Fluorescent probe studies of mixed micelles of phospholipids and bile salts. Effect of cholesterol incorporation

The binding of the fluorescent alkylamines, $\text{N-(2-}\text{aminoethyl}\text{)-5-}\text{dimethylamino-1-naphthalene}$ sulfonamide, $\text{N-(5-}\text{aminopentyl}\text{)-5-}\text{dimethylamino-1-naphthalene}$ sulfonamide (dansyl cadaverine) and $\text{N-(10-}\text{aminodecyl}\text{)-5-}\text{dimethylamino-1-napthalene}$ sulfonamide with phospholipid and phospholipid-deoxycholate micelles, has been shown to increase with the length of the alkyl spacer chain. The probes bind more effectively to micelles containing unsaturated phospholipids and do not interact strongly with bile salt solutions at low concentrations. Cholesterol incorporation into mixed micelles results in a quenching of probe fluorescence due to displacement of probe molecules. The enhanced rigidity of the mixed micelles on solubilizing cholesterol is established by a decrease in pyrene excimer fluorescence and by the less effective perturbation of the micellar structure by 1-anilino-8-naphthalene sulfonate. The anionic probe 1-anilino-8-naphthalene sulfonate is also displaced from the mixed micelles when cholesterol is incorporated, suggesting a dominant role for packing and hydrophobic effects in binding both positively and negatively charged probes.     

Relation between algal available phosphate in the sediments of the River Garonne and chemically-determined phosphate fractions

Concentrations of total and inorganic phosphate were measured in forty-seven sediments of the River Garonne (France) using an anion resin, NaOH 0.1 M, Ca-NTA and Na-EDTA. Algal available P was measured using Scenedesmus crassus. The sediments presented a wide range of Tot-P concentrations (226 to 923 μg g⁻¹). Resin P varied between 1.1 to 55.5 μg g⁻¹ and NaOH-P between 3.5 to 262 μg g⁻¹. NTA-P and EDTA-P varied between 13.9 and 178 μg g⁻¹ and between 14.4 to 261 μg g⁻¹ respectively. Algal available P varied between 8.8 to 262 μg g⁻¹/ All forms of P are highly correlated and specially with algal available P (r = 0.70, 0.77, 0.88 and 0.77 for resin-P, NaOH-P, NTA-P and EDTA-P respectively). Nevertheless the partial correlation between EDTA-P and algal available P dropped to 0.05 when the concentration of NTA-P was considered as constant, indicating a spurious correlation with apatitic phosphate (extracted by Na-EDTA). Because of the strongest R ² and the lowest standard error of estimate, phosphate extracted by Ca-NTA can be considered as the best predictor of algal available phosphate.     

酿酒酵母HAL1基因的克隆及植物表达载体的构建

HAL1基因是酵母中重要的耐盐基因。以酿酒酵母AS2.375菌株的DNA为模板,根据已发表的序列设计引物,经PCR扩增得到约900 bp的HAL1基因片段,连接到pMD18-T载体上,转化大肠杆菌JM109,筛选重组质粒进行酶切分析和序列测定,结果显示已克隆到完整的可读框,该基因的序列与已知序列同源性达99%。将HAL1基因从T-载体上切下连接到pAM194载体上构建了HAL 1基因的植物表达载体,用于烟草的转化获得了耐盐性提高的转化植株。     

Expression in Escherichia coli of Three Different Soybean Late Embryogenesis Abundant （LEA） Genes to Investigate Enhanced Stress Tolerance

In order to identify the function of late embryogenesis abundant (LEA) genes, in vitro functional analyses were performed using an Escherichia coli heterologous expression system. Three soybean late embryogenesis abundant (LEA) genes, PMll (GenBank accession No. AF004805; group 1), PM30(AF117884; group 3), and ZLDE-2 (AY351918; group 2), were cloned and expressed in a pET-28a system.The gene products were separated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and identified by mass spectrometry. E. coli cells containing the recombinant plasmids or empty vector as controls were treated by salt and low temperature stress. Compared with control cells, the E. coli cells expressing either PMll or PM30 showed a shorter lag period and improved growth when transferred to LB (Luria-Bertani) liquid media containing 800 mmol/L NaC1 or 700 mmol/L KC1 or after 4℃ treatment. E. coli cells expressing ZLDE-2 did not show obvious growth improvement both in either high KC1 medium or after 4℃ treatment. The results indicate that the E. coli expression system is a simple, useful method to identify the functions of some stress-tolerant genes from plants.