INHIBITION OF DNA REPAIR AND PRODUCTION OF SINGLE-STRAND BREAKS IN ESCHERICHIA COLI BY REDUCTONE

Abstract— Reductone (HOCH₂COCHO), a keto-aldehyde produced by thermal degradation of some sugars, at alkaline pHs, blocks the excision repair of DNA lesions in uv-irradiated wild type Escherichia coli. This probably occurs as a result of inhibition of the exonucleolytic activity of DNA polymerase I. In addition, reductone alone induces DNA single-strand breaks. Repair of this damage is mainly dependent on the polA gene products.     

PHOTOTOXICITY FROM BENOXAPROFEN: IN VIVO AND IN VITRO STUDIES

Abstract Benoxaprofen (2-[4-chlorophenyl]-α-methyl-5-benzoxazole acetic acid), a non-steroidal antiinflammatory drug, was found to provoke phototoxicity reactions in humans. Exposure of the skin of benoxaprofen-treated subjects to either solar simulating radiation or a broad UV-A wavelength band produced intense itching and burning sensations, followed by the development of a classical wheal and flare response within 2-4 min. Phototoxicity was related to both the UV radiation fluence and the dose of orally administered benoxaprofen. Wavelengths between 320 and 340nm were active in provoking urticaria. In vitro studies demonstrated that benoxaprofen and UV irradiation produced a dose-dependent lysis of sheep erythrocytes which did not appear to be dependent on the presence of oxygen. Red cells were not lysed by pre-irradiated benoxaprofen arguing against the production of stable lytic photoproducts. Human neutrophils were lysed by benoxaprofen and UV light which resulted in the liberation of both cytoplasmic and lysosomal enzymes. Benoxaprofen failed to induce photolysis of human platelets and photoactivation of complement in human serum. It is suggested that phototoxic urticaria provoked by benoxaprofen may be due to a direct photolytic effect on human dermal mast cells.     

THE EFFECT OF APPLIED THICKNESS ON SUNSCREEN PROTECTION: IN VIVO AND IN VITRO STUDIES

The effect of applied thickness of sunscreen on the degree of protection against ultraviolet exposure has been investigated using an in vitro model (excised human epidermis) and phototesting in human subjects. The agreement between the protection factors obtained by each technique was excellent. It is shown that the influence of applied thickness on sunscreen protection factors is much less than would be predicted by Beer's law.     

PHOTOBINDING OF CHLORPROMAZINE AND ITS SULFOXIDE IN VITRO AND IN VIVO

Abstract— Photosensitivity as observed after chlorpromazine (CPZ) treatment is enhanced in the UVA- rather than the UVB region, whereas CPZ has its absorption maximum at 305 nm. This long wavelength sensitivity has sometimes been ascribed to CPZ-sulfoxide (CPZSO) which has an absorption maximum at 340 nm. We compared the photobinding properties of CPZSO and CPZ under both in vitro and in vivo conditions.
With 310 and 370 nm lamps CPZSO absorbs twice as much light as CPZ but still binds less efficiently to HSA in vitro. At wavelengths longer than 380 nm CPZSO does not absorb nor photobind to HSA (420 nm lamps) in contrast to CPZ.
In vivo the bioavailability of CPZ and CPZSO in ears, eyes and skin of the back of Wistar rats is comparable, yet irradiation with 370 nm light caused more CPZ-photobinding in these tissues. Chlorpromazine binds relatively more compared to CPZSO, to constituents of deeper lying tissues (dermis). This corresponds with the observation that both the ratio of in vitro CPZ photobinding to CPZSO photobinding, and the penetrating ability of light in the skin increase with wavelength.
In the eyes, where the lens efficiently filters out light with wavelengths shorter than 370 nm, no CPZSO photobinding was observed, in contrast to CPZ; this also corresponds with the in vitro experiments. Therefore it seems more likely that the observed wavelength maximum in the photosensitivity action spectrum after CPZ treatment should be attributed to the non-sulfoxidated drug rather than to the sulfoxidated compound.     

