用离心逆流分配色谱仪分离POLY I:C

用两相溶剂系统的离心逆流分配色谱仪,分离人工合成聚肌胞Poly I:C.采用步进洗脱和梯度洗脱.在梯度洗脱中对Ito氏的缓冲液进行改进,得到了很好的分离结果,分成四个组分,其沉降系数分别为12s,7.0s,6.3s,和3.8s.此分离结果优于普通柱色的结果.     

ON "REVERSAL" OF PHOTOTROPISM IN PHYCOMYCES

Alleged reversal of the phototropism of the sporangiophores of Phycomyces by high intensities of light does not occur if infra-red radiation is properly excluded. Phototropic "indifference" alone occurs at high intensities due to equal photic action on both sides of the sporangiophore. If heat radiation is not screened out, a gradual, negative thermotropic bending takes place.     

OCTAHEDRAL CRYSTALS IN PHYCOMYCES. II

"Phycomyces blakesleeanus" sporangiophores contain octahedral crystals throughout their cytoplasm and vacuole. More octahedral crystals were found in the wild-type strain G5 (+) than in the β-carotene-deficient mutant C5 (-), and much more than in the mutant C141 (-), which is sensitive to only high light intensity. In the wild type, the number of crystals per sporangiophore increased until the sporangiophore reached stage IV, and then decreased. Stage I contained the most crystals per unit volume. Cultures grown in darkness had the maximum number of crystals. Under high light intensity, there was an overall reduction of crystals. The crystals are regular octahedrons. The crystals were isolated from the sporangiophores by a method of sucrose density-gradient centrifugation. They contain nearly 95% protein, are stable in organic solvents, but can be solubilized in buffer solution above pH 9.5 and below 2.5. The crystals weakly fluoresce with an emission peak at 540 nm, which is affected by irradiation with white light. Absorption spectra of freshly prepared crystals show absorption maxima around 265–285 nm, 350–380 nm, and 450–470 nm. These absorption peaks for the crystals are close to those of the phototropic and light-growth action spectra. These data suggest that the crystals may contain a flavoprotein which may be the photoreceptor pigment of "Phycomyces".     

THE ORGANIZATION AND EVOLUTION OF MICROTUBULAR ORGANELLES IN CILIATED PROTOZOA

(1) Ciliated protozoa are viewed as unicellular organisms structured in a hierarchy of organizational levels that include the macromolecular, suborganellar, unit organellar, organellar complex, and organellar system. (2) The ciliate cortex is divided into two major functional regions, the somatic region and the oral region. The fundamental component of the cortex is an organellar complex, the kinetid, whose organizing centre is the kinetosome with which are associated three fibrillar associates diagnostic of ciliates. These three fibrillar associates are the periodically striated kinetodesmal fibril and two microtubular ribbons, the transverse and postciliary ribbons. (3) Somatic and oral kinetids are found to be of three major types: monokinetids are composed of one kinetosome and its fibrillar associates; dikinetids are composed of two kinetosomes and their fibrillar associates; polykinetids are composed of more than two kinetosomes and their fibrillar associptes. (4) The mechanisms underlying kinetid function and development remain largely unexplored. Research into the molecular biology and ultrastructure, especially of mutant forms, should provide basic insights in the near future. (5) The conservation of kinetid structure across major phyla of organisms suggests that this subcellular structure should be useful in phylogenetic analysis despite the concepts of ‘chemical identity’ and ‘organic design’. (6) The evolutionary rate of change of oral features is greater than that of somatic features, probably due to developmental and ecological factors. Nevertheless both cortical regions are constrained by the phenomenon of structural conservatism; that is, the conservation of structure through time is inversely related to the level of biological organization. (7) Eight major groupings of ciliate species are recognized, based on ultrastruc-tural features of the cortex. Several examples of differences between these eight groups and the groups presently recognized are discussed.     

