Flotation of lipid-protein particles containing triacylglycerol and phospholipid from the cytosol of carnation petals

Lipid-protein particles ranging from 20 to 250 nm in diameter have been isolated from the cytosol of carnation petals by flotation centrifugation and also by ultrafiltration. The cytosolic lipid-protein particles resemble oil bodies, lipid-protein particles found in oil-bearing seeds, in that they contain triacylglycerol, are circumscribed by phospholipid that is not organized in a bilayer, appear to be derived from membranes and can be isolated by flotation. However, the cytosolic particles are distinguishable from oil bodies in that triacylglycerol is not the dominant lipid. Indeed, they contain a spectrum of lipids in addition to phospholipids and triacylglycerol including free fatty acids, sterol and wax esters, phosphatidic acid and diacylglycerol. These same lipids are present in corresponding microsomal membranes as well, but in much smaller proportions relative to phospholipid. The lipid-protein particles from carnation petals contain a 17-kDa protein that is of similar size to oil body oleosin, but does not cross-react with anti-oleosin antibodies. The data indicate that these cytosolic particles are structurally and chemically similar to oil bodies and are consistent with the notion that their genesis may be a means of removing destabilizing lipids from membrane bilayers.     

Preferential regeneration of the NADPH: protochlorophyllide oxidoreductase oligomer complexes in pea epicotyls after bleaching

The regeneration and stability of the NADPH:protochlorophyllide oxidoreductase (POR, EC 1.3.1.33) enzyme complexes were studied in bleached epicotyls of 9-day-old dark-germinated pea ( Pisum sativum L. cv. Zsuzsi) seedlings. Middle segments were illuminated with 1300 µmol m⁻² s⁻¹photon flux density (PFD) white light and subsequently incubated in total darkness for 4–24 h at 24°C. Almost the full amount of protochlorophyllide (Pchlide) was degraded after 60 min illumination. The preferential regeneration of the 655 nm emitting Pchlide form was observed after 4 h dark incubation; the accumulation of the short-wavelength Pchlide form—dominating in epicotyls of dark-grown seedling—required 18–24 h dark. The Pchlide content of bleached samples was around 2.5% of that of the etiolated samples; after 4 h of dark incubation this value increased to 4–7%. Polyacrylamide gel electrophoresis and western blot showed that the amount of the POR protein decreased to about 50% during bleaching; after 4 h regeneration it reached almost the same level as that of dark-grown samples. We concluded that much more POR protein compared with Pchlide pigment remained stable during bleaching and the non-destroyed POR units were able to form preferentially oligomers during the dark-regeneration which could collect de novo synthesized Pchlide into 655 nm emitting complexes. These data indicate the high stability of the POR protein in pea epicotyls and the importance of the molecular environment in stimulating the aggregation of POR units.     

Pervaporation-aided enzymatic esterifications in non-conventional media

This paper focuses on enzymatic esterifications in non-conventional media (organic solvents, ionic liquids, and solvent-free systems) with reference to the water removal. Different types of water removal techniques are reviewed with a special emphasis on pervaporation. Pervaporation is a separation process in which liquid is transported through a selective membrane with simultaneous evaporation of permeates. In an integrated process where pervaporation is coupled with a bioreactor where esterification is performed, selective removal of water or other esterification products can be achieved. In this manner benefit can be doubled, due to the equilibrium shift and possible pure product recovery. Available literature on esterifications coupled with pervaporation is presented in detail. Reviewed examples are divided according to the type of reaction media.     

Geographical dispersion of ragweed leaf beetle (Ophraella communa) based on climatic and biological characters in the Palearctic habitats

1. The accidentally introduced ragweed leaf beetle (Ophraella communa) is a most promising biological control agent for common ragweed (Ambrosia artemisiifolia), which herbivore has already emerged in several areas of the Palearctic region.
2. The aim of our study was to model the expansion of O. communa and the number of generations in the various Palearctic regions. Furthermore, our objective was to determine the effect of the prevailing wind on the direction of its spread and to ascertain the relationship between the green biomass production of ragweed and individual numbers of this leaf beetle.
3. According to our meta-analytical findings, the advancement of O. communa is continuous in the Palearctic areas. This phytophagous insect invades new habitats, which are occupied by A. artemisiifolia, and spreads quickly. The stable populations of O. communa seem to be strictly linked to the presence of its primary host, A. artemisiifolia.
4. We show that the rapid spread of this insect is due to the combination of wind direction and topography features, which was reinforced by our analysis. O. communa possesses uniformly multivoltine populations in its Palearctic habitats. So, insects possessing facultative diapause are able to colonize northern areas depending on the presence of their host, which statement is based on the processing of 143 East- and 68 West-Palearctic records
5. According to our investigations, the mass appearance of this phytophagous insect coincided with the assimilation peak of its main host, common ragweed.

