STEROLS OF DICTYOCHA FIBULA (CHRYSOPHYCEAE) AND OLISTHODISCUS LUTEUS (RAPHIDOPHYCEAE)1

Sterols from cultured Dictyocha fibula Ehrenberg and Olisthodiscus luteus Carter were extracted and identified for comparison with sterols from other Chromophycota species. Although orientation at C-24 was not absolutely determined, the sterols of Dictyocha, a silicoflagellale, appeared to consist of only 24-methyl-22-dehydrocholesterol and 24-methylenecholesterol, a sterol composition not known in any other alga. This is in keeping with the taxonomic isolation Dictyocha has among algae. On the other hand, Olisthodiscus luteus contained 24-ethylcholesterol, 24-ethylcholestanol, 24-methylcholesterol, and cholesterol. This composition is in accord with sterols of members of the Xanthophyceae and Raphidophyceae.     

大鼠大脑皮层细胞核体外转录模型

本文用改良的 Giuffrida法分离纯化大鼠大脑皮层细胞核,产率为41—52％,具有很高的体外转录活性。参照Blatti硫酸铵浓度法建立了大鼠大脑皮层细胞核体外转录模型,能分别测定真核基因三类 RNA聚合酶转录活性,并对有关问题进行了讨论,指出本系统具有操作简便、省时、省实验材料等优点,适用于大脑皮层细胞核体外转录调控的研究。     

OLISTHODISCUS LUTEUS (CHRYSOPHYCEAE). III. UPTAKE AND UTILIZATION OF NITROGEN AND PHOSPHORUS1

Uptake and assimilation of nitrogen and phosphorus were studied in Olisthodiscus luteus Carter. A diel periodicity in nitrate reductase activity was observed in log and stationary phase cultures; there was a 10-fold difference in magnitude between maximum and minimum rates, but other cellular features such as chlorophyll a, carbon, nitrogen, C:N ratio (atoms) · cell^?1 were less variable. K_s values (~2 μM) for uptake of nitrate-N and ammonium-N were observed. Phosphorus assimilated · cell^?1· day^?1 varied with declining external phosphorus concentrations; growth rates <0.5 divisions · day^?1 were common at <0.5 μM PO_4-P. Phosphate uptake rates (K_s= 1.0–1.98 μM) varied with culture age and showed multiphasic kinetic features. Alkaline phosphatase activity was not detected. Comparisons of the nutrient dynamics of O. luteus to other phytoplankton species and the ecological implications as related to the phytoplankton community of Narragansett Bay (Rhode Island) are discussed.     

OLISTHODISCUS LUTEUS (CHRYSOPHYCEAE) I. EFFECTS OF SALINITY AND TEMPERATURE ON GROWTH. MOTILITY AND SURVIVALS1, 2

The effect of salinity and temperature on Olisthodiscus luteus Carter has been examined to across the relative importance of these factory on dynamics of natural population. A salinity range 2–50% was observed with increased tolerance to low salinity (<5%.) at higher temperature (20–30°C). Slinities at 4–5%. Had densities of 10³ cells/ml^?1, and growth >0.5 division day^?1 at temperature of 15–30°C higher salinities (5–50%.) variable but distinct optima for density, growth and motility were observed 5, 10 and 30°C. Density and motility showed no clear optima from 10–10%.15–25°C where maximum growth rates >1.0 division/day^?1 were common. Temperature increased from (0.5–1.9 division. Day^?1) and increases of three orders of magnitude (10^2?10³) for maximum densities. Temperature optima 20°C for growth 5–35%. And 25°C for >40%. were observed. The implications of these findings to natural populations of O. luleus are discussed.     

THE ISOLATION OF CELL NUCLEI FROM RAT BRAIN

A method for preparing highly pure cell nuclei from adult rat brain, using both differential and isopycnic centrifugation in sucrose media, is described. The morphology of these preparations was examined by both phase contrast and electron microscopy. The isolated nuclei retained many aspects of their in situ morphology; in particular, the nuclear envelope was double layered and interrupted by pore-like discontinuities, and the nucleoli consisted of irregular masses of densely packed granules. Analyses of these nuclear preparations for cytochrome oxidase and cholinesterase activity, as well as RNA/DNA ratio, indicated minimal contamination with mitochondria and microsomes. Problems involving the homogenization technique, choice of ionic conditions in the homogenization medium, and choice of optimal density of the sucrose solution used for the final purification of nuclei are discussed. Results of application of the technique to isolation of adult rat liver nuclei are also reported.     

