SENSITIVITY OF MONONUCLEAR CELLS TO UV RADIATION

Abstract—The viability of peripheral blood mononuclear cells, as measured by trypan blue dye exclusion, is decreased by exposure to UV radiation in vitro . The toxicity of the UV radiation is doseand wavelength-dependent; UVC is approximately 10 times more effective than UVB and 10⁵ times more effective than UVA.     

EFFECT OF UV RADIATION ON SURVIVAL OF NON-HAIRED MICE

Abstract— Patterns of mortality in a series of photocarcinogenesis experiments were examined. All experiments involved chronic irradiation of genetically non-haired mice with simulated sunlight from a Xe lamp. Experimental variables included genetic origin of the test animals, incident dose of radiation, and the spectral quality of the radiation. In 16 experiments involving 10 genetic origins of mice the following patterns were detected: (1) survival was inversely proportional to the delivered radiation dose; (2) within origins the life-shortening efficacy of radiation was closely correlated with its carcinogenic efficacy; (3) between genetic origins the carcinogenicity and lethality of a radiation dose were qualitatively correlated, but relative efficacy for the two effects varied; (4) altering the source spectrum by modifying the short-wave (UVB) cutoff produced similar changes in carcinogenicity and lethality, suggesting that UVB was a significant contributor to lethal efficacy; (5) nature and relative timing of the carcinogenic response were such that carcinogenesis was not likely to have caused the observed mortality. It is speculated that systemic effects, possibly immunologic or toxic, are produced by chronic UV irradiation, and that these apparently cumulative, dose-dependent effects result in premature death of non-haired mice.     

RESISTANCE OF HUMAN and MOUSE MYELOID LEUKEMIA CELLS TO UV RADIATION

Sensitivity of mouse bone marrow and myeloid leukemia cells as well as the sensitivity of human myeloid leukemia cells to UV light was tested. Criteria were the in vivo colony-forming ability of UV exposed cells and the inhibition of DNA synthesis during post-irradiation incubation for 24 h in vitro. Mouse bone marrow cells irradiated with a small dose of UV light (5 J/m2) and injected into x-irradiated animals did not form hemopoietic colonies on the recipients' spleens, and the recipients died. However, mouse leukemia cells, after irradiation with higher doses of UV light, retained the ability to form colonies on the spleens, and all recipient mice died with typical symptoms of leukemia. In vitro, mouse bone marrow cells exhibited high sensitivity to UV light as compared to mouse myeloid leukemia cells. Human leukemia cells were also resistant to UV light, but more sensitive than mouse leukemia cells. These results indicate that myeloid leukemia cells are resistant to UV light as compared with normal bone marrow cells.     

THE EFFECT OF CHANGES IN CELL GEOMETRY ON THE SENSITIVITY TO ULTRAVIOLET RADIATION OF MAMMALIAN CELLULAR CAPACITY

Abstract— We have measured a calcium and magnesium dependent change in cell shape when mammalian cell monolayers are being prepared for irradiation by replacing their growth medium with certain buffers. In some cases, flattened cells (umbonate) assumed a spherical configuration. In order to assume a centrally located target molecule, we used a DNA-dependent cellular function–pacity for herpes viral growth–as the parameter to measure ultraviolet (UV) sensitivity of cells irradiated while in either of the two shapes. Umbonate cells were more sensitive to UV than were spherical cells. Exposures to the cell that lowered the cellular capacity of umbonate cells to the 10% survival level only lowered spherical cells to the 50% level. Twenty-seven per cent additional UV exposure to spherical cells was required to get the same effect as with umbonate cells. Included in the text are photographs of both cell types, survival curves for cellular capacity, a measure of the absorbance of cell homogenates, and a calculation of the relative number of photons absorbed by each cell nucleus.     

EFFECT OF PSORALEN AND NEAR UV ON VERTEBRATE CELLS IN CULTURE: COMPARISON OF LASER WITH STANDARD LAMP

Abstract. 4'-Aminoethyl-4,5',8-trimethylpsoralen, a DNA photoreagent, was used in conjunction with near UV light to modify cell growth and morphology. Since near UV radiation is needed to trigger the photoreactions, various doses of classical and laser near UV light were exposed to cells growing in media containing psoralen. It was found that near UV light caused a reduction in cell viability as indicated by complete inhibition of growth. The specificity of psoralens for nucleic acids was also investigated by using a tritium labeled psoralen derivative and tracing its appearance in different fractions of DNA from treated and untreated cells.     

