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15 results on '"V S, Baranov"'

1. [Immunocytochemical analysis of human metaphase chromosome methylation status]

Author

A A, Pendina, O A, Efimova, A N, Kaminskaia, T V, Kuznetsova, and V S, Baranov

Subjects
5-Methylcytosine, Antibodies, Monoclonal, Chromosomes, Human, Fluorescent Antibody Technique, Humans, Lymphocytes, DNA Methylation, Metaphase
Abstract

The present paper describes a distribution of 5-methylcytosine-rich DNA in human metaphase chromosomes from PHA-stimulated lymphocytes. Immunocytochemical detection of 5-methylcytosine was carried out with monoclonal antibodies. Fluorescent signals were preferentially localized in certain chromosomal regions, corresponding to R-, some T-bands, pricentromeric heterochromatin, and short arms of acrocentric chromosomes. Specificity of fluorescent signals distribution along chromosomes allowed to describe a new type of human metaphase chromosomes banding pattern, which we call M-banding. Specific M-markers of landmarks were identified for each chromosome pair. The analysis of M-bands methylation status was carried out taking into account data available in literature on their nucleotide structure features, namely GC-rich H3 isochore content and CpG-islands concentration. According to our results, a high level of methylation is typical for the majority of GC-rich regions. However, certain bands of 6, 9, 10, 13, 15 chromosomes (6q15, 6q21, 6q23, 9p13, 9p22, 9p32, 10q24, 13q22, 15q15, 15q24) were shown to be hypomethylated, suggesting their special functional status in lymphocytes.

Published
2006

2. [Isolation and characterisation of continuous human embryonic stem cell lines]

Author

T A, Krylova, V V, Zenin, N S, Musorina, V S, Baranov, N K, Bichevaia, V S, Korsak, N N, Nikol'skiĭ, G P, Pinaev, and G G, Polianskaia

Subjects
Mice, Organic Cation Transport Proteins, Stem Cells, Antigens, Surface, Animals, Humans, Alkaline Phosphatase, Embryo, Mammalian, Coculture Techniques, Cell Line
Abstract

A long-term cultivation (5-8 months) of human blastocyst-derived embryonic cells (hES) was performed. Several properties of hESs were examined to prove the state of continuous cell lines. These cells have passed through 100-175 population doublings with the average population doubling time equal to 37.0 +/- 1.5 h. Isolated hESs, referred to as HESC-1, HESC-2, HESC-3, HESC-4, cultivated on mitotically inactivated mouse embryonic fibroblasts (STO continuous cell line), formed multilayer colonies of various shape. The cells maintained stable proliferative activity, high activity of alkaline phosphatase and expression of transcription factor Oct4, and all this characterizes embryonic stem cells of different origin. Expression of hES specific cell surface antigens (SSEA-3, SSEA-4, TRA-1-81 and TRA-11-81 and TRA-1-60) was confirmed by immunofluorescence analysis with the corresponding monoclonal antibodies. An additional prove for species specificity of HESC lines is the lack of expression of mouse specific surface antigen SSEA1. The cell cycle of HESC-1 undifferentiated cells and embryoid bodies was analysed cytofluorimetrically.

Published
2004

3. [The methylation peculiarities of pericentromeric heterochromatin of chromosomes 1,9 and 16 in human embryo]

Author

A A, Pendina, T V, Kuznetsova, Iu A, Loginova, and V S, Baranov

Subjects
Chromosomes, Human, Pair 1, Heterochromatin, Centromere, Humans, Trisomy, DNA Methylation, Chromosomes, Human, Pair 9, Embryo, Mammalian, Chromosomes, Human, Pair 16
Abstract

