竹红菌光敏作用的初步探讨*

用纸片法作为筛选光敏物质及光敏作用的研究方法。结果证实了(1)竹红菌Hypo crella bambusae中含有对革兰氏阳性细菌具光敏活性的成分;(2)从中筛选到一种红色的光敏色素,属苝醌的一个新的衍生物,取名竹红菌甲素(Hypocrellin A简称“甲素”);(3)揭示了“甲素”是对可见光敏感、作用光谱较宽的光动力学(photodynamic)物质。从化合物的类型、光敏特性、治疗方法、治疗对象及其效果看,可以认为甲素是一新型的光化学疗法药物。     

竹红菌光敏作用的初步探讨

用纸片法作为筛选光敏物质及光敏作用的研究方法。结果证实了(1)竹红菌Hypo crella bambusae中含有对革兰氏阳性细菌具光敏活性的成分;(2)从中筛选到一种红色的光敏色素,属苝醌的一个新的衍生物,取名竹红菌甲素(Hypocrellin A简称“甲素”);(3)揭示了“甲素”是对可见光敏感、作用光谱较宽的光动力学(photodynamic)物质。从化合物的类型、光敏特性、治疗方法、治疗对象及其效果看,可以认为甲素是一新型的光化学疗法药物。     

人胎肝中低分子天然抑瘤物对小鼠肉瘤S—180作用的研究

从人胎儿肝脏中分离出一种分子量较小的抑瘤物质(FLS-MeOH),观察了它对小鼠肉瘤S-180细胞生长的抑制效应。在体外琼脂培养中,当FLS-MeOH浓度达到300μg/ml时,可完全抑制S-180细胞的集落形成;给荷瘤小鼠每日注射FLS-MeOH8mg/g体重,共20d,可明显延长小鼠的存活时间,部分小鼠可以无病存活。这些结果说明FLSMeOH在体内外均有明显的抗肿瘤活性,而且具有分子量小、无组织和种系特异性,以及对肿瘤细胞不可逆的毒性作用等特性。     

膜脂过氧化产物在光敏诱发细胞突变中的作用

本文选用ＣＨＯ细胞,通过竹红菌甲素（ＨＡ）光敏诱变及ｏｕａ选择性培养液的筛选,证实甲素光敏反应对细胞Ｎａ＾＋／Ｋ＾＋ ＡＴＰ酶基因具有诱变致突作用。对其突变效应与脂质过氧化反应及ＤＮＡ加成物形成关系的分析表明,ＴＢＡ反应产物随着光照时间的增加而增加,同时ＤＮＡ加成物生成迅速增加,突变频率也随之增高。维生素Ｅ可抑制脂质过氧化反应,并减少ＤＮＡ加成物生成,阻止细胞突变率的增加。提示光敏诱发细胞脂质过氧     

竹红菌乙素对小鼠腹水型肝癌细胞的光敏杀伤作用

研究了竹红菌乙素(以下简称乙素,HB)对小鼠腹水型肝癌细胞(AH)的杀伤作用,并初步解释了其杀伤机理。实验证明乙素对AH细胞杀伤与乙素浓度的平方根成正比。乙素杀伤细胞的能力与竹红菌甲素(以下简称甲素,HA)相等,比血卟啉强,但比原卟啉弱,电镜观察可见:损伤细胞的膜失去连续结构,线粒体,内质网等细胞器变形,最终导致细胞空泡化。此外,细胞变形,表面微绒毛精细结构丧失,也是光敏损伤的主要特征。造成细胞死亡的原因包括~1O,O_2~-和·OH在内的活性氧,而·OH主要由O_2~-转换而来。     

竹红菌甲素光敏作用所致的HeLa细胞DNA单链断裂重接的研究

本文采用羟基磷灰石离心法对竹红菌甲素光敏作用所致的HeLa细胞DNA的单链断裂进行荧光定量测定。以单链DNA的含量变化衡量DNA链断裂程度及其修复活性,并与γ射线的作用进行了比较。细胞经γ射线和甲素的光敏作用后,DNA产生单链断裂,当细胞存活率为0.1时,前者是6.0×10~(-10)断裂/道尔顿,后者是2.3×10~(-10)断裂/道尔顿,两者之比为2.8。细胞本身具有修复能力,当最初的单链断裂频率相等时,γ射线处理的细胞其DNA单链断裂重接能力高于光敏作用的细胞。后者的修复能力能被羟基脲、放线菌素D及丁酸钠等所抑制。细胞修复能力的差别指出两种作用产生的单链断裂的化学性质有重要差别。     

竹红菌甲素-脂质体的制备及其特性

利用反相蒸发技术制备了竹红茵甲素脂质体体系,测定了其光谱和稳定性,结果表明:在该体系中,竹红菌甲素的Ⅰ吸收峰、荧光峰均出现红移且有荧光增强效应。竹红菌甲素-脂质体(浓度0.05～0.5mg/ml)在4℃下存放2-3d,光密度下降5％左右。     

