Your search keyword '"S. B. Akopov"' showing total 20 results

1. Binding of Protein Factor CTCF within Chicken Genome Alpha-Globin Locus

Author

N. V. Petrova, Olga V. Iarovaia, S. B. Akopov, Sergey V. Razin, D. A. Didych, Lev G. Nikolaev, and E. S. Kotova

Subjects

0301 basic medicine, Chicken Cells, Biology, Biochemistry, Molecular biology, In vitro, DNA binding site, 03 medical and health sciences, Cell nucleus, chemistry.chemical_compound, 030104 developmental biology, 0302 clinical medicine, medicine.anatomical_structure, chemistry, CTCF, medicine, Molecular Medicine, Electrophoretic mobility shift assay, Molecular Biology, Chromatin immunoprecipitation, 030217 neurology & neurosurgery, DNA, Biotechnology

Abstract

A systematic search for DNA fragments containing potential CTCF transcription factor binding sites in the chicken alpha-globin domain and its flanking regions was performed by means of the two-dimension electrophoretic mobility shift assay. For the alpha-globin domain fragments selected, the occupancy by the CTCF in erythroid and lymphoid chicken cells was tested by chromatin immunoprecipitation. Only one of 13 DNA fragments capable of CTCF binding in vitro was efficiently bound to this protein in vivo in erythroid cells, and somewhat less efficiently - in lymphoid cells. So, binding of CTCF to the DNA fragment in vitro in most cases does not mean that this fragment will be occupied by CTCF in the cell nucleus. Yet, CTCF binding in vivo, as a rule, is accompanied by the binding of the protein to this DNA region in vitro. During the erythroid differentiation, no significant changes in CTCF binding to the DNA fragments studied were detected.

Published

2016

2. Expression of chicken CTCF gene in COS-1 cells and partial purification of CTCF protein

Author

I. V. Sorokina, Lev G. Nikolaev, S. B. Akopov, E. S. Kotova, and E.D. Sverdlov

Subjects

Cell Nucleus, CCCTC-Binding Factor, COS cells, Gene Expression, General Medicine, Biology, Biochemistry, Molecular biology, Repressor Proteins, Cell nucleus, chemistry.chemical_compound, medicine.anatomical_structure, chemistry, CTCF, COS Cells, Chlorocebus aethiops, Gene expression, medicine, Animals, Electrophoretic mobility shift assay, Polyhistidine-tag, Chickens, Transcription factor, Gene

Abstract

The chicken gene for transcription factor CTCF was expressed in COS-1 mammalian cells. The CTCF protein containing polyhistidine tag was partially purified using metallo-affinity and ion-exchange chromatography. The expressed protein localized in the cell nucleus and was shown to be functionally active in the electrophoretic mobility shift assay and specifically interacted with anti-CTCF antibodies.

Published

2013

3. Assay of insulator enhancer-blocking activity with the use of transient transfection

Author

N. A. Smirnov, D. A. Didych, S. B. Akopov, Eugene D. Sverdlov, and Lev G. Nikolaev

Subjects

animal structures, CHO Cells, beta-Globins, Biology, Transfection, Biochemistry, Genome, chemistry.chemical_compound, Cricetulus, Plasmid, Animals, Humans, Promoter Regions, Genetic, Enhancer, Regulation of gene expression, Genome, Human, Chinese hamster ovary cell, DNA, Hep G2 Cells, General Medicine, Molecular biology, Enhancer Elements, Genetic, chemistry, embryonic structures, Biophysics, Biological Assay, Insulator Elements, Human genome, Chickens, HeLa Cells, Plasmids

Abstract

We used a transient transfection of cultured cells with linearized plasmids to analyze the enhancer-blocking activity of potential insulators including the standard cHS4 chicken beta-globin insulator and several DNA fragments selected from the human genome sequence. About 60-80% of the potential insulators do reveal the enhancer-blocking activity when probed by the transient transfection assay. The activity of different sequences is characterized by certain tissue specificity and by dependence on the orientation of the fragments relative to the promoter. Thus, the transfection model may be used for quantitative analysis of the enhancer-blocking activity of the potential insulators.