银杏精子细胞生毛体及其它细胞器的超微结构

生毛体与嗜锇颗粒是银杏 (Ginkgobiloba)精子细胞中最具有标志性的结构。生毛体是细胞质内一直径为 3～ 4μm的圆球形结构 ,它由一个电子致密的核心和由此向周边发散出的辐射状中心粒组成 ,致密核心上具有微管结构的弱电子染色区域 ,并有微管从生毛体延伸到细胞质。嗜锇颗粒直径为 1 0～ 2 0μm,呈圆球状 ,位于生毛体和细胞核之间 ,其相对的另一侧存在纤维颗粒体。在精子细胞质内 ,特别是嗜锇颗粒和生毛体周围线粒体、质体、内质网、高尔基体等细胞器丰富。银杏精子细胞核较大 ,在细胞核内 ,核仁结构呈球形 ,电子染色致密的颗粒区在周围 ,而纤维组分则在圆球的中间。在核膜表面布满了分布不均匀的核孔复合体。     

FERRITIN IN THE FUNGUS PHYCOMYCES

The iron-protein ferritin has been purified from mycelium, sporangiophores, and spores of the fungus Phycomyces blakesleeanus. It has a protein-to-iron ratio of 5, a sedimentation coefficient of 55S, a buoyant density in CsCl of 1.82 g/cm³, and the characteristic morphology of ferritin in the electron microscope. Apoferritin prepared from Phycomyces ferritin has a sedimentation coefficient of 18S and consists of subunits of molecular weight 25,000. In the cytoplasm of Phycomyces, ferritin is located on the surface of lipid droplets (0.5–2.0 µ in diameter) where it forms crystalline monolayers which are conspicuous in electron micrographs of sporangiophore thin-sections. Ferritin is found in all developmental stages of Phycomyces but is concentrated in spores. The level of ferritin iron is regulated by the iron level in the growth medium, a 50-fold increase occurring on iron-supplemented medium.     

INTRACELLULAR LOCALIZATION OF KYNURENINE IN THE FATBODY OF DROSOPHILA

Light blue fluorescent globules accumulate in the cells of the anterior region of the fatbody of Drosophila larvae near the time of pupation. This fluorescent material appears in the Ore-R wild type strain as well as mutant strains in which the synthesis of both the red and brown eye pigments is affected. The vermilion mutant, which is characterized by the absence of the brown pigment component in the eye, was the only strain among those examined which did not develop the light blue fluorescent globules. Utilizing chromatographic techniques together with the information gained by examination of the mutant strains, the fluorescent material has been identified as kynurenine. Of particular interest is the manner of appearance of the fluorescent material in the vicinity of the nuclear membrane of the fat cells.     

超氧物歧化酶在植物细胞内的分布

大豆幼苗下胚轴的SOD活性主要存在于细胞溶质,约占细胞内总活性的87.3％,其次分布在线粒体,约占总活性的6.8～7.2％。细胞溶质的SOD以Cu-Zn-SOD(SODb_1b_2b_2)类型为主,它在细胞溶质中约占86％。线粒体的SOD主要是Mn-SOD(SOD_a)类型,它在线粒体中约占74～76％。大豆幼苗下胚轴的SOD同工酶活性,SOD_a(Mn-SOD)约占13％,SODb_1b_2b_2(Cu-Zn-SOD)约占77％,SODc_1c_2c_2(Cu-Sn-SOD)约占10％,表明大豆幼苗下胚轴的三组同工酶以SODb_1b_1b_2为最强。比较绿色与黄化花生幼苗子叶SODc_1c_2c_2的差异,证明SODc_1c_2c_2的形成与光照下叶绿体的正常发育有关。     

FINE STRUCTURES OF INTRACYTOPLASMIC ORGANELLES OF MYCOBACTERIA

The fine structure of the intracytoplasmic organelles of mycobacteria was studied by means of electron microscopy of ultrathin sections. A well-preserved nuclear apparatus was obtained by fixation with OsO₄ in acetate-veronal buffer, containing calcium and tryptone, or in collidine-HCl buffer, followed by uranyl-acetate treatment and embedding in araldite. A low density nuclear region was filled with fine fibrils, 30 A in diameter, in parallel or concentric arrangement. A membranous organelle, tentatively designated as "lamellar structure," consists of unit membranes in lamellar arrangement. The thickness of each lamella in this membranous organelle coincides with that of the three-layered cytoplasmic membrane Moreover, the continuity of this unit membrane with the cytoplasmic membrane was demonstrated.     

