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3. 2-Amino-3'-dialkylaminobiphenyl-based fluorescent intracellular probes for nitric oxide surrogate N 2 O 3 .

Author

Escamilla PR, Shen Y, Zhang Q, Hernandez DS, Howard CJ, Qian X, Filonov DY, Kinev AV, Shear JB, Anslyn EV, and Yang Y

Abstract

Fluorescent probes for nitric oxide (NO), or more frequently for its oxidized surrogate dinitrogen trioxide (N 2 O 3 ), have enabled scientists to study the contributions of this signaling molecule to many physiological processes. Seeking to improve upon limitations of other probes, we have developed a family of fluorescent probes based on a 2-amino-3'-dialkylaminobiphenyl core. This core condenses with N 2 O 3 to form benzo[ c ]cinnoline structures, incorporating the analyte into the newly formed fluorophore, which results in product fluorescence with virtually no background contribution from the initial probe. We varied the substituents in the core in order to optimize both the reactivity of the probes with N 2 O 3 and their cinnoline products' fluorescence wavelengths and brightness. The top candidates were then applied to cultured cells to verify that they could respond to NO within cellular milieus, and the top performer, NO 530 , was compared with a "gold standard" commercial probe, DAF-FM, in a macrophage-derived cell line, RAW 264.7, stimulated to produce NO. NO 530 demonstrated similar or better sensitivity and higher selectivity for NO than DAF, making it an attractive potential alternative for NO tracking in various applications., Competing Interests: DYF and AVK are employees of Creative Scientist, Inc., (This journal is © The Royal Society of Chemistry.)

Published
2020
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5. Targeting Fluorescent Nanodiamonds to Vascular Endothelial Growth Factor Receptors in Tumor.

Author

Torelli MD, Rickard AG, Backer MV, Filonov DS, Nunn NA, Kinev AV, Backer JM, Palmer GM, and Shenderova OA

Subjects
Animals, Click Chemistry, Female, HEK293 Cells, Humans, Mice, Inbred BALB C, Mice, Nude, Models, Molecular, Optical Imaging methods, Fluorescent Dyes chemistry, Nanodiamonds chemistry, Neoplasms diagnostic imaging, Receptors, Vascular Endothelial Growth Factor analysis, Vascular Endothelial Growth Factor A chemistry
Abstract

The increased expression of vascular endothelial growth factor (VEGF) and its receptors is associated with angiogenesis in a growing tumor, presenting potential targets for tumor-selective imaging by way of targeted tracers. Though fluorescent tracers are used for targeted in vivo imaging, the lack of photostability and biocompatibility of many current fluorophores hinder their use in several applications involving long-term, continuous imaging. To address these problems, fluorescent nanodiamonds (FNDs), which exhibit infinite photostability and excellent biocompatibility, were explored as fluorophores in tracers for targeting VEGF receptors in growing tumors. To explore FND utility for imaging tumor VEGF receptors, we used click-chemistry to conjugate multiple copies of an engineered single-chain version of VEGF site-specifically derivatized with trans-cyclooctene (scVEGF-TCO) to 140 nm FND. The resulting targeting conjugates, FND-scVEGF, were then tested for functional activity of the scVEGF moieties through biochemical and tissue culture experiments and for selective tumor uptake in Balb/c mice with induced 4T1 carcinoma. We found that FND-scVEGF conjugates retain high affinity to VEGF receptors in cell culture experiments and observed preferential accumulation of FND-scVEGF in tumors relative to untargeted FND. Microspectroscopy provided unambiguous determination of FND within tissue by way of the unique spectral shape of nitrogen-vacancy induced fluorescence. These results validate and invite the use of targeted FND for diagnostic imaging and encourage further optimization of FND for fluorescence brightness.

Published
2019
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6. Long-term observation of amphibian populations inhabiting urban and forested areas in Yekaterinburg, Russia.

