THE INTRAMEMBRANOUS PARTICLE PROFILE OF THE PARAMYLON MEMBRANE DURING PARAMYLON SYNTHESIS IN EUGLENA (EUGLENOPHYCEAE)1

Paramylon is the β-1, 3-glucan storage product in euglenoid algae. It is a fibrous crystal that occurs as membrane-bound granules in the cytosol. The role of the surrounding membrane in paramylon synthesis was investigated by the use of freeze-etch electron microscopy. When Euglena gracilis Klebs strain Z (Pringsheim) cells were frozen in supercooled liquid nitrogen, the fracture plane primarily was throuh the paramylon membrane. A large intramembranous particle (IMP, mean diam range 5.6-6.5 nm) and a small IMP (mean diam range 9.6-10.3 nm) were predominant in both PF (protoplasmic fracture) and EF (exoplasmic fracture) faces of the paramylon membrane. During paramylon synthesis induction, the ratio of small to large IMPs increased in both fracture faces. The IMP density decreased in both fracture faces concomitant to paramylon synthesis increase. These changes in IMP profile and density suggest that the paramylon membrane is involved in the synthesis of paramylon.     

人血小板生成素全长分子在酵母系统中的分泌表达及活性分析

外源基因可通过整合型载体被整合到毕赤酵母（Ｐｉｃｈｉａｐａｓｔｏｒｉｓ）染色体上,获得遗传性稳定分泌表达株．利用酵母信号肽ＭＦα,对该信号肽蛋白酶识别位点的相关序列进行重新设计,使天然人ＴＰＯ成熟肽在毕赤酵母系统中分泌表达成功．表达产物经Ｗｅｓｔｅｒｎ－ｂｌｏｔ进行分析,分子量约为６６ｋＤ处蛋白条带可被ＴＰＯ抗体识别;表达量约为０．１ｇ／Ｌ;Ｎ端氨基酸序列分析结果与设计的一致;表达产物对小鼠骨髓细胞形成巨核细胞集落形成单位（ｍｅｇａｋａｒｙ－ｏｃｙｔｅｃｏｌｏｎｙｆｏｒｍｉｎｇｕｎｉｔ,ＣＦＵ－Ｍｅｇ）具有明显的刺激作用．     

人肝金属硫蛋白-I_A基因在鱼腥藻中的克隆与表达

将人工合成的人肝金属硫蛋白（ｍｅｔａｌｏｔｈｉｏｎｅｉｎ,简称ＭＴ）－ＩＡ基因插入至中间载体ｐＲＬ－４３９上强启动子ｐｓｂＡ后,再将其与穿梭载体ｐＫＴ－２１０相连,得到大肠杆菌－蓝藻穿梭表达载体ｐＫＴ－ＭＴ,用三亲接合转移法将ｐＫＴ－ＭＴ转入丝状体蓝藻－鱼腥藻７１２０,经链霉素筛选,得到了稳定的转人肝ＭＴ－ＩＡ基因鱼腥藻．纯化单藻落,液体扩大培养．从鱼腥藻中提取的质粒经Ｓｏｕｔｈｅｒｎ印迹分析,确定人肝ＭＴ－ＩＡ基因已转入鱼腥藻７１２０中,Ｗｅｓｔｅｒｎ印迹分析表明,金属硫蛋白在转人肝ＭＴ－ＩＡ基因鱼腥藻中得到了表达．经原子吸收光谱法测定表达量约为７００μｇＭＴ／ｇ鲜藻,重金属耐受性实验表明,得到了能耐受重金属－镉的转人肝ＭＴ－ＩＡ基因鱼腥藻,它将在清除水域中重金属污染和医药研究方面发挥重要作用．     

Effects of light quality on growth, biochemical composition and photo synthetic production in Cyclotella caspia Grunow and Tetraselmis gracilis (Kylin) Butcher

The effects of light quality on growth, biochemical composition and photosynthetic production in Cyclotella caspia Grunow and Tetraselmis gracilis (Kylin) Butcher were evaluated under controlled laboratory conditions. Cyclotella caspia had the highest values for maximum growth rate in blue-green light, whereas T. gracilis grew faster in red light. The highest cellular contents of chlorophylls [a, (c₁ + c₂)] and carotenoids of C. caspia were found respectively in red and blue-green light, while protein content did not change in response to spectral quality. Tetraselmis gracilis cells were more stimulated to synthesize pigments and protein when incubated in white light. For both species, pigment ratios showed intermediate values in white regime. The maximum values for photosynthetic rates were obtained in blue-green and red regimes in C. caspia and in red light in T. gracilis. The chromatic adaptive mechanisms shown for both species are compared and discussed in light of recent works presented for different phytoplankters, with emphasis on ecophysiological responses obtained in distinct spectral regimes.     