THE ROLE OF ZINC FINGER PROTEIN IN RNAi INTERFERENCE IN A UNICELLULAR GREEN ALGA CHLAMYDOMONAS REINHARDTII (CHLOROPHYCEAE)

In our previous study, we generated a strain of 19‐P (1030) in which artificial RNA interference (RNAi) was induced by transcribing a hairpin RNA of ~780‐bp stem. We utilized this RNAi‐induced strain to uncover RNAi‐related genes. Random insertional mutagenesis was performed to generate tag‐mutants that show a RNAi deficient phenotype. The 92‐12C is one such tag‐mutant, which bears a 14‐kb deletion in chromosome 1. Complementation of 92‐12C revealed that a protein gene, including a Cys‐Cys‐Cys‐His‐type zinc finger motif and an ankyrin repeat motif, is essential for effective RNAi in Chlamydomonas reinhardtii (Dangeard). BLAST analysis revealed that the zinc finger protein is homologous to an mRNA splicing‐related protein of other species. Therefore, one of the probable scenarios is that mRNA coding for RNAi‐related proteins cannot be properly spliced, which causes RNAi deficiency in the 92‐12C tag‐mutant.     

ADAPTATION OF THE UNICELLULAR ALGA DUNALIELLA PARVA TO A SALINE ENVIRONMENT1

The holophilic alga Dunaliella parva produces glycerol as a major product of photosynthetic ¹⁴CO₂ incorporation and accumulates very large amounts of intracellular glycerol. A method was adopted for the determination of the cell water space based on the distribution of ¹⁴C sorbitol and ³H₂O between the cells and the medium. Using these measurements the internal concentration of glycerol was found to be isoomotic with that of the medium over a broad range of 0.6 to 2.1 m NaCl. When the extracellular salt concentration of an algal suspension was increased or decreased, the intracellular water content immediately varied so as to keep an osmotic equilibrium between the cells and the medium. During the following 90 min under metabolic conditions, glycerol content changed until a new level was reached. Since no leakage of intracellular glycerol was observed above 0.6 m NaCl, these alterations in glycerol content are interpreted as due to metabolic formation and degradation of intracellular glycerol. Determination of the glycerol sensitivity of enzymic and photosynthetic reactions of cell-free preparations from D. parva showed a broad range of tolerance to high concentrations of glycerol. These results indicate that osmoregulation in Dunaliella depends on the synthesis or degradation of intracellular glycerol in response to the external salt concentration. A proposed scheme of glycerol synthesis in Dunaliella is suggested.     

OLSTHODISCUS LUTEUS (CHRYSOPHYCEAE) II. FORMATION AND SURVIVAL OF A BENTHIC STAGE1

Motile unicells of Olisthodiscus lutheus Carter aggregated to form encapsulated masses of nonmotile cells in a benthic stage throughout a temerature range of 15–30°C at salinities o f 10–50%. Motile cells were released from beneathic masses at 10–30°C but at 5°C, cells were not motile and at 0°C cells lysed. Exposure of benthic masses of I day to 8 wk to temperatures of 0–30C in lighted growth chambers resulted in mortality to cells kept below 10°C and normal growth at higher temperatures. Benthic stage cells kept tn darkness at the same temperatures exhibited mortality in all but those at 5 and 10°C. Cells at these thmoeratures remained viable 15 wk in continual darkness. Comparison of cell morphology of matile and benthic stage O. luteus to other Olisthodiscus species and the ecological implications o fthe benthic stage are discussed.     

PROTEOMICS OF THE RED ALGA,GRACILARIA CHANGII (GRACILARIALES,RHODOPHYTA)1

The application of proteomics in alga research is still quite limited. The present report describes the establishment of the proteome of a red alga of economic importance, Gracilaria changii (Xia et Abbott) Abbott, Zhang et Xia. Initially, four protein extraction methods including direct precipitation by trichloroacetic acid/acetone, direct lysis using urea buffer, Tris buffer, and phenol/chloroform extraction were compared for their suitability to generate G. changii proteins for two‐dimensional gel electrophoresis (2‐DE). The phenol/chloroform protein extraction method gave the best 2‐DE resolution of the proteins. Using these 2‐DE gels and mass spectrometry, several proteins including pigment proteins, metabolic enzymes, and ion transporters were identified. These findings highlight the potential of using proteomic approaches for the investigation of G. changii protein function.     