By means of in situ nick-translation technique, methylation patterns of pericentric heterochromatin of chromosomes 1, 9 and 16 in extraembryonic (chorion) and embryonic cells of 5-8 week old human fetuses with normal karyotype (5), and in one specimen with trisomy for chromosome 16 were studied. Fixed metaphase chromosomes from direct chromosome preparations were digested with either endonuclease Msp I or its isoshizomer Hpa II recognizing and restricting the same sDNA sequence C decreases CGC with Hpa II, but not Msp I sensitive to methylation state of internal cytosin. According to our results, heterochromatin of extraembryonic, but not embryonic cells is hypomethylated. An obvious difference was registered in signal strength between homologous regions in iq12 of both parental chromosomes 1 in early (5-6 week old), but not in more advanced fetuses. Methylation pattern difference was detected in pericentric chromatin of triple copies of chromosome 16 in extraembryonic tissues of the 47,XY, + 16 fetus. These results are in line with a hypothesis of intraheterochromatin location of "early" genes governing initial stages of embryonic development in humans.

Published
2001

4. [Ultrastructural and morphometrical analysis of apoptosis stages in cardiomyocytes of MDX mice]

Author

V M, Mikhaĭlov, S A, Komarov, V K, Nilova, G I, Shteĭn, and V S, Baranov

Subjects
Cell Nucleus, Mice, Inbred C57BL, Mice, Nuclear Envelope, Stress, Physiological, Myocardium, Mice, Inbred mdx, Animals, Apoptosis, Chromatin, Mitochondria
Abstract

Our previous study of apoptosis in mdx mouse myocardium cells demonstrated the presence of middle-sized DNA fragments (60-65 kbp) in extracts of myocardium DNA, and irregular shape of membrane enveloped nuclei in cardiomyocytes. The DNA fragmentation (DNA laddering) was observed after biomechanical stress (5 min sweeming) only. Based on these results we concluded that the majority of cardiomyocytes were at the first stage of apoptosis. The purpose of this work was to provide some morphometrical quantitive characteristics of ultrastructural properties of the nuclei and mitochondria, and to determine morphological patterns of apoptosis in cardiomyocytes of mdx and C57B1 mice. To resolve the task, we made a morphometrical analysis of the electron microscope images of nuclei and mitochondria. First of all, we divided all nuclear images into three categories: normal, semi-pathological, and pathological forms according to the extent of nuclear membrane invaginations and that of condensed chromatin spreading. The most part of C57B1 cardiomyocyte nuclei belonged to the normal form (88.9 +/- 4.3%), while the smaller part (11.1 +/- 4.3%) was regarded as semi-pathological forms. Just a reverse was observed in mdx mice: the largest part of cardiomyocytes fell into category of semi-pathological (54.6 +/- 4.4%) and pathological (31.5 +/- 4.1%) forms while, the smallest part belonged to the normal form (13.8 +/- 3.0%). 24 h after biodynamic stress, the quantity of normal nuclei of C57B1 cardiomyocytes decreased to 61 +/- 5%, the number of semi-pathological nuclei increased to 39.0 +/- 4.4% (P0.05). The number of pathological nuclei of mdx, cardiomyocytes fell to 15.4 +/- 3.0% (P0.05). It means that mdx cardiomyocytes with pathological form of their nuclei disappear because of emerging the second, destructive stage of apoptosis. To estimate the degree of ultrastructural changes in the nuclei of all three forms of cardiomyocytes we counted the square/perimeter ratio in each nucleus (circle shape factor; CSF). The value of CSF for normal nuclei of all the forms of cardiomyocytes varied between 0.65 +/- 0.02 and 0.71 +/- 0.04. In semi-pathological and pathological nuclei a significant decrease in CSF to 0.56 +/- 0.02 and 0.56 +/- 0.03 was observed, respectively (P0.05). The biodynamical stress did not reduce the CSF value below this level. We also counted the ratio of the square to the product of a long and a short axes (ellipse shape factor; ESF). The ESF value for normal nuclei of all forms of cardiomyocytes varied between 0.97 +/- 0.01 and 0.99 +/- 0.01. In the case of mdx mice the biodynamical stress reduced ESF to 0.95 +/- 0.01 (P0.05) for pathological form of nuclei. The specific density of mitochondria in mdx cardiomyocytes (0.274 +/- 0.016) was less than that in C57B1 cardiomyocytes (0.329 +/- 0.018). At the destructive stage of apoptosis, the nuclei of cardiomyocytes were round in shape, the nuclear chromatin being hypercondensed, and mitochondria swollen. The cardiomyocyte morphology was in agreement with the definition of the final stage of apoptosis as secondary necrosis. Morphometrical results show that as many as 86-90% of nuclei of mdx cardiomyocytes have abnormal structure that confirms our conclusion that mdx cardiomyocytes were at the first stage of apoptosis. The final stage of apoptosis is rarely observed by biochemical or morphological methods. It suggests the presence of some inner mechanisms regulating the initiation of the final (destructive) stage of mdx cardiomyocyte apoptosis.