SPECTROSCOPIC ANALYSIS OF BACTERIOCHLOROPHYLLS IN VITRO AND IN VIVO*

Abstract— Chromatophores from Rhodopseudonionas spheroides were treated with potassium iridic chloride so as to destroy the major complement of bacteriochlorophyll (BChl) without harming the photochemically active P870. A band at 802 mμ, attributed to a pigment P800, survived this treatment along with P870. Extraction of such chromatophores with a mixture of acetone and methanol removed the absorption bands of P800 and P870; a corresponding amount of BChl was found in the extract. The yield of BChl was too great to have been derived from either P800 or P870 alone; analysis of extinction cofficients and band areas of these pigments indicates that they are both specialized fornis of BChl, in a molecular ratio of 2P800:1P870. Bleaching of P870, without attenuation of the absorption band of P800, could be effected by adding potassium ferricyanide to the iridic chloride-treated chromatophores. Extraction of chromatophores in this condition gave a reduced yield of BChl, consistent with a 2:1 ratio of P800 to P870 under the assumption that the BChl in the extract was derived in this case from P800 alone. An absorption band at 600 mμ in iridic chloride-treated chromatophores, characteristic of BChl and ascribed to P800 and P870, is partly bleached and shifted to shoiter wavelengths upon illumination. This reversible effect, and a similar one near 375 mμ (corresponding to the Soret band maximum of BChl), has the combined attributes of the blue-shift of P800 and the bleaching of P870 seen in a spectrally resolved form near 800 and 865 mμ respectively. The 600 mμ band is bleached by about 30 per cent, again consistent with a ratio of 2P800:1P870. These data, in conjunction with information published elsewhere, support the view that two molecules of P800 and one of P870 are associated jointly with a photosynthetic reaction center. It was observed that the long wave absorption bands of BChl in vivo are sometimes narrower than the narrowest bands that have been observed for BChl in dilute organic solutions. Sharpness of these bands is most conspicuous in some forms absorbing near 800 mμ.     

A COMPARISON OF IN VIVO AND IN VITRO TESTING OF SUNSCREENING FORMULAS

Abstract— Seven commercially available sunscreens were compared by three different methods. Absorbance spectra were measured for each product in isopropanol solution and also on hairless mouse epidermis. In vivo tests were performed on human volunteers using a Xe arc solar simulator. Sun Protection Factors (SPF) were calculated by each method for each product tested and the results compared. By all methods used, the combination of 7% octyl dimethyl para-aminobenzoic acid and 3% oxybenzone provided the most protection from U.V. light. While estimates of the effectiveness of all products were much too high when calculated by the isopropanol solution method, the hairless mouse epidermis technique seems to be an accurate tool for predicting product efficacy in vivo .     

FLUENCE-RATE DEPENDENCE OF MONOPHOTONIC REACTIONS OF NUCLEIC ACIDS IN VITRO AND IN VIVO

The Bunsen-Roscoe law, also known as the reciprocity law ( E = f(F) with F = I t ) has only limited validity for monophotonic reactions of nucleic acids. Especially at low fluence rates, the extent of in vitro and in vivo photoreactions of nucleic acids in the far-UV and near-UV range is a function of the fluence and of the fluence rate ( E = f (F;I)). In vitro experiments with poly(dA)poly(dT) clearly show that the far-UV (254 nm) response, indicated by the changes of the ellipticity at 315 nm, does not obey the Bunsen-Roscoe law at low fluence rates in the range between 1 W m^-2 and 20 W m^-2. In vivo experiments with Escherichia coli revealed very similar anomalies. Studying the growth delay after irradiation with far-UV light at 280 nm or near-UV light at 334 nm, we have confirmed the lack of reciprocity in both spectral ranges. The failure of the Bunsen-Roscoe law for the 280 nm and 334 nm UV irradiation effect at low fluence rates was in the range O < I < 40 W m^-2. In both cases reciprocity occurred at higher fluence rates (40 < I < 100 W m^-2).     