INTRACELLULAR LOCALIZATION OF PHENOL SULPHOTRANSFERASE IN RAT BRAIN

—The intracellular localization of phenol sulphotransferase in rat brain was studied The distribution pattern found after differential centrifugation closely resembles that of lactate dehydrogenase and does not change during postnatal development. The distribution of the enzyme in discontinuous and continuous sucrose gradients, however, shows a deviation from the lactate dehydrogenase pattern and a shift towards a higher sucrose concentration during development. In the adult the phenol sulphotransferase coincides with monoamine oxidase, succinate dehydrogenase and β-glucuronidase. Disruption experiments, purification of mitochondria and electron microscopy exclude localization of phenol sulphotransferase in mitochondria. These studies support the idea of phenol sulphotransferase as a cytoplasmic enzyme with a preferential binding to or localization in oligodendroglial cells or, more probably, a specific type of synaptosomes.     

INTRACELLULAR LOCALIZATION OF NATIVE AUXIN IN AVENA COLEOPTILE

Intracellular localization of the native auxin in the Avenacole-optile tip was investigated by separating cellular fractionsby differential centrifugation. Each fraction was extractedwith ether and the auxin activity was measured by the sensitizedAvena curvature test. After the removal of the native free auxin,each fraction was alkaline-hydrolyied, and from these hydrolyzatesthe bound auxin was extracted with ether and its activity wasmeasured. Both the native free auxin and the native bound auxinin these extracts were identified as IAA by paper chromatography.The results show that the native free auxin occurs only in thesupernatant soluble cytoplasm, and that the native bound auxinlocalizes also in the supernatant. The distribution of the externallyapplied IAA was also investigated. (Received February 27, 1962; )     

罗氏沼虾卵母细胞细胞器与卵黄发生的关系

作者研究了罗氏沼虾卵母细胞细胞器与卵黄发生的关系。细胞核物质通过核孔与细胞质进行物质交换,由核仁而来的核糖体前体物在细胞质中形成大量的核糖体。一部分核糖体附着在内质网囊泡的膜上,形成粗糙型内质网。粗糙型内质同囊泡具有合成和运输卵黄物质的功能。一部分核糖体是游离的,它们可在细胞质中合成致密蛋白质小颗粒,随后这些颗粒逐渐聚集融合成致密的卵黄粒。溶酶体可吞噬这些由游离核糖体形成的蛋白质颗粒团或其它膜状物,并将它们消化、融合,从而形成大的卵黄粒。部分线粒体参与了卵黄粒的合成并最终演变成卵黄体。微丝也参与了卵黄粒的形成。       

热暴露大鼠心肌细胞钙稳态及其调节机制的研究

本文观察了离体成年大鼠心室肌肌质网、线粒体Ｃａ＾２＋－ＡＴＰ酶活性和总钙含是到及原代培养乳腺心肌细胞＾４６Ｃａ摄取、活性钙调素相对含量、胞浆内游离钙浓度在不同温度热暴露４０ｍｉｎ后的变化。结果表明：热暴露后,心肌奖浆、肌质网及线粒体中的Ｃａ＾２＋－ＡＴＰ酶活发表 所下降,心肌肌质网及线粒体中的总钙含量亦有降低趋势,心肌细胞活性钙调素相对含量显著下降,＾４６Ｃａ摄取量及胞浆内游离浓度显著升高。提示,