Published

2013

4. Affinity capture of specific DNA fragments with short synthetic sequences

Author

V. K. Potapov, N. V. Amirkhanov, Lev G. Nikolaev, V. S. Mikhailov, R. N. Amirkhanov, Valentina F. Zarytova, S. S. Bulanenkova, S. B. Akopov, and Eugene D. Sverdlov

Subjects

chemistry.chemical_compound, Peptide nucleic acid, chemistry, Biochemistry, Oligonucleotide, Organic Chemistry, Bioorganic chemistry, Biology, Combinatorial chemistry, Strong binding, DNA

Abstract

The ability of short peptide nucleic acid (PNA) oligomers and oligonucleotides containing modified residues of 5-methylcitidine, 2-aminoadenosine, and 5-propynyl-2′-deoxyuridine (strong binding oligonucleotides, SBO) to affinity capture the target double-stranded DNA fragment from mixture by means of the end invasion was compared. Both types of probes were highly effective at the conditions used. The SBO-based probes may represent a handy and easily prepared alternative to PNA for selection of target DNA fragments in mixtures.

Published

2013

5. Identification of recognition sites for Myc/Max/Mxd network proteins by a whole human chromosome 19 selection strategy

Author

Therese Wahlström, S. B. Akopov, Igor P. Chernov, Marie Henriksson, G. Klein, M. B. Kostina, and Lev G. Nikolaev

Subjects

Genetics, Binding Sites, Base Sequence, Basic Helix-Loop-Helix Leucine Zipper Transcription Factors, Molecular Sequence Data, Intron, General Medicine, Plasma protein binding, Biology, Biochemistry, In vitro, Proto-Oncogene Proteins c-myc, Repressor Proteins, Genetic Techniques, In vivo, Cell Line, Tumor, Chromosome 19, Humans, Binding site, Chromosomes, Human, Pair 19, Gene, Transcription factor, Protein Binding

Abstract

In this study, we have identified 20 human sequences containing Myc network binding sites in a library from the whole human chromosome 19. We demonstrated binding of the Max protein to these sequences both in vitro and in vivo. The majority of the identified sequences contained one or several CACGTG or CATGTG E-boxes. Several of these sites were located within introns or in their vicinity and the corresponding genes were found to be up- or down-regulated in differentiating HL-60 cells. Our data show the proof of principle for using this strategy in identification of Max target genes, and this method can also be applied for other transcription factors.

Published

2008

6. [Untitled]

Author

A. N. Domansky, Eugene D. Sverdlov, S. B. Akopov, Lev G. Nikolaev, and Yu. B. Lebedev

Subjects

Genetics, Reporter gene, Polyadenylation, viruses, TATA box, Organic Chemistry, Human endogenous retrovirus K, Biology, Enhancer, Biochemistry, Gene, Genome, Long terminal repeat

Abstract

The transient expression of the luciferase reporter gene was used to detect the tissue-specific enhancer activity of the solitary extraviral long terminal repeat (LTR) of the human endogenous retrovirus K (HERV-K). The LTR was previously mapped to the 19q13.2 locus. It contains a number of potential regulatory elements including TATA box, binding sites for some nuclear factors, and a polyadenylation signal. However, an analysis of the genomic sequences close to the LTR did not reveal any known genes or the expressed sequences (EST), whose functioning could be regulated by this LTR. The enhancer activity can be preserved in the solitary LTR due to its involvement in the long-range control of genome functioning or by the absence of functional disruptive mutations within the human-specific LTR, because it is of a relatively young evolutionary age.

Published

2002

7. Identification and mapping of nuclear matrix-attachment regions in a one megabase locus of human chromosome 19q13.12: Long-range correlation of S/MARs and gene positions

Author

Lev G. Nikolaev, Igor P. Chernov, Eugene D. Sverdlov, and S. B. Akopov

Subjects

Genetics, Chromosome 19, Chromosome, Locus (genetics), Cell Biology, Mars Exploration Program, Biology, Scaffold/matrix attachment region, Nuclear matrix, Molecular Biology, Biochemistry, Gene, Genome