盐酸地尔硫卓药物树脂复合物的制备及其体外释药动力学研究

本文以强酸性阳离子交换树脂为载体，制备了盐酸地尔硫卓(DH)药物树脂复合物。研究了DH与001×7树脂的交换反应动力学以及药物树脂复合物在去离子水、0.5mol/L、1.0mol/L、2.0mol/L NaCl和在0.5mol/L HCl以及0.5mol/L KCl溶液中的释药动力学。结果表明，在制备药物树脂的过程中，随温度的升高，药物与树脂的交换速率增加，及有利于反应的进行；药物树脂复合物在去离子水中不释放药物，但其释放随释放介质浓度的增加而增加，并且属于粒扩散的离子交换控制，粒扩散系数Dr随离子强度的增加而增加，DH的释药动力学过程符合对数方程（Visuanathan方程），001×7树脂可有效地控制DH在体外的释放。     

PRODUCTION OF BREAKS IN SINGLE- AND DOUBLE-STRANDED FORMS OF BACTERIOPHAGE øx174 DNA BY PROFLAVINE AND LIGHT TREATMENT

Abstract— Irradiation at 440 + 360 nm and a fluence rate of 3.8 kJm^-2 min^-1, of both complexes previously formed between proflavine and either øX circular single-stranded (ss) DNA or øX supercoiled duplex (RFI)DNA, induces single-strand scissions in the two DNAs under consideration. Linear øXSS DNA molecules are detected by sedimentation through alkaline sucrose gradients. After treatment of the øXRFI DNA, however, the degree of degradation is the same whether it is measured under neutral or alkaline conditions, indicating that alkaline-labile bonds are not created; moreover, double-strand breaks can only be detected after accumulation of single-strand breaks. In addition to the amount of proflavine bound to the DNA and the duration of irradiation, the following factors are shown to influence the nicking activity of the treatment: (1) the DNA structure (the øXRFI DNA is much more sensitive than the øXss DNA); (2) the ionic strength of the medium during irradiation (a high value of 0.5 leads to a markedly increased efficiency); (3) the addition of cysteamine (this latter compound decreases the reaction rate) and (4) the irradiation wavelength (after irradiation at 440 nm alone, the reaction occurs at a reduced rate and is sensitive to NaN₃). The kinetics of the nicking reaction does not follow a single-hit curve showing that at least one primary lesion occurs prior to strand breakage. On the other hand, strand scission cannot be detected after irradiation of the proflavine-DNA complexes at the low fluence rate causing a decrease in the infectivity of both øXSS and øXRFI DNAs. Similarly. the sedimentation pattern of the DNA extracted from treated øx174 phages 99.9% inactivated, is identical to that of the control ss DNA, although more drastic treatments are susceptible to induce single strand breaks inside the phage head. Finally, the unknown lesion (s) that is biologically important does not prevent the treated DNAs from penetrating into the hostcells.     

IN VITRO AND IN VIVO PROTECTION AGAINST PHOTOTOXIC SIDE EFFECTS OF PHOTODYNAMIC THERAPY BY RADIOPROTECTIVE AGENTSWR–2721 ANDWR–77913

Abstract— The experimental radioprotective agentsS–2-(3-aminopropylamino) ethyl phosphorothioate(WR–2721) and 3-amino-2-hydroxypropyl phosphorothioate(WR–77913) are also protective against photosensitized oxidation. They reduce porphyrin-induced photopolymerization of lens cytosol proteins in vitro, and phototoxic damage to mouse skin in vivo. The phototoxic dose modification factor (DMF) was 1.5 which is similar to that found in ionizing radiation. Part of the mechanism by which sulfhydryls afford this protection is by accelerating photobleaching of the porphyrins.     

用DSC研究阻燃PET的结晶性和结晶动力学

<正> 聚对苯二甲酸乙二酯(PET)是一种熔点较高的结晶性聚合物,其结晶性和结晶动力学已得到了广泛的研究。我们最近合成的一种含磷聚合物(或齐聚物)聚苯基磷酸二苯砜酯(PSPPP),可作为PET纺丝较为理想的阻燃剂。当PET中添加5wt％的这种阻燃剂时,其极限氧指数可达到30。然而,有关这种阻燃剂的加入对PET结晶特性的影响方面的研究鲜见报道。本文用DSC方法研究了阻燃剂添加量的多少对PET结晶程度的影响,并且对纺制阻燃PET纤维的实用添加量5wt％的试样进行了结晶动力学研究。     

