashion with injected dose. Loss of porphyrin fluorescence (photobleaching) and intra-tumoral porphyrin level has been demonstrated both in vitro (NHIK cells) and in vivo (SMT-F tumor) during illumination with light following exposure to Hpd or DHE. This process is essentially independent of porphyrin tumor level in vivo and could lead to tumor protection at very low porphyrin levels. On the other hand, this photobleaching process which occurs concurrent with cellular inactivation and tissue damage due to the photodynamic process can be exploited to protect normal tissue during photodynamic therapy (PDT) and thus greatly enhance the therapeutic ratio. This has been demonstrated in patients undergoing PDT.     

EFFECTS OF INTENSITY AND FLUENCE UPON DNA SINGLE-STRAND BREAKS INDUCED BY EXCIMER LASER RADIATION

Abstract— A Xenon-chloride excimer laser emitting energy at 308 nm was used to induce single-strand breaks (SSBs, frank breaks plus alkali-labile lesions as assayed by alkaline sucrose sedimentation techniques) in purified DNA from Bacillus subtilis . A fluence response study and a peak pulse intensity study were performed. At a pulse energy of 0.1 mJ/pulse, the radiation induced SSBs in a linear fashion (91 SSB/10⁸ Da per MJ/m²) to a maximum exprimental fluence of 1.28 MJ/m². The pulse intensity study showed that there were no significant changes in DNA breakage (105 SSB/10⁸ Da) between 2.93 times 10⁹ and 5.86 times 10¹¹ W/m² (0.11 and 22.0 mJ/pulse) at a constant total fluence of 1.1 MJ/m² (27000 mJ dose). This study has verified and extended previous work by quantifying the yield of SSBs induced in DNA by this laser radiation.     

MECHANISM OF PHOTOREDUCTION OF THIAZINE DYES BY EDTA STUDIED BY FLASH PHOTOLYSIS-II. pH DEPENDENCE OF ELECTRON ABSTRACTION RATE CONSTANT OF THE DYES IN THEIR TRIPLET STATE

Abstract— The pH dependence of the apparent reactivity of thiazine dyes in their triplet states has been studied in aqueous solutions, using as electron donor HY^-3, the trianionic species of ethylene diamine tetraacetic acid (EDTA), in the pH range 4–8. The pH dependence is found to be related to a change in the degree of protonation of the triplet excited dye. The apparent reactivity and lifetime of two differently protonated forms of thionine, azur B and methylene blue were determined by classical and dye-laser flash techniques, making it possible to evaluate the rate constant for electron abstraction of these molecules in their triplet states. It is found that: (a) protonation on the ring nitrogen increases the electron-abstraction rate constant of the triplet-state species about twenty-fold, and (b) methylation on the side amino groups decreases it.     

聚羧基脂肪酸酯细菌合成的生长环境依赖性

聚羟基脂肪酸酯（Ｐｏｌｙｈｙｄｒｏｘｙａｌｋａｎｏａｔｅ,ＰＨＡ）是一类由许多细菌合成的、结构多变的能量和碳源的储藏物质,为了得到能合成新型ＰＨＡ的菌种,或得到能在便宜简单碳源上合成ＰＨＡ的菌种,以我们实验室开发的傅立叶红外（ＦＴ－ＩＲ）细胞无损检测技术和常规气相色谱（ＧＣ）法对全国各地的采集的不同样品中分离的菌种进行了筛选,往往在不同的地理环境中,筛选出的菌株所合成的ＰＨＡ的单体组成不同,有以含四个或五个碳原子的短链单体ＰＨＡ（Ｓｈｏｒｔ－ｃｈａｉｎ－ｌｅｎｇｔｈＰＨＡ,ｓｃｌＰＨＡ）为主,有的以含六个到十六个碳原子的中长链单体ＰＨＡ（Ｍｅｄｉｕｍ－ｃｈａｉｎ－ｌｅｎｇｔｈＰＨＡ,ｍｃｌ ＰＨＡ）为主,在我们以六种底物为碳源培养的３７１株形态不一的菌株中,有４０％的菌可以合成ＰＨＡ,而其中许多可以同时合成ＰＨ     

聚羟基脂肪酸酯细菌合成的生长环境依赖性

聚羟基脂肪酸酯 (Polyhydroxyalkanoate,PHA)是一类由许多细菌合成的、结构多变的能量和碳源的储藏物质 .为了得到能合成新型PHA的菌种 ,或得到能在便宜简单碳源上合成PHA的菌种 ,以我们实验室开发的傅立叶红外 (FT IR)细胞无损检测技术和常规气相色谱 (GC)法对全国各地的采集的不同样品中分离的菌种进行了筛选 .往往在不同的地理环境中 ,筛选出的菌株所合成的PHA的单体组成不同 ,有的以含四个或五个碳原子的短链单体PHA(Short chain lengthPHA ,sclPHA)为主 ,有的以含六个到十六个碳原子的中长链单体PHA(Medium chain lengthPHA ,mclPHA)为主 .在我们以六种底物为碳源培养的 371株形态不一的菌株中 ,有 40 %的菌可以合成PHA ,而其中许多可以同时合成PHB与中长链PHA共混的聚合物 .本研究为进行PHA研究的高分子同行提供了寻找能合成PHA的微生物菌种的依据