Abstract

The first draft human genome sequence now available allowed the identification of an enormous number of gene coding areas of the genomic DNA. However, a great number of regulatory elements such as enhancers, promoters, transcription terminators, or replication origins can not be identified unequivocally by their nucleotide sequences in complex eukaryotic genomes. One important subclass of these type of sequences is scaffold/matrix attachment regions (S/MARs) that were hypothesized to anchor chromatin loops or domains to the nuclear matrix and/or chromosome scaffold. We developed an experimental selection procedure to identify S/MARs within a completely sequenced one megabase (1 Mb) long gene-rich D19S208-COX7A1 locus of human chromosome 19. A library of S/MAR elements from the locus was prepared and shown to contain -20 independent S/MARs. Sixteen of them were isolated, sequenced, and assigned to certain positions within the locus. A majority of the S/MARs identified (11 out of 16) lie in intergenic regions, suggesting their structural role, i.e., delimitation of chromatin domains. These 11 S/MARs subdivide the locus into 10 domains ranging from 6 to 272 kb with an average domain size of 88 kb. The remaining five S/MARs were found within intronic sequences of APLP1, HSPOX1, MAG, and NPHS1 genes, and can be tentatively characterized as regulatory S/MARs. The correspondence of the chromatin domains defined by the S/MARs to functional characteristics of the genes therein is discussed. The approach described can be a prototype of a similar search of long sequenced genomic stretches and/or whole chromosomes for various regulatory elements.

Published

2002

8. Destabilase from the medicinal leech is a representative of a novel family of lysozymes

Author

Irena I. Artamonova, V.I. Kiseleva, I. P. Baskova, D.G. Kozlov, S.V. Benevolensky, A. V. Sass, S. A. Lukyanov, L. L. Zavalova, V.A. Nesmeyanov, A.M. Poverenny, S. B. Akopov, E. V. Snezhkov, E.D. Sverdlov, and V.S. Archipova

Subjects

DNA, Complementary, Molecular Sequence Data, Biophysics, Gene Expression, Leech, Sequence alignment, Saccharomyces cerevisiae, Biology, Biochemistry, Antibodies, Cell Line, Substrate Specificity, chemistry.chemical_compound, Structural Biology, Leeches, Carbon-Nitrogen Lyases, Endopeptidases, Escherichia coli, Animals, Gene family, Amino Acid Sequence, Molecular Biology, Gene, Peptide sequence, Caenorhabditis elegans, Genetics, biology.organism_classification, Isoenzymes, chemistry, Muramidase, Lysozyme, Baculoviridae, Sequence Alignment, Function (biology)

Abstract

Intrinsic lysozyme-like activity was demonstrated for destabilase from the medicinal leech supported by (1) high specific lysozyme activity of the highly purified destabilase, (2) specific inhibition of the lysozyme-like activity by anti-destabilase antibodies, and (3) appreciable lysozyme-like activity in insect cells infected with recombinant baculoviruses carrying cDNAs encoding different isoforms of destabilase. Several isoforms of destabilase constitute a protein family at least two members of which are characterized by lysozyme activity. The corresponding gene family implies an ancient evolutionary history of the genes although the function(s) of various lysozymes in the leech remains unclear. Differences in primary structures of the destabilase family members and members of known lysozyme families allow one to assign the former to a new family of lysozymes. New proteins homologous to destabilase were recently described for Caenorhabditis elegans and bivalve mollusks suggesting that the new lysozyme family can be widely distributed among invertebrates. It remains to be investigated whether the two enzymatic activities (isopeptidase and lysozyme-like) are attributes of one and the same protein.

Published

2000

9. Genes from the medicinal leech (Hirudo medicinalis) coding for unusual enzymes that specifically cleave endo-ɛ(γ-Glu)-Lys isopeptide bonds and help to dissolve blood clots

Author

S. B. Akopov, S. Berezhnoy, L. L. Zavalova, E. V. Snezhkov, I. P. Baskova, Ekaterina A. Bogdanova, S. A. Lukyanov, Ekaterina V. Barsova, and Eugene D. Sverdlov

Subjects

DNA, Complementary, Tissue transglutaminase, Molecular Sequence Data, Spodoptera, Protein Structure, Secondary, Cell Line, chemistry.chemical_compound, Protein structure, Protein sequencing, Leeches, Endopeptidases, Genetics, Animals, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, Peptide sequence, chemistry.chemical_classification, Base Sequence, Sequence Homology, Amino Acid, biology, Hydrolysis, Chromatography, Ion Exchange, biology.organism_classification, Recombinant Proteins, Amino acid, Isopeptidase activity, Hirudo medicinalis, chemistry, Biochemistry, biology.protein, Peptides, DNA