Published
2001

5. [Polymorphism of nucleolar organizer regions of chromosomes in human embryos]

Author

A A, Pendina, T V, Kuznetsova, and V S, Baranov

Subjects
Polymorphism, Genetic, Nucleolus Organizer Region, Chromosomes, Human, Humans, Embryo, Mammalian
Abstract

NOR activity in metaphase chromosomes from extraembryonic and embryonic tissues of 9-12 week human fetuses was studied after standard silver staining. Significant interidividual variations in the average cummulative NOR activity was assessed by means of one-factor dispersion analysis. No significant intertissue fluctuation of NOR activity was found. Total number of NOR+ chromosomes demonstrated no correlation with the embryonic age. Steady growth of an average cummulative NOR activity respective of progressive embryonic age was proven by correlation analysis method. Unequal participation of NOR-bearing chromosomes of D- and G-groups during early embryonic development in human was shown.

Published
2000

6. [Differentiation of muscle fibers in mdx mice after ballistic transfection of cDNA of the human dystrophin gene]

Author

V M, Mikhaĭlov, A V, Zelenin, G I, Shteĭn, O A, Tarasenko, V A, Kolesnikov, I A, Zelenina, R A, Shafei, and V S, Baranov

Subjects
Dystrophin, Mice, DNA, Complementary, Muscle Fibers, Skeletal, Mice, Inbred mdx, Animals, Humans, Cell Differentiation, Biolistics, Transfection, Plasmids
Abstract

Changes in morphological dimensions of MDX mouse myofibres in M. rectus femoris were recorded after ballistic transfection (BT) with pHSADys and pVMMDys plasmids containing cDNA of the full-length human dystrophin gene. The dystrophin expression was observed by an immunomorphological procedure with P6 antibody and PAP method. Dystrophin positive (dyst+) myofibres were divided into two types, with a typical dystrophin expression under sarcoplasma membrane and an atypical expression through the whole sarcoplasm, respectively. The share of atypical dyst+ myofibres was seen to rise during the experiment from 27%, at 2-3 weeks after BT, up 84% by 2 months after BT. The atypical dyst+ myofibres usually underwent destruction. At the same time, the share of entire dyst+ myofibres decreased from 17 to 2-5% by 2 months. Morphological dimensions of the myofibres (square in mkm2, perimeter, smallest and largest diameters) were calculated with the help of computer analyser. The middle square of both types of dyst+ myofibres was larger than that of dyst- myofibres, both in BT target M. rectus femoris and in the same contralateral muscle, but never exceeded the value of middle square of C57B1 mouse myofibres in the same muscle. The form of dyst+ myofibres was not modified by the dystrophin expression. The nuclei of dyst+ myofibres remained in the central region of sarcoplasm. A conclusion is made that BT of human dystrophin gene inside MDX mouse myofibres allows dystrophin gene expression and enlargement of the dyst+ myofibres. Dystrophin expression is not able to induce a complete and stable differentiation of striated muscle of adult MDX mice.