竹红菌甲素对红细胞膜的光损伤

光敏化剂竹红菌甲素在可见光区有三个吸收峰,其波长为475nm、545nm和585nm。在有竹红菌甲素存在时,红细胞膜样品用250W碘钨灯照射,其光强度为48尔格/平方毫米·秒。辐照后观察到以下一些效应:1)膜蛋白SH基含量减少。2)膜蛋白敏感的氨基酸残基,如组氨酸、半胱氨酸和色氨酸含量降低。3)膜蛋白发生光??聚集作用。4)多聚不饱和类脂发生过氧化作用。竹红菌甲素光照不同时间后和竹红菌甲素光照后放置一段时间,再加到红细胞膜中,均能观察到膜蛋白SH基含量降低。提示竹红菌甲素的光氧化产物是稳定的,能引起红细胞膜的光损伤。     

地鳖虫蛋白提取物对小鼠S180肉瘤及鸡胚尿囊膜血管生成的抑制作用

用不同浓度的地鳖虫蛋白粗提物(0.2~0.8g/ml)作用于S180肉瘤荷瘤小鼠,观察各组的抑瘤效果及重要生理指标的差异;同时分别用地鳖虫蛋白粗提物以及经过盐析、离子交换层析、分子筛由地鳖虫蛋白粗提物分离纯化得到的活性蛋白,作用于鸡胚尿囊膜,观察它们对新生血管生成的抑制作用。结果显示,地鳖虫蛋白粗提物对S180肉瘤荷瘤小鼠有显著的抑瘤作用;蛋白质粗提物以及纯化得到的活性蛋白对鸡胚尿囊膜新生血管的生成有明显的抑制作用,纯化品的抑制活性高于粗品,且二者对鸡胚生长发育的影响较阳性对照(地塞米松组)小,差异显著。因此,地鳖虫蛋白提取物有良好的体内抑瘤作用及血管生成抑制活性。     

竹红菌甲素对红细胞膜和几种磷脂脂质体膜的流动性的光敏损伤

本文以荧光探针为手段,通过测量膜偏振度的变化,探讨了竹红菌甲素光敏作用对红细胞膜和几种磷脂脂质体膜的流动性的损伤。结果表明,甲素光敏作用使不同种类的磷脂(DPPC,DPPC/DPPE,红细胞膜磷脂)脂质体的流动性增加,其对光敏作用的敏感程度为红细胞膜磷脂脂质体显著小于DPPC/DPPE脂质体及DPPC脂质体。对红细胞膜来说,甲素光敏作用使其流动性呈现先降低而后增加的现象。去除膜上的spectrin以及用胰蛋白酶处理可使这种流动性变化的幅度受到抑制。据此,我们认为,膜磷脂,膜蛋白对甲素光敏作用中膜流动性的变化有着不同的影响,膜蛋白,特别是spectrin,是其中极重要的因素。     

白介素3治疗小鼠造血功能低下的疗效及机理初探

通过整体实验观察国产重组白介素３（ＩＬ－３）对射线和环磷酰胺所致小鼠造血功能低下的疗效;以体外实验分析其疗效机理。实验结果表明：（１）ｒｈＩＬ－３腹腔或皮下连续５天注射能全面提高７Ｇｙ照射小鼠９天时股骨骨髓ＣＦＵ－Ｅ、ＢＦＵ－Ｅ、ＣＦＵ－Ｍｉｘ和ＣＦＵ－ＧＭ的产率和数量,其效果强弱与注射途径和用药剂量有关。ｒｈＩＬ－３对小鼠股骨骨髓有核细胞总数和内源性脾结节数的改善影响小。（２）ｒｈＩＬ－３对环磷酰胺所致小鼠造血功能低下亦有改善效果,并与起用时间和剂量有关。（３）ｒｈＩＬ－３对人骨髓细胞和ＣＦＵ－ＧＭ集落形成有明显的增强作用。小鼠骨髓细胞对ｒｈＩＬ－３缺乏反应;对ｒｍＩＬ－３有增殖分化加强的反应。ｒｍＩＬ－３体外共育能提高正常及照射２Ｇｙ小鼠骨髓细胞体外培养后ＣＦＵ－ＧＭ的产率和数量。文中讨论了ＩＬ－３的应用前景及合理方案问题。     