Abstract

We previously detected in salivary gland secretions of the medicinal leech (Hirudo medicinalis) a novel enzymatic activity, endo-epsilon(gamma-Glu)-Lys isopeptidase, which cleaves isopeptide bonds formed by transglutaminase (Factor XIIIa) between glutamine gamma-carboxamide and the epsilon-amino group of lysine. Such isopeptide bonds, either within or between protein polypeptide chains are formed in many biological processes. However, before we started our work no enzymes were known to be capable of specifically splitting isopeptide bonds in proteins. The isopeptidase activity we detected was specific for isopeptide bonds. The enzyme was termed destabilase. Here we report the first purification of destabilase, part of its amino acid sequence isolation and sequencing of two related cDNAs derived from the gene family that encodes destabilase proteins, and the detection of isopeptidase activity encoded by one of these cDNAs cloned in a baculovirus expression vector. The deduced mature protein products of these cDNAs contain 115 and 116 amino acid residues, including 14 highly conserved Cys residues, and are formed from precursors containing specific leader peptides. No homologous sequences were found in public databases.

Published

1996

10. Functional dissection of an enhancer-like element located within the second intron of the human U2AF1L4 gene

Author

D. A. Didych, Eugene D. Sverdlov, S. B. Akopov, N. A. Smirnov, E. S. Kotova, and Lev G. Nikolaev

Subjects

Genetics, Reporter gene, Base Sequence, Molecular Sequence Data, Intron, Nuclear Proteins, Enhancer RNAs, General Medicine, Biology, Splicing Factor U2AF, Biochemistry, Introns, Conserved sequence, Evolution, Molecular, Enhancer Elements, Genetic, Ribonucleoproteins, Genes, Reporter, Enhancer trap, Humans, Human genome, Enhancer, Gene, Conserved Sequence, HeLa Cells, Protein Binding

Abstract

A detailed functional and evolutionary analysis of an enhancer element of the human genome (enhancer 12) located in the second intron of the U2AF1L4 gene, which we identified earlier, is presented. Overlapping fragments of the studied genome region were analyzed for enhancer activity, and the site responsible for the activity of this element was identified using transient transfections of HeLa cells. Comparison of the enhancer 12 sequence with orthologous sequences from seven primate species revealed the existence of evolutionarily conserved sequences within this element. One of the identified conservative regions is likely responsible for the enhancer activity and is able to specifically interact in vitro with proteins of HeLa cell nuclear extract. The ability of orthologous primate sequences to compete with enhancer 12 for binding with HeLa cell nuclear extract proteins and to enhance the activity of the reporter gene in transient transfection of HeLa cells is demonstrated.

Published

2011

11. Identification and mapping of ten new potential insulators in the FXYD5-COX7A1 region of human chromosome 19q13.12

Author

D. A. Didych, E. V. Snezhkov, S. B. Akopov, N. V. Skaptsova, Eugene D. Sverdlov, and Lev G. Nikolaev

Subjects

Genetics, Membrane Glycoproteins, Microfilament Proteins, Chromosome Mapping, General Medicine, Biology, Biochemistry, Ion Channels, Neoplasm Proteins, Electron Transport Complex IV, genomic DNA, Functional mapping, Chromosome 19, Humans, Human genome, Insulator Elements, Enhancer, Promoter Regions, Genetic, Gene, Chromosomes, Human, Pair 19, Selection system

Abstract

A positive-negative selection system revealed 10 potential insulators able to block enhancer interaction with promoter in the 10(6) bp human chromosome 19 region between genes FXYD5 and COX7A1. Relative positions of insulators and genes are in accord with the hypothesis that insulators subdivide genomic DNA into independently regulated loop domains.

Published

2009

12. Methods for identification of epigenetic elements in mammalian long multigenic genome sequences

Author

S. S. Bulanenkova, S. B. Akopov, Lev G. Nikolaev, Igor P. Chernov, Yu. V. Skvortsova, and A. S. Vetchinova

Subjects

Genetics, Base Sequence, Genomics, General Medicine, Computational biology, Epigenome, Biology, DNA Methylation, ENCODE, Physical Chromosome Mapping, Biochemistry, Genome, Chromatin, Epigenesis, Genetic, Epigenetics of physical exercise, DNA methylation, Animals, Humans, CpG Islands, Epigenetics, Regulatory Elements, Transcriptional, Epigenomics

Abstract

Epigenetic elements of the genome, i.e. elements that determine stably inherited changes in gene expression without changes in the genomic DNA sequence, are essential tools of genetic regulation in higher eukaryotes. The complete sequencing of the human and other genomes allowed studies to be started on positioning of these elements within long multigenic regions of the genome, which is a prerequisite for a comprehensive functional annotation of genomes. This mini-review considers some recent experimental approaches to the high-throughput identification and mapping of epigenetic elements of mammalian genomes, including the mapping of methylated CpG sites, open and closed chromatin regions, and DNase I hypersensitivity sites.