NUCLEAR BASIC PROTEINS FROM THE BINUCLEATE DINOFLAGELLATE PERIDINIUM FOLIACEUM (PYRROPHYTA)1

Histories of the endosymbiont nucleus of the binucleate dinoflagellate Peridinium foliaceum Stein were prepared from isolated nuclei and analyzed by peptide mapping, ammo acid composition, and two-dimensional gel electrophoresis. Using these criteria, we identified the presence of two HI-like histories and the core histones H3, H2A, H2B, and H4. These histones are similar but not identical to those of the endosymbiont nucleus of the bi-nucleate dinoflagellate Peridinium balticum Levander.     

CHARACTERIZATION OF A RABE (RAS GENE FROM RAT BRAIN E) GTPASE EXPRESSED DURING MORPHOGENESIS IN THE UNICELLULAR GREEN ALGA MICRASTERIAS DENTICULATA (ZYGNEMATOPHYCEAE,STREPTOPHYTA)1

Rab GTPases are central regulators of cell shape in land plants by coordinating vesicle trafficking during morphogenesis. To date, relatively little is known about the role of these ubiquitous signaling proteins during cell growth in microalgae, in particular in the related charophyte algae. This article identifies the first charophyte Rab GTPase, MdRABE1, in Micrasterias denticulata Bréb., a convenient model organism for studying morphogenesis. Its expression correlated with the onset of morphogenesis, and structural analysis indicated that it belongs to the RABE (Ras gene from rat brain E) subclass. Confocal fluorescence and immunoelectron microscopy (IEM) of transiently GFP‐MdRABE1 overexpressing interphase cells demonstrated that the GFP‐MdRABE1 protein was localized to the endoplasmic reticulum, dictyosomes, exocytotic vesicles, the cell margin, the membranes of cell organelles, and in the isthmus zone around the nucleus. Although overexpression phenotyping of both N‐ and C‐terminal green fluorescent protein (GFP) fusions failed to indicate additional functional evidence of the MdRABE1 protein due to mortality of those transgenic cells, its expression profile, bioinformatics, and intracellular localization suggest a role in vesicle trafficking during morphogenesis.     

PARTIAL CHARACTERIZATION OF THE CHLOROPLAST GENOME FROM THE CHROMOPHYTIC ALGA SYNURA PETERSENII (SYNUROPHYCEAE)1

Hoechst dye 33258-CsCl density gradients were used to isolate two satellite DNA species from Synura petersenii Korsh. sensu lato, a member of the Synurophyceae. One satellite DNA was identified as the chloroplast genome. The chloroplast genome is the smallest (91.5 kb) published for any chromophyte and approximates the size of the smallest functional chlorophyte chloroplast genome (Codium fragile, 89 kb). The second satellite DNA was small (34.5 kb), and its origin is undetermined. The potential of using the S. petersenii chloroplast genome in comparative studies for evaluating organellar evolution and algal systematics is discussed.     

人头发DNA的提取及其基因扩增

头发是犯罪现场最容易得到的材料之一。本文报道从人的头发中提取DNA的方法以及利用PCR(聚合酶链反应)技术,从少量人发DNA扩增大量拷贝数的基因片段。对基因扩增得到的大量基因片段进行进一步的基因分析,将为法医物证学提供客观证据,具有重要价值。     

THE TOCOPHEROL,VITAMIN K,AND RELATED ISOPRENOID QUINONE COMPOSITION OF A UNICELLULAR RED ALGA (PORPHYRIDIUM CRUENTUM)1

The total lipids of axenically cultivated cells of Porphyridium cruentum were extracted with aqueous methanol-chloroform mixture and fractionated into neutral and polar lipids by silicic acid column chromatography. Thin-layer and reversed-phase paper chromatographic analyses of the neutral lipid fractions revealed the occurrence of plastoquinones (PQ) A and C, vitamin K₁ (K), ubiquinone-10 (Q₁₀), α-tocopherol (α-T), and α-tocopherolquinone (α-TQ) in the photoautotrophically cultured alga, and the same quinones but no tocopherol in the alga grown photoheterotrophically on glycerol. The plastoquinone A and vitamin K₁ were isolated, identified, and estimated by spectroscopic methods. The results indicated the following decreasing order of concentrations: autotrophic culture, PQ A > K > Q₁₀ > PQ C, α-TQ, α-T; heterotrophic culture, PQ A > Q₁₀ > K > PQ C, α-TQ. Except for the absence of plastoquinone B, the overall quinonoid composition was in general agreement with those previously reported for multicellular members of Rhodophyta, but the concentration level in total lipid was markedly lower.