涉及光疗机制的生物光化学

本文对光生物和光化学的定义,反应机制的类型和光敏化作用等做了阐述。下面例举几个光疗的成果 1.光疗牛皮癣 经常使用的8-甲氧基补骨脂素在UVA的照射下,从基态被激发到三重态。它主要和DNA中的胸腺嘧啶,其次和色氨酸进行光环合加成,形成交联,阻止DNA和RNA的合成,抑制具过度增生 2.血卟啉衍生物(HPD)治癌 HPD有定位于癌组织的能力和光动力作用,可推断病人体内癌部位。 讨论了HPD的光疗机制,和酞菁相比,有各自的优缺点。 3.竹红菌素 主要治疗妇女外阴白色病变和疤痕疙瘩,抑制癌细胞生长。 讨论了竹红菌甲素和乙素及它们的氧化物的结构和活性。 在大于510nm的光照射下,也可抑制癌细胞的生长。列举了竹红菌素的优缺点。     

Enhancing effects of mini-cells prepared from Salmonella typhimurium on anti-tumor immunity in sarcoma 180-bearing mice

Summary The enhancing effect of mini-cells of Salmonella typhimurium which do not contain chromosomal DNA on anti-tumor immunity in mice was studied. The growth of sarcoma 180 cells which were subcutaneously transplanted into ICR mice was significantly retarded in mice treated with Salmonella mini-cells at the same time or 7 days after S180 transplantation, while no or only a little growth inhibition was observed in mice treated 7 days prior to S180 transplantation. Treatment with mini-cells inoculation alone did not increase the survival time of mice that had received intraperitoneal transplants of S180 cells. However, a statistically significant increase of survival time was observed in mice treated with a combination of mini-cells and surgical resection of subcutaneous tumors when S180 cells were injected 7 days after the surgical resection. The injection of mini-cells restored macrophage chemotaxis in S180-bearing mice in which macrophage chemotaxis was greatly retarded but lymphocyte activity was not.     

Tissue-selective inhibition of cholesterol synthesis in vivo by pravastatin sodium, a 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitor

Tissue selectivity of pravastatin sodium (pravastatin) in inhibition of cholesterol synthesis was investigated and its effect was compared with other 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors, such as lovastatin, simvastatin and ML-236B. Inhibition of cholesterol synthesis in vivo was measured by incorporation of radioactivity into the sterol fraction 1 h after intraperitoneal injection of [14C]acetate to mice. The drugs were orally administered to mice 2 h before the acetate injection. When pravastatin at a dose of 20 mg/kg was administered to mice, about 90% inhibition of cholesterol synthesis was observed in liver and ileum, but the inhibition was less than 14% in kidney, spleen, adrenal, testis, prostate and brain. This tissue selectivity of pravastatin was also demonstrated even in varying doses (5-100 mg/kg) and time (75-180 min) after drug administration. Other 3-hydroxyl-3-methylglutaryl coenzyme A reductase inhibitors did not show such a tissue-selective inhibition of sterol synthesis under the same conditions. These results obtained with the in vivo study were confirmed in vitro by the inhibition of sterol synthesis in various cultured cells and rats lenses, as well as by cellular uptake of 3-hydroxy-3-methylglutaryl coenzyme A reductase inhibitors.     

Biochemical and cellular mechanisms of low-dose effects

Low-dose irradiation is usually considered to be rather ineffective in producing biologically relevant effects. Yet, individual radiation absorption events within cell nuclei or whole cells interact stochastically with subcellular structures due to the multiple ionizations along primary or secondary particle tracks, depending on ionization density. Whereas radiation effects are usually seen in the context of structure and function of DNA, other cellular effects, perhaps influencing DNA by secondary biochemical mechanisms, also warrant attention. Thus, previous work from this laboratory with bone marrow that was obtained from whole-body exposed mice, has shown that single or few instantaneous radiation absorption events per cell from gamma-rays produce an acute and temporary partial inhibition of the enzyme thymidine kinase; the effect appears within about 1 h after the event, reaches its maximum at approximately 4 h and disappears completely within another 6 h. This pattern of enzyme inhibition is fully concordant with the pattern of inhibition of uptake of tritiated thymidine or 125I-labelled deoxyuridine into the DNA; also concordant is a temporary increase in the concentration of free thymidine in the blood serum of the exposed mice. The particular response of thymidine kinase was considered to relate to some, thus far unknown, repair systems and/or to a defence mechanism of the hit cells. In order to further elucidate the role of the acute and temporary partial inhibition of thymidine kinase in cellular metabolism, experiments were carried out in which mice were acutely exposed to 0.01 or 0.1 Gy and again exposed to the same dose at different times up to 12 h after the first exposure. At regular time intervals after the second exposure bone marrow cells were obtained and thymidine kinase activity was studied by various assays. The results indicate that the first acute irradiation conditioned the cells in such a way that the second acute irradiation produced either an enhanced inhibition and recovery of thymidine kinase activity, or no effect at all was seen, when the second irradiation was given between about 3 and 8 h after the first irradiation. From 8 to 12 h after the first irradiation the cells apparently resumed their original state, so that the second irradiation produced effects quite similar to those seen after a single irradiation in unconditioned cells.(ABSTRACT TRUNCATED AT 400 WORDS)     