Published

2007

13. Identification of tissue-specific DNA-protein binding sites by means of two-dimensional electrophoretic mobility shift assay display

Author

Kira A. Timchenko, Lev G. Nikolaev, Eugene D. Sverdlov, Igor P. Chernov, and S. B. Akopov

Subjects

Biophysics, Protein dna, Electrophoretic Mobility Shift Assay, Biology, Biochemistry, Sensitivity and Specificity, Chromosome 19, Tissue specific, Humans, Electrophoretic mobility shift assay, Electrophoresis, Gel, Two-Dimensional, Tissue Distribution, Binding site, Molecular Biology, Cells, Cultured, Gene Library, Cell Nucleus, Electrophoresis, Agar Gel, Differential display, Binding Sites, Base Sequence, Chromosome Mapping, Nuclear Proteins, Cell Biology, Molecular biology, DNA binding site, DNA-Binding Proteins, Genetic Techniques, Data Display, Electrophoresis, Polyacrylamide Gel, Isoelectric Focusing, Protein target, Transcription Factors

Abstract

We developed a technique of differential electrophoretic mobility shift assay (EMSA) display allowing identification of tissue-specific protein-binding sites within long genomic sequences. Using this approach, we identified 10 cell type-specific protein-binding sites (protein target sites [PTSs]) within a 137-kb human chromosome 19 region. In general, tissue-specific binding of proteins from different nuclear extracts by individual PTSs did not follow the all-or-nothing principle. Most often, PTS-protein complexes were formed in all cases, but they were different for different nuclear extracts used.

Published

2006

14. Tissue specificity of methylation of cytosines in regulatory regions of four genes located in the locus FXYD5-COX7A1 of human chromosome 19: correlation with their expression level

Author

T. V. Chalaya, Eugene D. Sverdlov, S. B. Akopov, and Lev G. Nikolaev

Subjects

Gene Expression, Biology, Biochemistry, Methylation, Ion Channels, Cell Line, Electron Transport Complex IV, Cytosine, Epigenetics of physical exercise, Hepcidins, Histone methylation, Humans, Tissue Distribution, Promoter Regions, Genetic, RNA-Directed DNA Methylation, Uroplakin Ia, Genetics, Regulation of gene expression, Adenosine Triphosphatases, Membrane Glycoproteins, Pioneer factor, Microfilament Proteins, General Medicine, Molecular biology, Neoplasm Proteins, Protein Subunits, DNA methylation, Illumina Methylation Assay, RNA, CpG Islands, Chromosomes, Human, Pair 19, Antimicrobial Cationic Peptides

Abstract

In this study, we compared degree of methylation of selected CpG sites in CCGG sequences located in promoter regions of four human genes with expression level of these genes in several human cell lines and tissues. These genes were subdivided into two groups according to the dependence of their expression on CpG methylation in the 5′-regions. The first group, characterized by clear correlation of methylation with the transcription level, includes housekeeping gene COX6B (the absence of methylation unambiguously correlates with expression) and urothelium-specific uroplakin gene (the methylation coincides with absence of expression). The second group includes genes that are expressed in many, but not all tissues and cells. For these genes (LEAP-1 and ATP4A), there was no correlation between methylation and expression. It is possible that methylation provides some basal level of gene repression, which is overcome by binding of tissue-specific transcription factors, whereas lack of methylation gives the opportunity for gene expression in various cells and tissues.

Published

2006

15. Two-dimensional electrophoretic mobility shift assay: identification and mapping of transcription factor CTCF target sequences within an FXYD5-COX7A1 region of human chromosome 19

Author

Eugene D. Sverdlov, Lev G. Nikolaev, Igor P. Chernov, A. S. Vetchinova, and S. B. Akopov