Published
1998

7. [Apoptosis and DNA degradation of cardiomyocytes of mdc and C57Bl mice]

Author

V M, Mikhaĭlov, V I, Kazakov, S A, Komarov, V K, Nilova, G I, Shteĭn, and V S, Baranov

Subjects
Electrophoresis, Mice, Inbred C57BL, Mice, Microscopy, Electron, Stress, Physiological, Myocardium, Mice, Inbred mdx, Animals, Apoptosis, DNA, Swimming
Abstract

DNA destruction and apoptosis of ventricular cardiomyocytes were studied using DMX and C57Bl10/J mice. According to our electron microscope observations the cardiomyocyte nuclei undergo chromatin condensation with the nuclear membrane folding. In cardiomyocytes with significant nuclear destruction, structural disturbances in the cytoplasm are also seen. The 0.5% agarose gel electrophoresis reveals DNA fragments, sized 64 kb and more, inside the total DNA of MDX mice myocardium. No kinds of DNA fragments are available inside samples of the total DNA of C57Bl mice myocardium. Swimming during 5 min induces formation of the same type of DNA fragments inside the total of DNA of C57Bl mice myocardium, which was registered after 2 and 22 hours of the experiment. The DNA fragments disappear from the total C57Bl mice myocardium DNA within 48 h after the stress. Trypan blue evokes formation of the same 64 kb fragments inside DNA of myocardium within 24 h after injection to C57Bl mice. Electrophoresis of the total DNA with 2% agarose gel or 5% PAAG revealed no DNA samples analysed during this study. The authors conclude that DNA destruction and apoptosis characteristic features of MDX mice cardiomyocytes of mice, have a common mechanism of DNA degradation that works both after the stress of trypan blue action in case of C57Bl mice, and as a consequence of dystrophin absence in cardiomyocytes in the case of MDX mice.

Published
1998

8. [A cytogenetic study of the human chorion for the purpose of the prenatal diagnosis of hereditary diseases]

Author

V S, Baranov, M V, Popova, T N, Novikova, I Ia, El'gart, T V, Kharchenko, E P, Mikhaĭlova, V N, Gorbunova, T V, Pigina, L K, Tsuladze, and Iu B, Iurov

Subjects
Chromosome Aberrations, Sex Determination Analysis, Ploidies, Mosaicism, Genetic Diseases, Inborn, Abortion, Induced, Chromosome Disorders, Diagnosis, Differential, Fetal Diseases, Chorionic Villi Sampling, Pregnancy, Prenatal Diagnosis, Humans, Female
Abstract

Cytogenetical investigation of 50 diagnostic chorionic villus samples from women with a high risk of giving birth to babies with chromosomal and genic pathology, and of 128 chorionic samples obtained from medical abortions, both on the 8-12th weeks of gestation was performed by means of original direct chromosomal analysis. Chromosomal anomalies were found in 6 cases of diagnostic chorion biopsies (12%) and in 4 cases (3%) of medical abortions. The former group included 5 embryos with autosomal trisomy (4--Ts21 and 1--Ts13) and one embryo with monosomy 18. The latter group contained 2 embryos with X-chromosome monosomy and 2 other with chromosomal mosaicism. A significant prevalence of the female sex was found in the diagnostic group (sex ratio 0.56), but not in the medical abortion one (sex ratio 1.0). Analysis of routine chromosomal preparations and those after in situ hybridization with X-chromosome alfoid-probe YAP 1-10 revealed polyploidy in average in 0.8-1% chorion cells. The feasible causes of sex ratio distortion in embryos of diagnostic group and factors responsible for the rate of polyploidy are discussed. High reliability of originally elaborated direct "shaking-blotting" method of chromosomal preparations from chorionic villus samples is stressed.

