Chemical forms of zinc in light chestnut soil under mono- and multielement types of pollution

Chemical forms of zinc in light chestnut soil polluted by zinc, copper, cadmium, and lead, introduced separately or jointly, were studied. A change in the initial relations between the element forms was found for all types of pollution. An increase in pollution of any type led to the accumulation of the most mobile forms of zinc in the soil. It was revealed that ion exchange is of the greatest significance in the fixation of zinc in polluted soil.     

Interaction of Tetrahydrocortisol–Apolipoprotein A-I Complex with Eukaryotic DNA and with Single-Stranded Oligonucleotides

The complex formed by tetrahydrocortisol (THC) and apolipoprotein A-I (ApoAI) specifically interacts with eukaryotic DNA from rat liver. Taken together, physical and chemical data and the results of small-angle X-ray scattering analysis show that interaction of the THC–ApoAI complex with eukaryotic DNA results in deformation of the DNA double helix. Single-stranded fragments were demonstrated to cause deformation of the double helix. In this state DNA forms complexes with DNA-dependent RNA polymerase. This interaction is cooperative and of saturating type; up to six enzyme molecules bind with one DNA molecule. The putative site of complex binding with DNA is the sequence CC(GCC)_n found in many genes including the human ApoAI gene. An oligonucleotide of this type was synthesized. Its association constant (K _a) was 1.66·10⁶ M^–1. Substitution of THC with cortisol considerably decreases the K _a. We suggest that THC interacting with GC pairs of the binding site forms hydrogen bonds with cytosine, inducing rupture of the bonds within the complementary nucleic base pair.     

Effect of combined glucocorticoids and low density lipoproteins on structural and functional changes in hepatocytes and Kupffer cells

The combined action of cortisol and low density lipoproteins (LDL) on the hepatic cell functional activity associated with protein biosynthesis was investigated by biochemical, radioisotope, and ultrastructural methods. The preferential uptake from blood serum of high and low density lipoproteins and glucocorticoids in vivo is enhanced, when residential macrophages are stimulated by prodigiozanum belonging to lipopolysaccharides (LPS). Liver macrophages actively take up colloidal gold (labeled LDL) by receptor-mediated endocytosis. The labels are followed in endosomes and lysosomes of Kupffer cells, and in Disse's space, though there are only single granules in hepatocytes. It is suspected that products of glucocorticoid chemical modification (tetrahydrosubstances) and LDL of limited proteolysis, while entering hepatocytes, may co-operatively activate their nucleolar DNA, that manifests in the increase in nucleolar dimensions and relative volume of granular component in them. In the cytoplasm, the density of ribosomes on the rough ER membranes significantly grows, the relative volume of the smooth ER and the number of primary lysosomes increase. In the co-culture of hepatocytes and Kupffer cells under the combined influence of cortisol, LDL and LPS, the protein biosynthesis considerably accelerates. One may suppose that LDL, on transporting steroid hormones and lipophilic xenobiotics into hepatic cells, may take part in the induction of lysosomal and monooxygenase oxidative system enzymes attributed to smooth ER.     

Tetrahydrocortisol-apolipoprotein A-I complex specifically interacts with eukaryotic DNA and GCC elements of genes

Tetrahydrocortisol stimulates DNA and protein biosynthesis in hepatocytes only when it enters the complex with apolipoprotein A-I. Tetrahydrocortisol–apolipoprotein A-I (THC–apoA-I) complex specifically interacts with eukaryotic DNA isolated from rat liver. In the process of interaction, rupture of hydrogen bonds between the pairs of nitrous bases occurs with the formation of single-stranded DNA structures. In such state DNA forms complexes with DNA-dependent RNA-polymerase. The most probable site of binding the tetrahydrocortisol–apolipoprotein A-I complex with DNA is the sequence of CC(GCC)_n type entering the structure of many genes, among them the structure of human apolipoprotein A-I gene. Oligonucleotide of this type has been synthesized. Association constant (K_ass) of it with tetrahydrocortisol–apolipoprotein A-I complex was shown to be 1.66×10⁶ M⁻¹. Substitution of tetrahydrocortisol for cortisol in the complex results in a considerable decrease of K_ass. It was assumed that in the GC-pairs of the given sequence tetrahydrocortisol itself participates in the formation of hydrogen bonds with cytosine, favoring their rupture with complementary base—guanine.     

Functional characterization of Drosophila sialyltransferase

Sialylation is an important carbohydrate modification of glycoconjugates in the deuterostome lineage of animals. By contrast, the evidence for sialylation in protostomes has been scarce and somewhat controversial. In the present study, we characterize a Drosophila sialyltransferase gene, thus providing experimental evidence for the presence of sialylation in protostomes. This gene encodes a functional alpha2-6-sialyltransferase (SiaT) that is closely related to the vertebrate ST6Gal sialyltransferase family, indicating an ancient evolutionary origin for this family. Characterization of recombinant, purified Drosophila SiaT revealed a novel acceptor specificity as it exhibits highest activity toward GalNAcbeta1-4GlcNAc carbohydrate structures at the non-reducing termini of oligosaccharides and glycoprotein glycans. Oligosaccharides are preferred over glycoproteins as acceptors, and no activity toward glycolipid acceptors was detected. Recombinant Drosophila SiaT expressed in cultured insect cells possesses in vivo and in vitro autosialylation activity toward beta-linked GalNAc termini of its own N-linked glycans, thus representing the first example of a sialylated insect glycoconjugate. In situ hybridization revealed that Drosophila SiaT is expressed during embryonic development in a tissue- and stage-specific fashion, with elevated expression in a subset of cells within the central nervous system. The identification of a SiaT in Drosophila provides a new evolutionary perspective for considering the diverse functions of sialylation and, through the powerful genetic tools available in this system, a means of elucidating functions for sialylation in protostomes.     

Activation of nucleolar DNA and ribosome biosynthesis in hepatocytes under the effect of glucocorticoids and high density lipoproteins

The structural bases of cooperative effect of glucocorticoids and HDL brings about the activation of protein biosynthesis in hepatocytes. Using surviving rat liver it was shown that these two compounds together activate the gene expression which was indicated by increased 3H-uridine incorporation into the total RNA pool. The enhanced incorporation of 14C-leucine into proteins in these experiments confirms protein biosynthesis acceleration. With the use of liver perfusion technique it was morphologically demonstrated that the earliest changes in hepatocyte genome take place in nucleoli. The increase of nucleolar dimensions and granular component reflects the activation of ribosomal precursors synthesis. Considerable number of ribosomes in the hepatocyte perinuclear space indicates their active transport across the numerous nuclear membrane pores into the cytoplasm. In the first place and more prominently in hepatocytes the protein synthesis "for export" is stimulated, which was proved by the dynamics of ribosome accumulation on the membranes of endoplasmic reticulum according the perfusion duration. The kupffer cells play a significant role in HDL transcytosis and in the realization of their cooperative effect with glucocorticoids.     

Evaluation of the binding of benzo-a-pyrene by blood serum lipoproteins using the cellulose disk method

A simple and convenient method has been developed for evaluation binding capacity of lipophilic ligands with lipoproteins or other transport proteins. For this purpose cellulose discs (Whatman 3 MM) were loaded with the constant quantity of 3H-benzopyrene and increasing amounts of unlabelled benzo[a]pyrene in dimethylsulfoxide, dried up and incubated in solution of lipoproteins. Dissociation constants were deduced from the remained disk radioactivity using the Scatchard plot method. The obtained values of the dissociation constants were: HDL--4.1 x 10(-5) M; LDL--1.5 x 10(-6) M; VLDL--8.8 x 10(-6) M.