Subjects

CCCTC-Binding Factor, Chromatin Immunoprecipitation, Biophysics, Electrophoretic Mobility Shift Assay, Biology, Biochemistry, Ion Channels, Electron Transport Complex IV, Alu Elements, Chromosome 19, Humans, Electrophoretic mobility shift assay, Binding site, Molecular Biology, Transcription factor, Genetics, Binding Sites, Membrane Glycoproteins, Models, Genetic, Microfilament Proteins, Chromosome Mapping, Cell Biology, Introns, Neoplasm Proteins, DNA binding site, DNA-Binding Proteins, Repressor Proteins, CTCF, Human genome, DNA, Intergenic, Chromatin immunoprecipitation, Chromosomes, Human, Pair 19, HeLa Cells

Abstract

An approach for fast identification and mapping of transcription factor binding sites within long genomic sequences is proposed. Using this approach, 10 CCCTC-binding factor (CTCF) binding sites were identified within a 1-Mb FXYD5-COX7A1 human chromosome 19 region. In vivo binding of CTCF to these sites was verified by chromatin immunoprecipitation assay. CTCF binding sites were mapped within gene introns and intergenic regions, and some of them contained Alu-like repeated elements.

Published

2006

16. [Regulatory potential of S/MAR elements in transient expression]

Author

Lev G. Nikolaev, Vera M. Ruda, S. B. Akopov, E. V. Snezhkov, Eugene D. Sverdlov, and A. V. Sass

Subjects

Regulation of gene expression, Chinese hamster ovary cell, Organic Chemistry, Mars Exploration Program, CHO Cells, Nuclear matrix, Matrix Attachment Regions, Biochemistry, Molecular biology, In vitro, Cell biology, chemistry.chemical_compound, Enhancer Elements, Genetic, chemistry, Gene Expression Regulation, Cricetinae, Animals, Humans, Scaffold/matrix attachment region, Enhancer, Chickens, DNA

Abstract

S/MARs (scaffold/matrix attachment regions) are the DNA regions that are involved in the interaction with the nuclear matrix and are identified by in vitro methods. According to the available information, S/MARs possess an insulating activity, i.e., the ability to block the interaction between the enhancer and promoter in vivo, and are, probably, intact insulators or their fragments. Nevertheless, there is still no direct proof for this correspondence. To obtain additional information on the insulator activity of S/MARs, we selected five DNA fragments of different lengths and affinities for the nuclear matrix from the previously constructed library of S/MARs and tested their ability to serve as insulators. Two of five elements exhibited an insulator (enhancer-blocking) activity upon the transient transfection of CHO cells. None of the S/MARs displayed either promoter or enhancer/silencer activities in these cells.

Published

2005

17. Recombinant destabilase-lysozyme: synthesis de novo in E. coli and action mechanism of the enzyme expressed in Spodoptera frugiperda

Author

Ekaterina V. Barsova, I. P. Baskova, E. V. Snezhkov, L. L. Zavalova, S. A. Lopatin, and S. B. Akopov

Subjects

Signal peptide, Spodoptera, medicine.disease_cause, Hirudo medicinalis, Biochemistry, Catalysis, Chromatography, Affinity, law.invention, Acetylglucosamine, Substrate Specificity, chemistry.chemical_compound, law, Complementary DNA, Endopeptidases, medicine, Animals, Escherichia coli, Expression vector, biology, Escherichia coli Proteins, General Medicine, biology.organism_classification, Fusion protein, Molecular biology, Recombinant Proteins, chemistry, Recombinant DNA, Muramidase, Lysozyme

Abstract

Destabilase-lysozyme (DL) from salivary gland secretion of the medicinal leech (Hirudo medicinalis) is as a member of the invertebrate lysozyme family, which sharply differs from other lysozyme families. In this study, DL lysozyme function was confirmed during expression of a gene encoding DL in Escherichia coli. Several constructs of the expression vectors pKK OmpA and pET-3A with or without bacterial, leech, or yeast signal peptides (SP) were used. The use of a construct without signal peptide genes resulted in normal growth of the transformed cells. Transformation of E. coli cells with the constructs containing SP was accompanied by the disruption of the forming cells. The use of the expression vector pET-32 LTC-System for production of DL as a fusion protein with thioredoxin also resulted in normal cell growth. However, specific activity of DL isolated from such cells was significantly lower than that of enzyme purified from extracts of Spodoptera frugiperda cells, which were infected with the baculovirus vector carrying DL cDNA. It is shown that the action mechanism of invertebrate lysozyme does not differ from that of other families: recombinant DL from S. frugiperda extracts catalyzed cleavage of synthetic substrate, hexamer of N-acetylglucosamine, to di- and tetramers, which is typical for enzymatic function of other lysozyme families.