Author

Vershinin VL, Vershinina SD, Berzin DL, Zmeeva DV, and Kinev AV

Subjects
Animals, Cities, Forests, Russia, Amphibians, Ecosystem
Abstract

This article presents data derived from a 36 year-long uninterrupted observational study of amphibian populations living in the city and vicinity of Yekaterinburg, Russia. This area is inhabited by six amphibian species. Based on a degree of anthropogenic transformation, the urban territory is divided into five highly mosaic zones characterized by vegetation, temperature, and a distinctive water pollution profile. Population data is presented year-by-year for the number of animals, sex ratio, and species-specific fecundity including the number and quality of spawns for the following amphibian species: Salamandrella keyserligii, Rana arvalis, R. temporaria, Lissotriton vulgaris, and Pelophylax ridibundus. These data provide an excellent opportunity to assess an urban environment from an animal population-wide perspective, as well as revealing the forces driving animal adaptation to the anthropogenic transformation of habitats.

Published
2015
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7. Endothelial colony forming cells (ECFCs) as a model for studying effects of low-dose ionizing radiation: growth inhibition by a single dose.

Author

Kinev AV, Levering V, Young K, Ali-Osman F, Truskey GA, Dewhirst MW, and Il'yasova D

Subjects
Cells, Cultured, Endothelial Cells physiology, Humans, Models, Biological, Primary Cell Culture, Radiation Injuries pathology, Stem Cells physiology, Cell Proliferation radiation effects, Endothelial Cells radiation effects, Stem Cells radiation effects
Abstract

Identification of measurable nontransient responses to low-dose radiation in human primary cell cultures remains a problem. To this end, circulating endothelial colony-forming (progenitor) cells (ECFCs) were examined as an experimental model. ECFCs were isolated from three cord blood donors. Cells were positive for endothelial cell markers and remained highly proliferative after long-term cryopreservation. A single dose of X-ray radiation (0.06-0.38 Gy) inhibited ECFC culture growth. This effect was evident at 48 hours and persisted up to 72 hr postirradiation. Such protracted cytostatic response of ECFCs to low-dose radiation suggests that ECFC primary cultures can be used to study low-dose radiation effects.

Published
2013
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8. Novel mechanism of Hsp70 chaperone-mediated prevention of polyglutamine aggregates in a cellular model of huntington disease.

Author

Guzhova IV, Lazarev VF, Kaznacheeva AV, Ippolitova MV, Muronetz VI, Kinev AV, and Margulis BA

Subjects
Cell Line, Tumor, Gene Expression, Gene Expression Regulation, Glyceraldehyde-3-Phosphate Dehydrogenases metabolism, HSP70 Heat-Shock Proteins genetics, Humans, Huntington Disease genetics, Protein Binding, Solubility, HSP70 Heat-Shock Proteins metabolism, Huntington Disease metabolism, Peptides metabolism
Abstract

The key feature of polyglutamine aggregates accumulating in the course of Huntington disease (HD) is their resistance to protein denaturants, and to date only chaperones are proved to prevent mutant protein aggregation. It was suggested that expanded polyglutamine chains (polyQ) of mutant huntingtin are cross-linked to other proteins such as glyceraldehyde-3-phosphate dehydrogenase (GAPDH). Here we clarify the roles of GAPDH and molecular chaperone Hsp70 in the formation of sodium dodecyl sulfate (SDS)-insoluble polyQ aggregates. First, the addition of pure GAPDH was found to enhance the aggregation of polyQ in a cell-free model of HD. Secondly, the immunodepletion of GAPDH dose-dependently decreased polyQ aggregation. Finally, siRNA-mediated inhibition of GAPDH protein in SK-N-SH neuroblastoma cells has also reduced the aggregation of cellular polyQ. Regulated over-expression of Hsp70 decreased the amount of GAPDH associated with SDS-insoluble polyQ aggregates. Physical association of Hsp70 and GAPDH in SK-N-SH cells was shown by reciprocal immunoprecipitation and confocal microscopy. Pure Hsp70 dose-dependently inhibited the formation of polyQ aggregates in cell-free model of HD by sequestering both GAPDH and polyQ. We demonstrated that Hsp70 binds to polyQ in adenosine triphosphate-dependent manner, which suggests that Hsp70 exerts a chaperoning activity in the course of this interaction. Binding of Hsp70 to GAPDH was nicotinamide adenine dinucleotide-dependent suggesting another type of association. Based on our findings, we conclude that Hsp70 protects cells in HD by removing/sequestering two intrinsic components of protein aggregates: the polyQ itself and GAPDH. We propose that GAPDH might be an important target for pharmacological treatment of HD and other polyglutamine expansion-related diseases.