PHOTOMIMETIC EFFECT OF SEROTONIN ON YEAST CELLS IRRADIATED BY FAR-UV RADIATION

Abstract— The effect of serotonin on the survival of far-UV irradiated cells of the yeast Candida guillier-mondii was studied. Serotonin was found to have a photomimetic property. Preincubation of cells with serotonin results in protection against far-UV inactivation, whereas the post-radiation treatment with serotonin causes a potentiation of far-UV lethality. Both effects are similar to those produced by near-UV (334 nm) radiation. The observations provide support to the idea advanced by us previously that photosynthesized serotonin is the underlying cause of the two effects of near-UV radiation, photo-protection and potentiation of far-UV lethality. Experiments with an excision-deficient strain of the yeast Saccharomyces cerevisiae suggest that the effect of serotonin is by its binding to DNA.     

EFFECT OF GROWTH TEMPERATURE ON LIPID COMPOSITION and ULTRAVIOLET SENSITIVITY OF HUMAN CELLS

Human skin fibroblasts were incubated at either 25 or 37 degrees C before UV irradiation. Cells incubated at 25 degrees C were more resistant to near UV radiation than cells grown at 37 degrees C, but cells grown at the lower temperature were more sensitive to 254 nm radiation. Fatty acid analysis of membranes of cells showed that cells incubated at the lower temperature contained significantly higher amounts of linoleic acid (18:2) and linolenic acid (18:3) than cells incubated at 37 degrees C. To determine if this difference in fatty acid content of the membranes was responsible for the UV survival characteristics of cells incubated at different temperatures, cells were enriched with either linoleate or linolenate during a 37 degrees C incubation period. Gas chromatography revealed that cells incorporated the supplied fatty acid. Fatty acid enriched cells were then irradiated with near UV, and survival characteristics were compared to those obtained with cells grown at the lower incubation temperature. The results suggest that the different proportion of fatty acid content of the cells is not the cause of different UV sensitivities of cells grown at 25 degrees C compared to cells grown at 37 degrees C.     

EFFECTS OF UV, SUNLIGHT AND X-RAY RADIATION ON QUIESCENT HUMAN CELLS IN CULTURE

Nondividing human diploid fibroblasts (HDF) in culture have been used to study the effect on cell lethality of ultraviolet light, natural sunlight and X-rays. A lethal effect is defined as cellular degeneration, loss from the culture and inability to exclude vital strains. Far-and mid-UV have a readily observable lethal effect (cell loss), with DNA and DNA damage as the critical target and critical damage respectively. In part, natural sunlight kills cells by a similar mechanism but has an additional lethal effect at longer exposure times. This additional effect is expressed by the retention of the dead cells in culture, in contrast to the UV-induced promotion of cell degeneration and loss. Relatively large doses of X-rays that destroy proliferative capacity, have no detectable lethal effect on the maintenance of nondividing cells. The biological response of nondividing HDF to radiations from different parts of the electromagnetic spectrum is dissimilar.     

THE EFFECT OF ALA AND RADIATION ON PORPHYRIN/HEME BIOSYNTHESIS IN ENDOTHELIAL CELLS

To study porphyrin biosynthesis in human microvascular endothelial cells, HMEC-1 cells, a transformed human microvascular endothelial cell line, were incubated with 5-aminolevulinic acid (ALA), the precursor of endogenous porphyrins, and porphyrin accumulation was measured spectro-fluorometrically. The HMEC-1 cells accumulated porphyrin in a concentration-related and a time-dependent fashion. Protoporphyrin was the predominant porphyrin accumulated in the cells. The effect of light on protoporphyrin accumulation was evaluated by exposing the ALA-loaded HMEC-1 cells to ultraviolet-A (UVA) and blue light, followed by another incubation with ALA for 2–24 h. Enhancement of protoporphyrin accumulation in irradiated HMEC-1 cells was observed 2–24 h after irradiation, which was associated with a decrease in ferrochelatase protein and activity. Porphyrin accumulation from ALA after irradiation was significantly decreased when catalase (750–3000 U/mL, 29.3–44.3% suppression) or superoxide dismutase (270 U/mL, 36.4% suppression) was present during irradiation. These data demonstrate that HMEC-1 cells were capable of porphyrin biosynthesis, and that exposure of protoporphyrin-containing HMEC-1 cells to UVA and blue light, which includes the Soret band spectrum, decreased the ferrochelatase activity and its protein. These changes were mediated, at least in part, by reactive oxygen species.     