OPTICAL PROPERTIES OF PHYTOCHROME IN THE BLUE- SPECTRAL REGION AS MEASURED IN VIVO AND IN VITRO

In the blue spectral region, the phototransformation difference spectrum of oat phytochrome extracted as P_fr differs from that of phytochrome extracted as P_r. The difference absorbance maximum for phytochrome extracted as P_fr is at 420 nm, while that extracted as P_r is at 412 nm. The phototransformation difference spectrum measured in the blue in oat coleoptile tips without inner leaves, corresponds very well with that of phytochrome as extracted in its P_fr form. There is, however, a slight apparent attenuation of the blue difference band relative to those in the red-far-red. In coleoptile tissue containing inner leaves, the blue difference band is relatively even more highly attenuated. A similar attenuation is observed in the blue, in the protochlorophyllide to chlorophyllide phototransformation difference spectrum. In the spectrum measured with excised coleoptile without inner leaves, there is a small attenuation, while in coleptile tissue with inner leaves the attentuation is nearly 9-fold. These data suggest that the observed attenuation is probably artifactual. Neither instrumental non-linearity nor fluorescence induced by the measuring beam could explain the observed attenuation. It is suggested that the observed attenuation is probably mainly the result of wavelength dependent scatter amplification, the amplification in the blue being attenuated by the high background absorption of other pigments in this region.     

IN VITRO STUDIES ON THE PHOTOSENSITIZED OXIDATION OF LENS PROTEINS BY PORPHYRINS

Abstract Porphyrins, which may be introduced into the eye as a result of abnormal porphyrin metabolism (uroporphyrin–Uro) or when used in the diagnosis or photodynamic therapy of certain tumors, including intraocular tumors (hematoporphyrin–Hp and'hematoporphyrin derivative'–Hpd and mesotetra( P -sulfonatophenyl)porphyrin–TPPS) are efficient photosensitizers in biological systems. We have been studying the potential phototoxic side effects of these drugs in the lens of the eye. Encapsulated in the human lens is a mixture of soluble protein crystallins. With little turnover of protein in the lens, any photosensitized modifications will accumulate and may result in an opacification of the lens. To evaluate the potential of different porphyrins to induce such damage, a series of porphyrins were photolyzed (transmission above 295 nm) in the presence of calf lens protein (2 mg m⁻¹). Marked photopolymerization and histidine destruction were observed for the lens protein photolyzed in the presence of all of the drugs. We have found that the relative effectiveness of the following porphyrins to induce that damage is: Uro = TPPS Hpd = Hp. Both the singlet oxygen quencher, azide, and the free radical scavenger, penicillamine, decrease this photosensitized oxidative damage to lens protein. TPPS binds significantly to lens protein and this binding leads to conformational changes in that protein.     

ANALYTICAL MODELING FOR THE OPTICAL PROPERTIES OF THE SKIN WITH IN VITRO AND IN VIVO APPLICATIONS

Abstract— Analytical modeling that interrelates the optical properties of multilayered structures is applied to the skin. The mathematical approach is based on relations of diffuse reflectance and transmittance of a multilayered system and the diffuse reflectance and transmittance of each component layer. The formula can also be derived from the Kubelka–Munk theory of radiation transfer. Using both collimated and diffuse incident irradiance, the applicability of the model to human epidermis over the UV and visible region has been verified. The model has been applied to calculate the absorption and scattering coefficients of human epidermis in vitro , and to estimate the epidermal transmittance under simulated in vivo condition.     