Published
2011
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9. [Accumulation of heat-shock proteins 70 in insect fat bodies as evidence of stress in Microsporidia-infected insects].

Author

Seleznev KV, Kinev AV, and Margulis BA

Subjects
Animals, Chromatography, Affinity, Corpora Allata metabolism, Fat Body parasitology, Gryllidae anatomy & histology, HSP70 Heat-Shock Proteins blood, Hemolymph chemistry, Host-Parasite Interactions, Juvenile Hormones metabolism, Microsporidia pathogenicity, Microsporidia ultrastructure, Fat Body metabolism, Gryllidae parasitology, Gryllidae physiology, HSP70 Heat-Shock Proteins metabolism, Microsporidia physiology
Abstract

At present a concept prevails that pathological alterations in insect hosts infected with microsporidia, and those associated with hormone imbalance may be explained by the production of juvenile hormone-like (JH) substances by microsporidia. According to another view point, this pathology is a consequence of the host response. We suggested that the microsporidian infection can provoke a stress reaction in insects, which may cause JH secretion by these insects. To confirm this hypothesis, we have analysed major stress protein Hsp70 levels in the infected insects. Using affinity chromatography on ATP-agarose and immunoblotting, we have shown that Hsp70 was accumulated in infected crickets, and that it was the host protein. The consequence of events accompanying the infection in the insects is discussed in relation to the response of hormonal system of the host organism.

Published
2003

10. A human BRCA2 complex containing a structural DNA binding component influences cell cycle progression.

Author

Marmorstein LY, Kinev AV, Chan GK, Bochar DA, Beniya H, Epstein JA, Yen TJ, and Shiekhattar R

Subjects
Amino Acid Sequence, Animals, Antibodies metabolism, BRCA2 Protein, Breast Neoplasms genetics, Cell Fractionation, Cell Nucleus chemistry, Chromosomes chemistry, Chromosomes metabolism, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, DNA-Binding Proteins isolation & purification, Embryo, Mammalian chemistry, Embryo, Mammalian metabolism, Female, HeLa Cells, High Mobility Group Proteins, Humans, In Situ Hybridization, Mice, Microinjections, Molecular Sequence Data, Neoplasm Proteins chemistry, Neoplasm Proteins genetics, Nucleic Acid Conformation, Ovarian Neoplasms genetics, Precipitin Tests, Protein Structure, Tertiary, Transcription Factors chemistry, Transcription Factors genetics, Chromatin metabolism, DNA-Binding Proteins metabolism, Mitosis physiology, Neoplasm Proteins metabolism, Transcription Factors metabolism
Abstract

Germline mutations of the human BRCA2 gene confer susceptibility to breast cancer. Although the function of the BRCA2 protein remains to be determined, murine cells homozygous for BRCA2 inactivation display chromosomal aberrations. We have isolated a 2 MDa BRCA2-containing complex and identified a structural DNA binding component, designated as BRCA2-Associated Factor 35 (BRAF35). BRAF35 contains a nonspecific DNA binding HMG domain and a kinesin-like coiled coil domain. Similar to BRCA2, BRAF35 mRNA expression levels in mouse embryos are highest in proliferating tissues with high mitotic index. Strikingly, nuclear staining revealed a close association of BRAF35/BRCA2 complex with condensed chromatin coincident with histone H3 phosphorylation. Importantly, antibody microinjection experiments suggest a role for BRCA2/BRAF35 complex in modulation of cell cycle progression.