ACTINIC RETICULOID–AN IDIOPATHIC PHOTODERMATOSIS WITH CELLULAR SENSITIVITY TO NEAR ULTRAVIOLET RADIATION

Abstract— Long wavelength UV radiations (320–400 nm) cause persistent inhibition of RNA synthesis and marked cytopathic changes in fibroblasts from patients with actinic reticuloid (AR) but not in those from patients with Bloom syndrome or xeroderma pigmentosum. Furthermore, the AR cells show abnormal DNA fragmentation when they are irradiated at temperatures compatible with enzyme activity. Germicidal UVR ( ca . 95% 254 nm) stimulates DNA repair synthesis and inhibits DNA replication to a normal extent in the AR cells.
Thus, actinic reticuloid, a severe photodermatosis, characterised by skin sensitivity to UV-B, UV-A and part of the visible spectrum and by infiltrates reminiscent of mycosis fungoides, is a human disease with in vitro cellular sensitivity to UV-A and, to our knowledge, is also the first to be reported.
We advance the hypothesis that inefficient cellular neutralisation of free radicals may explain the cellular phenotype of actinic reticuloid and contribute to the establishment of a vicious circle that would favour the chronic clinical course and persistent lympho-histiocytic skin infiltrates characteristic of the disease.     

EFFECT OF UV IRRADIATION ON LETHAL INFECTION OF MICE WITH Candida albicans

Exposure of mice to UV radiation inhibits the induction and elicitation of the delayed-type hypersensitivity (DTH) response to Candida albicans. To determine whether UV irradiation also affects the pathogenesis of systemic C. albicans infection, C3H mice were exposed to a single dose of 48 kJ/m² UV-B radiation from FS40 sunlamps 5 days before or 5 days after sensitization with formalin-fixed C. albicans and challenged intravenously (i.v.) with a lethal dose of viable fungi 6 days after sensitization (11 or 1 days after UV irradiation). Exposing unsensitized mice to UV radiation 11 days before lethal challenge had no effect on survival, but the survival time of mice exposed to UV radiation 1 day before challenge was reduced by more than 50%. In the latter group, decreased survival time correlated with persistence of C. albicans in the brain and progressive growth of C. albicans in the kidneys. Sensitization of unirradiated mice with formalin-fixed C. albicans extended their survival time following lethal i.v. challenge with viable C. albicans. Exposing the mice to UV radiation 5 days before sensitization did not abrogate this beneficial effect of sensitization on survival, even though it significantly reduced the DTH response. Thus, immunity to systemic infection did not depend on the ability of the mice to exhibit a DTH response to C. albicans. The beneficial effect of sensitization on survival after lethal infection was abrogated, however, in mice exposed to UV radiation 1 day before lethal challenge with C. albicans. Furthermore, these mice were unable to contain the progressive growth of C. albicuns in the kidneys, in contrast to sensitized, unirradiated mice. The induction of cutaneous inflammation with turpentine had no effect on the survival rate of mice lethally infected with C. albicans, suggesting that inflammation alone is not sufficient to decrease the survival time of C. albicans-infected mice.     

SENSITIVITY OF MARINE PHYTOPLANKTON TO UV-B RADIATION: IMPACT UPON A MODEL ECOSYSTEM

Abstract Human activities may cause a 16% reduction of stratospheric ozone. The concomitant increase in solar UV-B radiation reaching the surface of the earth could detrimentally affect the phytoplankton that form the base of the food web in oceanic and estuarine ecosystems. In the current study acute exposure of seven species of marine phytoplankton to UV–B radiation depressed the radiocarbon estimate of primary production. A model of a marine ecosystem was constructed based on the differential sensitivities of the seven species of phytoplankton. Increasing the UV–B exposure within the model from 100 Eff_DNAJ/m²/day to 150 Eff_DNAJ/m²/day significantly altered the community composition of the ecosystem. In nature, alteration of the phytoplanktonic community structure could result in a significant impact upon successional patterns and primary producer–consumer trophodynamics.     

EFFECT OF POLYAMINE DEPLETION ON DNA DAMAGE and REPAIR FOLLOWING UV IRRADIATION OF HeLa CELLS

Treatment of HeLa cells with the polyamine biosynthesis inhibitors, methylglyoxal bis(guanylhydrazone) (MGBG), difluoromethylornithine (DFMO) or a combination of the two, resulted in reduction in cellular polyamine levels. Analysis of UV light-induced DNA damage and repair in these polyamine depleted cells revealed distinct differences in the repair process relative to that seen in cells possessing a normal polyamine complement. Initial yield of thymine dimers and rate of removal of these lesions from cellular DNA appeared normal in polyamine-depleted cells. However, depleted cells exhibited retarded sealing of DNA strand breaks resulting from cellular repair processes, reduced repair synthesis and an increased sensitivity to UV killing. Incision at damaged sites was not affected since ara-C repair-dependent breaks accumulated in a normal fashion. Molecular analysis of inhibited repair sites by exonuclease III and T4 DNA ligase probes suggest that the strand interruptions consist of gaps rather than ligatable nicks, consistent with an interpretation of the repair defect being at the gap-filling stage rather than the ligation step. Observed patterns of differential polyamine depletion by DFMO and MGBG, and partial reversal of repair inhibition by polyamine supplementation, suggests that polyamine depletion per se, rather than some secondary effect of inhibitor treatment, is responsible for the inhibition of repair.     