Proton pumps of the plasmalemma of the yeast Rhodotorula gracilis Their coupling to fluxes of potassium and other ions

(1) Intact cells of the obligatory aerobic yeast Rhodotorula gracilis (glutinis) generate a difference of the electrochemical proton potential (Δμ_H⁺) across the plasmalemma. In the range from pH 4.0 to 7.0 its value remains close to 12 kJ/mol. At pH 4.0 it is composed of the pH difference (inside alkaline) alone, at pH 7.0 of the membrane potential alone. (2) Both components of Δμ_H⁺ are generated by an active process, as shown by their rapid dissipation under anaerobic conditions. (3) In order to find out by which type of mechanism Δμ_H⁺ is generated the effect of a number of inhibitors of transport-ATPases (among them ouabain, triphenyltin chloride, quercetin, oligomycin, venturicidin, dicyclohexylcarbodiimide, Dio-9) were tested both on the generation of the membrane potential and on the extrusion of protons either in the absence or the presence of potassium ions. We found that all three processes were inhibited by Dio-9 and dicyclohexylcarbodiimide, which are specific for H⁺-ATPases. Triphenyltin chloride inhibited the K⁺/H⁺-exchange without having any effect either on the extrusion of H⁺ alone or on the membrane potential. (4) Dicyclohexylcarbodiimide and Dio-9, but not triphenyltin chloride inhibited at pH 4.0 the active transport of sugars. This class of substrates has been shown earlier to be transported by an electrogenic H⁺ symport driven by Δμ_H⁺ across the cell membrane. (5) Neither the rate of respiration nor the intracellular level of ATP were significantly decreased by any of these inhibitors (except for venturicidin). (6) We conclude that in Rhodotorula gracilis the difference of the electrochemical potential of H⁺ is created by an electrogenic proton pump, presumably in ATPase. The extrusion of protons in exchange against potassium is catalyzed by a different energy-dependent but electroneutral system. This conclusion is based on the observation that the H⁺/K⁺ exchange does not work under conditions where the membrane potential is large, and vice versa.     

THE GENETIC CONSEQUENCES OF WORKER ANT POLLINATION IN A SELF-COMPATIBLE,CLONAL ORCHID

The self-compatible orchid Microtis parviflora is pollinated by the flightless worker caste of the ant Iridomyrmex gracilis. The orchid is clonal and forms small patches, usually less than 1 m², of disconnected individual ramets. Ant pollinators visited and revisited a limited proportion of available inflorescences, and 40% of all flower visits occurred within plants promoting self-pollination. Pollen labels indicated that self-pollination accounted for 51% of the pollen transfers, although pollen carryover extended beyond 16 flowers on 2 or 3 inflorescences. The distribution of ant movements between plants was leptokurtic with a mean of 12.4 ± 14.9 cm and a maximum of 89 cm, but a high proportion of movements were within clones accentuating the level of self-pollination. However, some pollen transfers between inflorescences of unlike genotypes contributed to a low incidence (max = 8%) of outcrossing. In 12 patches examined by electrophoresis, the density varied from 11 to 61 inflorescences per m² and a maximum of only 4 genotypes were detected. Electrophoretic analysis revealed populations were highly inbred: only 23% (N = 17) of the loci were polymorphic and the mean gene diversity h, was 2.7%. Heterozygotes were observed in only one population given a mean fixation index F, of 0.982. These results reflect the combined effects of restricted ant foraging and clonality. Nevertheless, while ant foraging was restricted, some outcrossing occurred and in the absence of clonality it is likely that ant foraging would have yielded a mixed mating system similar to those reported for a wide array of insect pollinators. Given the ability of ants to generate pollen flow, the reasons for the rarity of ant pollination appear to lie elsewhere.     

Ultrastructural Study of Secondary Wall Formation in the Stem Fiber of Phyllostachys pubescens

Ultrastructural changes in secondary wall formation of Phyllostachys pubescens Mazel fiber were investigated with transmission electron microscopy. Fiber developed initially with the elongation of cells containing ribosomes, mitochondria and Golgi bodies in the dense cytoplasm. During the wall thickening, the number of rough endoplasmic reticulum and Golgi bodies increased apparently. There were two kinds of Golgi vesicles, together with the ones from endoplasmic reticulum formed transport vesicles. Many microtubules were arranged parallel to the long axis of the cell adjacent to the plasmalemma. Along with the further development of fiber, polylamellate structure of the secondary wall appeared, with concurrent agglutination of chromatin in the nucleus, swelling and disintegration of organelles, while cortical microtubules were still arranged neatly against the inner side of plasmalemma. Lomasomes could be observed between the wall and plasmalemma. The results indicated that the organelles, such as Golgi bodies together with small vesicles, rough endoplasmic reticulum and lomasomes, played the key role in the thickening and lignification of the secondary wall of bamboo fiber, though cortical microtubules were correlative with the process as well.