Published
2001
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11. [A method for determining the constitutive and inducible forms of a heat-shock protein of 70 kDa in the human myocardium and lymphocytes].

Author

Karpishchenko AI, Demidov ON, Tyrenko VV, Komarova EIu, Kinev AV, and Margulis BA

Subjects
Adolescent, Adult, Aged, Child, Electrophoresis, Polyacrylamide Gel methods, Female, HSP70 Heat-Shock Proteins isolation & purification, HSP72 Heat-Shock Proteins, Heat-Shock Proteins analysis, Heat-Shock Proteins isolation & purification, Humans, Immunoblotting methods, Male, HSP70 Heat-Shock Proteins analysis, Lymphocytes chemistry, Myocardium chemistry
Published
2000

12. [Role of heat-shock proteins in cardioprotection of patients operated on for ischemic heart disease].

Author

Shevchenko IuL, Demidov ON, Tyrenko VV, Svistov AS, Belevitin AB, Karpishchenko AI, Komarova EIu, Popova TV, Kinev AV, and Margulis BA

Subjects
Adult, Aged, Aorta surgery, Biopsy, Cardiopulmonary Bypass, Creatine Kinase blood, Data Interpretation, Statistical, Electrophoresis, Polyacrylamide Gel, HSP70 Heat-Shock Proteins analysis, HSP70 Heat-Shock Proteins biosynthesis, HSP70 Heat-Shock Proteins physiology, Heat-Shock Proteins analysis, Heat-Shock Proteins biosynthesis, Humans, Immunoblotting, Male, Middle Aged, Myocardial Reperfusion Injury physiopathology, Myocardium metabolism, Time Factors, Coronary Artery Bypass, Coronary Disease surgery, Heat-Shock Proteins physiology, Myocardium chemistry
Abstract

Major stress protein HSP72 is known to participate in protecting cells and organisms against harmful factors including ischemia, trauma etc. Under study was the level of HSP72 in the myocardium of 32 patients with coronary disease operated in Military-medical academy. HSP72 was detected in probes of the right atria before and after pre-cardiopulmonary bypass in all cases induction of HSP72 was observed in 40% of patients, and directly correlated with the time of cardiopulmonary bypass and standing of the disease. The cardioprotective effect of the elevated pre-operational level of HSP72 was shown to be proportionate to the lower activity of cardiospecific enzymes, creatine phosphokinase (CK-MB). It is suggested that HSP72 is involved in the mechanism of cardioprotection during cardiopulmonary bypass.

Published
1999

13. Effects of exogenous stress protein 70 on the functional properties of human promonocytes through binding to cell surface and internalization.

Author

Guzhova IV, Arnholdt AC, Darieva ZA, Kinev AV, Lasunskaia EB, Nilsson K, Bozhkov VM, Voronin AP, and Margulis BA

Subjects
Animals, Antigens, CD analysis, Apoptosis, Carrier Proteins isolation & purification, Carrier Proteins metabolism, Cattle, Cell Differentiation, Cell Division, Cell Line, DNA metabolism, Endocytosis, Flow Cytometry, Genes, fos genetics, HSC70 Heat-Shock Proteins, HSP70 Heat-Shock Proteins isolation & purification, HSP70 Heat-Shock Proteins metabolism, Humans, Monocytes metabolism, Muscle, Skeletal, Promoter Regions, Genetic genetics, Tetradecanoylphorbol Acetate pharmacology, Transcription Factors metabolism, Tumor Necrosis Factor-alpha toxicity, Carrier Proteins pharmacology, HSP70 Heat-Shock Proteins pharmacology, Monocytes cytology
Abstract