含卤高聚物记录材料的研究——不同共聚单体对紫外光敏性的影响

研究了与偏二溴乙烯(VDBr,M_1)共聚的不同单体(M_2)——丙烯酸甲酯(MA)、甲基丙烯酸甲酯(MMA)和苯乙烯(St)的性质和共聚物的序列分布对记录材料紫外光敏性的影响。结果表明,含St的紫外光敏性最高,含MA的较差。对同一类共聚物记录材料而言,光敏性与共聚物的序列分布,主要是P_2(M_1M_2)有对应关系。本文还报道了VDBr与MA、MMA及St在55±0.2℃以偶氮二异丁腈为引发剂的自由基共聚反应竞聚率(r)分别为,VDBr-MA:r_1=0.72±0.05,r_1=0.72±0.05;VDBr-MMA:r_1=0.50±0.04,r_2=1.74±0.04;VDBr-St:r_1=0.40±0.04,r_2=1.12±0.04。     

SENSITIVITY OF HemA MUTANT Escherichia coli CELLS TO INACTIVATION BY NEAR-UV LIGHT DEPENDS ON THE LEVEL OF SUPPLEMENTATION WITH δ-AMINOLEVULINIC ACID

Abstract— Four strains carrying all four possible combinations of the alleles nur, nur⁺, uvr A6 and uvr A ⁺ were transduced to hemA8 . The hemA8 mutation blocks the synthesis of δ-aminolevulinic acid (δ-ALA), one of the first steps in the synthesis of porphyrin and, ultimately, cytochromes essential for aerobic respiration. The cells were grown either with or without δ-ALA and treated with broad-spectrum near-ultraviolet light (NUV; 300–400 nm). hemA8 defective cells grown without δ-ALA were resistant to inactivation by NUV while hemA8 cells were sensitive to such inactivation when supplemented with δ-ALA. The sensitivity to NUV inactivation conferred by the nur gene was retained in the hemA8 derivatives. The sensitivity of such cells to NUV inactivation can be controlled by varying the level of δ-ALA supplementation. The level of δ-ALA supplementation did not influence the sensitivity of the cells to inactivation by far-UV light (FUV; 200–300 nm). The near-UV sensitivity of hemA⁺ cells was not significantly altered when grown with δ-ALA suppiementation suggesting that endogenously formed δ-ALA supports the normal, regulated level of porphyrin synthesis. These results can be interpreted to mean that porphyrin components of the respiratory chain in E. coli represent chromophores involved specifically in broad-spectrum NUV inactivating events.     

单茂钛催化剂的丙烯无规聚合反应及其动力学研究

比较了不同钛化合物／甲基铝氧烷（ＭＡＯ）催化体系的丙烯无规聚合，催化活性次序为ＣｐＴｉ（ＯＲ）３＞ＣｐＴｉ（ＯＰｈ）３＞ＣｐＴｉＣｌ３＞Ｃｐ２ＴｉＣｌ２＞Ｔｉ（ＯＢｕ）４＞ＴｉＣｌ４＞Ｔｉ（ＯＢｕ）２Ｃｌ２，所得聚丙烯用沸庚烷抽提８ｈ，溶解９５％以上，可溶部分经１３Ｃ ＮＭＲ、ＷＡＤＸ、ＦＴＩＲ等分析证明为无规聚丙烯（ａＰＰ），是没有结晶性的弹性体．ＧＰＣ测出其分子量Ｍｗ＝８．０～１０．０×１０４，Ｍｗ／Ｍｎ≈２．０．探索了催化体系ＣｐＴｉ（Ｏ ｎ Ｐｒ）３／ＭＡＯ中钛的浓度、［Ａｌ］／［Ｔｉ］摩尔比，丙烯聚合压力，聚合温度和时间对丙烯聚合反应的影响．研究了该催化体系丙烯聚合反应动力学规律，表观聚合反应速率对催化剂浓度和单体压力（浓度）都呈一级反应关系，表观聚合速率常数ＫＰ＝２９２×１０５ｍｏｌ／Ｌ·ｈ（４０℃）．活化能ΔＥ＝－７．８８×１０３Ｊ·ｍｏｌ－１，碰撞因子Ａ＝１．４１×１０－４ｍｏｌ／Ｌ·ｈ．