Published
1990

9. [Prezygotic selection of male gametes in laboratory mice]

Author

V S, Baranov and A P, Dyban

Subjects
Chromosome Aberrations, Male, Mice, Reproduction, Mice, Inbred CBA, Animals, Mitosis, Mice, Inbred Strains, Aneuploidy, Spermatogenesis, Translocation, Genetic
Abstract

Frequency of aneuploid male gametes was related to the number of early embryos with numeral chromosomal aberrations in progeny of male mice, heterozygous for the Robertsonian translocations T1 (15.6) AID, and T1 (17.8) IEM. In mice heterozygous for translocation T1 (15.6) AID, the number of spermatocytes II with NF=21 was very low and corresponded to the number of trisomic embryos at stages of major organogenesis. In mice heterozygous for T1 (17.8) IEM translocation, the number of aneuploid gametes was 26.2%, but neither embryo of their progeny, on the 8 12th days of gestation, was found to be trisomic. The involvement of chromosomes 8 and 17 in the control of postmeiotic stages of spermatogenesis in mice is suggested.

Published
1976

10. [A method of shaking-blotting--a simple and reliable means for obtaining direct chromosomal preparations from chorionic biopsies]

Author

V S, Baranov

Subjects
Chorionic Villi Sampling, Pregnancy, Karyotyping, Chromosomes, Human, Humans, Female, Gestational Age, Chorion
Abstract

The method proposed is based on a gradual fixation, and short-term hydration before softening and on a new technique of chromosome preparation. The latter is based on the sample softening in 60% acetic acid directly on the slide, its gentle shaking and spot-blotting, a careful spreading of the cell suspension on slide surface avoiding the usage of micropipets and other handlings causing metaphase plate breakage. The method provides a highly efficient karyotyping of human embryos within the 7-12th weeks of gestation.

Published
1989

12. [Rb(2.6)4IEM: a new Robertsonian marker translocation in Mus musculus laboratory mice]

Author

V S, Baranov

Subjects
Genetic Markers, Male, Mice, Inbred C57BL, Heterozygote, Mice, Homozygote, Mice, Inbred CBA, Animals, Female, Crosses, Genetic, Translocation, Genetic
Abstract

A detailed cytogenetic analysis of mice, both heterozygous and homozygous, for a new translocation of a spontaneous origin has been performed. The differential staining of mitotic and meiotic chromosomes, and the analysis of F1-hybrides proved that this translocation of Robertsonian type resulted from the centromeric fusion between chromosomes 2 and 6 of the normal karyotype. According to the standards for genetic nomenclature of laboratory mouse, the translocation is called Rb(2.6)4IEM (Institute for Experimental Medicine). A stock of laboratory mice homozygous for two different Robertsonian translocation - Rb(2.6)4IEM and Rb(8.17)1IEM has been obtained (2n = 36, NF = 40). Feasible mechanisms of chromosomal rearrangements leading to new translocations of the Robertsonian type in laboratory mice are discussed.

Published
1981

13. [Variation in the number of C-heterochromatin blocks in the interphase nuclei of the cells of a transplantable murine rhabdomyosarcoma]

Author

E V, Kaminskaia, V S, Baranov, and Iu B, Vakhtin

Subjects
Cell Nucleus, Mice, Inbred C57BL, Mice, Lung Neoplasms, Skin Neoplasms, Heterochromatin, Rhabdomyosarcoma, Animals, Genetic Variation, Interphase, Neoplasm Transplantation, Clone Cells
Abstract

By means of staining procedure which reveals the constitutive heterochromatin (CH), the number of CH-blocks was detected in the nuclei of interphase cells obtained from the subcutaneously growing rhabdomyosarcoma and from its 10 lung colonies. The range of variability of the number of CH-blocks in tumor cell populations was greater than in the populations of normal lung cells and lymphocytes. The mean numbers of CH-blocks varied from 17.8 +/- 0.9 to 28.0 +/- 1.2 in cells of different clones, the mean number of CH-blocks in clones being the same as in the subcutaneously growing uncloned tumor. The coefficient of heritability h2 of character "the number of CH-blocks", calculated on the basis of population and interclonal variances, was equal to 0.15, and that calculated by one-factor dispersional analysis was actually the same (0.16). It is concluded that the high heterogeneity of tumor cells may be conditioned not only by their high phenotypic instability, but also by a high frequency of mutations.

Published
1985

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