     

Metal binding ability of hypermodified nucleosides of t-RNA. Potentiometric and spectroscopic studies on the metal complexes of N-[(9-β-D-ribofuranosylpurin-6-yl)carbamoyl] threonine

Copper(II), nickel(II), zinc(II), manganese(II), and magnesium(II) complexes of t⁶A (N-[9-β-D-ribofuranosylpurin-6-yl)carbamoyl] threonine and t⁶Ade (N⁶(threoninocarbonyl)adenine) were studied by potentiometric and spectroscopic methods. It was found that t⁶Ade has three dissociable protons in the accessible pH range (N¹ and N⁹ of purine and carboxylate), while only two pK values are characteristic of t⁶A. Magnesium(II) and manganese(II) do not interact effectively with these ligands, but copper(II) and nickel(II) ions form very stable complexes with the coordination of purine N¹, deprotonated amide nitrogen, and carboxy late oxygen donors.     

Crystal structure of the nucleotide‐metabolizing enzyme NTPDase4

The ecto‐nucleoside triphosphate diphosphohydrolases (NTPDases) are a family of enzymes found on the cell surface and in the lumen of certain organelles, that are major regulators of purinergic signaling. Their intracellular roles, however, have not been clearly defined. NTPDase4 (UDPase, ENTPD4) is a Golgi protein potentially involved in nucleotide recycling as part of protein glycosylation, and is also found in lysosomes, where its purpose is unknown. To further our understanding of NTPDase4 function, we determined its crystal structure. The enzyme adopts a wide open, inactive conformation. Differences in the nucleotide‐binding site relative to its homologs could account for its substrate selectivity. The putative membrane‐interacting loop of cell‐surface NTPDases is drastically altered in NTPDase4, potentially affecting its interdomain dynamics at the Golgi membrane.     

Challenges of unculturable bacteria: environmental perspectives

Reviews in Environmental Science and Bio/Technology - Environmental biotechnology offers several promising techniques for the rehabilitation of polluted environments. The modern industrialized...     

Synthesis and antibody recognition of synthetic antigens from MUC1.

In the altered form of MUC1 mucin associated with breast cancer, the highly immunogenic sequence PDTRPAP is exposed, and may be an immunologically relevant target for the development of diagnostics or cancer immunotherapy. In this study, we report the preparation and antibody binding properties of monomeric and dimeric MUC1 peptides containing the epitope region recognized by monoclonal antibody (mAb) C595. Peptides contained a single or two copies of the whole 20-mer repeat unit (VTSAPDTRPAPGSTAPPAHG) of MUC1 protein. MUC1 40-mer peptides were prepared by the condensation of semi-protected fragments of the repeat unit, in solution or by chemical ligation. In the first case, cyclohexyl-type protecting groups were used for the synthesis of semi-protected fragments by the Boc/Bzl strategy. Unprotected fragments were used in the chemical ligation to produce thioether linkages. In one of the fragments, a Gly residue was replaced by Cys at the C-terminus and the other fragment was chloroacetylated at the N-terminus. In addition, the short peptide APDTRPAPG, and its disulfide dimer, (APDTRPAPGC)(2) were produced. The antibody binding properties of these MUC1 peptide constructs were tested by competition enzyme-linked immunosorbent assay (ELISA). The short epitope region peptide, APDTRPAPG and its dimer (APDTRPAPGC)(2) showed higher IC(50) values (IC(50) = 56.3 and 53.2 micromol/l, respectively). While the 20-mer peptide (IC(50) = 25.9 micromol/l) and more markedly its 40-mer dimers (IC(50) = 0.62 and 0.78 micromol/l) were recognized better. CD data obtained in water or in TFE indicated no significant conformational differences between the 20-mer and 40-mer peptides. We found a high level of similarity between the binding properties of the 40-mer peptides with amide or thioether links, providing a new possibility to build up oligomeric MUC1 peptides by thioether bond formation.