PHOTOCONVERSION OF PHYTOCHROME IN VIVO STUDIED BY DOUBLE FLASH IRRADIATION IN Mougeotia AND Avena

Abstract— The kinetics of phytochrome phototransformation from the red-absorbing form (P_r) to the far-red-absorbing form (P_fr) in vivo at 22°C were studied using a double flash apparatus with 1-ms flashes. Photoconversion by simultaneous flashes of red light saturates at a low P_fr level, indicating the possible attainment of a photoequilibrium between the excitation of P_r and the photoreversion of intermediates in the course of the I-ms flashes. At saturation energy, simultaneous flashes resulted in about 50% as much P_fr as was produced by saturating irradiation with 5 s red light. Intermediates of the phototransformation pathway were analysed by separating two red or a red and a far-red flash by variable dark intervals. In both plants phototransformation intermediates with half-lives < 1 ms occur, but they are too short-lived to characterize by our method. The subsequent intermediates have half-lives of about 7 ms and 150 ms in A vena , 2 ms and 10 ms in Mougeotia. The conversion from P_r to P_fr seems to be completed 1 s after the red flash in Avena. In the alga Mougeotia , P_fr formation seems to be finished within only 50 ms after the inducing red flash. The kinetics obtained from physiological and spectrophotometric experiments with Avena mesocotyls are almost identical. These observations indicate that the physiological response corresponds directly to the amount of P_fr produced and not to phototransformation intermediates or "cycling" between P_r and P_fr.     

FLUORESCENCE AND LUMINESCENCE STUDIES OF IN VIVO CHLOROPHYLL WITH A LASER PHOSPHOROSCOPE*

Abstract— A simple apparatus using a He-Ne laser and a rotating sector gives repetitive light pulses with rise and fall times of a few μsec and intensities of up to 0.65 W/cm². Fluorescence during the actinic pulse and luminescence following it (after 20 μsec) may be recorded and compared. Sampling of the suspension of photosynthetic cells or chloroplasts by intermittent flow permits the averaging of 25 such measurements. With Chlorella, the fast (30 μsec) and the medium (30 msec) components of luminescence do not saturate at the same light intensity. The former saturates in the same range as the photochemical fluorescence rise, whereas the latter saturates at higher intensities. Under a variety of conditions, the decay of luminescence intensity is always strongly polyphasic. Analysis of the kinetics discloses a dependency with the log concentration of the hypothetical precursor, suggesting a connection of luminescence with electrochemical phenomena. The shape of the luminescence integral, as well as the light saturation pattern, suggests another kind of interpretation, in terms of several pools, possibly two of equal size. In the presence of hydroxylamine, only one pool is seen. The stimulating effect of preillumination is only observed for the medium component. However, a stimulation of short duration also exists for the fast component. The problems of number of pools, mechanism, and stimulation are briefly discussed.     

表面活性剂改性的铝交联粘土的表征及其水蒸汽减活动力学研究

以聚乙烯醇（ＰＶＡ）为支撑前体合成出改性的铝交联蒙脱土与铝交联累托土。采用ＸＲＤ、Ｎ２低温吸附脱附法、ＩＲ等手段对它们进行了表征，并研究了它们在不同时间与温度条件下的水蒸汽减活动力学。研究结果表明，ＰＶＡ的改性有助于铝交联粘土层间距与比表面积的增大及热稳定性与水热稳定性的提高，粘土基质对其热稳定性与水热稳定性有显著影响，该类催化材料的水蒸汽减活动力学遵循一级衰减反应方程式，其减活速率常数与温度的函数关系可用一个指数函数的经验式表示。     

KINETICS AND MECHANISM OF CATALYSIS BY FERRIHAEMS IN THE CHEMILUMINOGENIC OXIDATION OF LUMINOL BY HYDROGEN PEROXIDE

The kinetics of catalysis by deuteroferrihaem (deuterohaemin) were studied in the chemiluminogenic oxidation of luminol by hydrogen peroxide. The results imply that two distinct catalytic mechanisms operate to yield chemiluminescence from excited aminophthalate emitter in this system. The first mechanism involves initial one-electron oxidation of luminol by an oxidised derivative of deuteroferrihaem with well-established peroxidatic oxidant properties. The second mechanism involves a concerted pathway very similar to that which has been proposed [Olsson, T., L. Ewetz and A. Thore (1983), Photochem. Photobiol. 38 , 223–229] to explain protoferrihaem (haemin) catalysis in luminol oxidation. Deuteroferrihaem is a much more effective catalyst than protoferrihaem on a mole-for-mole basis and could be used with advantage in chemiluminescence analyses.