Published

2004

18. [Structure and function of nuclear matrix associated regions (S/MARs)]

Author

Igor P. Chernov, S. B. Akopov, and Lev G. Nikolaev

Subjects

Regulation of gene expression, Genetics, Scaffold, Base Sequence, Organic Chemistry, Molecular Sequence Data, Mars Exploration Program, DNA, Biology, Nuclear matrix, Biochemistry, Cell biology, Chromatin, chemistry.chemical_compound, Structure-Activity Relationship, chemistry, Bioorganic chemistry, Nuclear Matrix, Amino Acid Sequence, Scaffold/matrix attachment region

Abstract

Modern concepts on the chromatin loop-domain organization and the role of the DNA regions specifically binding the nuclear matrix (nuclear scaffold, or S/MARs) in its formation, maintenance, and regulation are discussed. Some S/MAR structural features, properties of binding the nuclear matrix, and probable mechanisms of their involvement in regulation of gene activity are considered. The English version of the paper: Russian Journal of Bioorganic Chemistry, 2004, vol. 30, no. 1; see also http://www.maik.ru.

Published

2004

19. Phosphorylation and biosynthesis of high molecular weight proteins of tumor nuclear matrix

Author

S. B. Akopov, T. V. Buldyaeva, T. M. Bazarnova, I. B. Zbarsky, and L. S. Filatova

Subjects

Male, medicine.drug_class, Proteolysis, Biology, Monoclonal antibody, chemistry.chemical_compound, Residue (chemistry), Mice, Biosynthesis, Neoplasms, medicine, Animals, Humans, Nuclear Matrix, Nuclear protein, Phosphorylation, Rats, Wistar, Phosphotyrosine, Molecular Biology, chemistry.chemical_classification, medicine.diagnostic_test, Nuclear Proteins, Antigens, Nuclear, Cell Biology, Nuclear matrix, Phosphoproteins, Molecular biology, Amino acid, Rats, Mice, Inbred C57BL, Molecular Weight, chemistry, Biochemistry, Mice, Inbred CBA, HeLa Cells

Abstract

Our previous studies showed a predominance of high molecular weight protein group in tumor nuclear matrices. Contrary to normal cells, proteins of this group are preferentially phosphorylated. Phosphoproteins of hepatoma nuclear matrix are selectively subjected to rapid proteolysis. By alkali treatment and a monoclonal antibody against phosphotyrosyl residue the presence of two high molecular weight bands of phosphotyrosyl-containing proteins was detected in nuclear matrices of tumor but not of normal liver cells. High molecular weight protein group of tumor nuclear matrices revealed also a rapid turnover and preferential incorporation of labeled amino acids selectively inhibited by chloramphenicol.

Published

1998

20. Long terminal repeats of human endogenous retrovirus K family (HERV-K) specifically bind host cell nuclear proteins

Author

Yuri B. Lebedev, Pavel P. Khil, Eugene D. Sverdlov, Lev G. Nikolaev, and S. B. Akopov

Subjects

viruses, Molecular Sequence Data, Biophysics, Endogenous retrovirus, CHO Cells, Biology, Biochemistry, Jurkat Cells, Long terminal repeat, Structural Biology, Cricetinae, Genetics, Animals, Humans, Human endogenous retrovirus K, Binding site, Nuclear protein, Molecular Biology, Transcription factor, Gene, Repetitive Sequences, Nucleic Acid, Binding Sites, Base Sequence, Nuclear Proteins, Human endogenous retrovirus, Cell Biology, DNA binding protein, HERV-K, Retroviridae, DNA, Viral, Human genome, HeLa Cells

Abstract

Solitary long terminal repeats (LTRs) of the human endogenous retroviruses, scattered in several thousand copies throughout the human genome, are potentially capable of affecting the expression of closely located genes. To assess their regulatory potential, the LTR sequences of one of the most abundant HERV families (HERV-K) were screened for the presence of binding sites for the host cell nuclear factors using mobility shift and UV-crosslinking assays. It was shown that the LTR sequences of two subfamilies harbor a specific binding site for a complex consisting of at least three proteins, ERF1, ERF2 and ERF3 of 98, 91 and 88 kDa apparent molecular mass, respectively. This binding site is located in the 5′ region of the LTR U3 element. The preservation of the specific protein binding site in different HERV-K LTR sequences suggests their possible role in regulation of nearby located genes.

Published

1998