竹红菌乙素对菌紫质荧光的影响

用荧光光谱方法研究了竹红菌乙素与菌紫质的相互作用。通过竹红菌乙素对菌紫质吸收光谱,对菌紫质荧光猝死的浓度和温度的依赖性以及竹红菌乙素对明暗适应菌紫质的荧光猝灭等研究表明,竹红菌乙素是一种新型的荧光猝灭剂,它对菌紫质的荧光猝灭属于动态猝死过程。竹红菌乙素对明暗适应菌紫质荧光猝灭的差别,说明这种猝灭剂可用于生物膜体系的蛋白质构象变化的研究。     

竹红菌甲素对红细胞膜内脂双层的微扰

本文以荧光探针为手段,以人红细胞膜为材料,测量了膜偏振度的改变,荧光探针能量转移,荧光峰的蓝移和甲素激发峰的分裂。结果表明在有竹红菌甲素存在时,红细胞膜偏振度增加,探针荧光强度减小,荧光峰蓝移。甲素浓度增加时,上述现象更加明显,即它们之间有正的相关关系。同时,甲素激发光谱的a带发生分裂。据此,我们认为甲素对红细胞膜内脂双层产生明显微扰,甲素与红细胞膜间存在着相互作用。在甲素浓度较大时,它主要是渗入到红细胞膜脂双层的深层部位(膜脂肪酸链的12—16位)。     

Induction of allograft tolerance after total lymphoid irradiation (TLI): development of suppressor cells of the mixed leukocyte reaction (MLR).

We searched for the presence of suppressor cells of the MLR in C57BL/Ka leads to BALB/c chimeras. The chimeras were made with total lymphoid irradiation (TLI) and marrow transplantation. Spleen cells from the old chimeras inhibited the MLR of BALB/c responder cells against C57BL/Ka stimulator cells. Inhibition was specific for the stimulator cells, since no effect on the MLR was observed with C3H or BALB.C3H stimulator cells. Maximal inhibition was achieved when the responder cells in the MLR shared the H-2 haplotype of the chimeric recipient. Spleen cells obtained from chimeras young 30 to 40 days after BM transplantation inhibited the MLR nonspecifically, since similar marked inhibition was observed regardless of the H-2 haplotype of the responder or stimulator cells. The finding of antigen-specific and nonspecific suppressor cells is similar to that observed in mice rendered tolerant to bovine serum albumin after treatment with TLI.     

Observations on the effect of radiotherapy,followed by injection of pig lymph node cells,in reducing the number of pulmonary tumors induced by intravenous injection of tumor cells into isogenic mice

Summary Pulmonary tumors were produced in A. strain mice by intravenous injection of A. strain mammary carcinoma cells. The mesenteric lymph nodes of pigs were immunized by implantation of fragments from the same tumors into the pig mesentery.Tumor-immune pig lymph node cells when injected IV 7 days after tumor cells did not reduce the number of tumors, counted on day 14. However, when preceded by 200 rad thoracic irradiation on day 3 (which increased the number of pig cells settling in the lungs) tumor-immune cells given IV reduced the number of tumors compared with the effect of irradiation alone, or in combination with nonimmune pig cells.When tumor-immune pig cells were injected IP on day 7 (following thoracic irradiation on day 3), no antitumor effect was observed. Thus immediate pig cell/tumor cell contact is important in order to obtain an antitumor effect.Pig cells immunized against a human bladder carcinoma did not reduce pulmonary tumor formation by one of the mouse tumors.     

Allosensitization induced suppression of various murine tumors: role of non-H-2 antigens in antitumor immunity

Presence of alloantigens on various murine tumors was tested by tumor rejection in allosensitized Swiss mice. The results indicated the presence of alloantigen on immunogenic tumors like chemically induced fibrosarcoma (FS), ascitic sarcoma 180 (S 180) and immunogenic variant of lymphosarcoma (LS-A) in Swiss mice, while these antigens could not be detected by this procedure on spontaneous lymphosarcoma (LS). Allosensitization with skin graft was found to offer quantitatively higher antitumor resistance than the allosensitization achieved by allogeneic lymphocytes. Antitumor effect was not seen when tumor cells were inoculated earlier than day 3 of grafting. Further, host immunosuppression with whole body irradiation up to day of 3 of skin grafting abrogated the antitumor effect. H-2 compatible and non-H-2 incompatible skin graft sensitization of host could offer resistance against both S 180 and LS-A. Further, tumor immune mice rejected H-2 compatible, non-H-2 incompatible skin graft significantly earlier.