The presence of antibodies against the major stress protein, Hsp70, in patients with autoimmune diseases led us to hypothesize that Hsp70 may occur extracellularly, and could exert chaperoning and regulatory effects on various cells. We examined the action of pure Hsp/Hsc70 on the main physiological functions of human promonocytic U-937 cells. The protein was isolated from calf muscle and was shown to be a mixture of inducible Hsp70 (60%) and constitutive Hsc70 (40%) isoforms. It was observed that the addition of the protein up-regulated two major monocyte/macrophage differentiation markers, CD11c and CD23, by 20-35%, while it had no effect on CD14. The experiments performed to investigate the influence of Hsp/Hsc70 on the reaction of U-937 cells to differentiation stimuli demonstrated that the addition of the protein prior to PMA was able to inhibit binding of proper transcription factors to double-symmetry and cAMP-response elements of the c-fos early response gene promoter. Administration of exogenous Hsp/Hsc70 prior to treatment with the tumor necrosis factor-alpha significantly lowered the number of apoptotic and necrotic cells. In no case did the control protein, ovalbumin, taken in the same concentration give a comparable effect on U-937 cells. Since the Hsp/Hsc70 effects occurred within the first hour of co-incubation, and therefore they might be explained by its interaction with the cell surface, we assayed binding of the biotinylated protein to U-937 cells by immunoenzyme assay, flow cytometry and indirect immunofluorescence. Using these three techniques we were able to detect Hsp/Hsc70 bound to cells after a 20 min incubation. According to flow cytometry data, at this time 32% of cells were positively stained with streptavidin-FITC. Immunofluorescence studies demonstrated Hsp/Hsc70 bound to the cell surface after a 20 min incubation followed by induction of patch and cap-like structures. One hour later, the majority of the protein had been internalized by U-937 cells.

Published
1998
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14. [Effect of an extracellular heat shock protein on chromosome variability in Indian muntjak cultured skin fibroblasts].

Author

Polianskaia GG, Kinev AV, Sakuta GA, and Aseeva EV

Subjects
Animals, Cells, Cultured, Ciprofloxacin pharmacology, Extracellular Space, Fibroblasts drug effects, Lipopolysaccharides pharmacology, Muntjacs, Skin cytology, Chromosome Aberrations, HSP70 Heat-Shock Proteins pharmacology, Skin drug effects
Abstract

It is known that the essential function of extracellular HSP70 (e-HSP70) to protect cell processes, indirectly associated with the genetic structures. A direct influence of e-HSP70 on chromosomal stability has not been studied. This explains actuality of the suggested investigation. A study was made of the influence of e-HSP70 on chromosomal variability at different phases of the first mitotic cycle in both intact and ciprofloxacin (CF) treated cells of the Indian muntjac skin fibroblasts. E-HSP70 (10 mg/ml) exerts no influence on the level of chromosomal aberrations, typical of the control. After a joint action of e-HSP70 and CF (50 mg/ml) no influence was also exerted on the antibiotic induced genotoxicity effect. CF and e-HSP70 (50 and 100 mg/ml, resp.) acting apart on intact cells during 6 and 24 h induce a significant increase of chromosomal aberrations compared to the control, primarily at the expense of chromatid or chromosomal breaks (depending on the duration of respective effect). CF and e-HSP70 acting apart on intact cells during 6 h with the following cultivation for 18 h in the fresh medium prior to fixation also induce a significant increase of chromosomal aberrations compared to the control, primarily at the expense of both breaks and dicentrics (telomeric associations). The joint action of CF and e-HSP70 on cultivated cells during 6 and 24 h and when CF and e-HSP70 were added respectively on 24 and 6 h prior to fixation, a significant decrease in chromosomal aberrations compared to the control level was induced. A simultaneous addition of CF and e-HSP70 in 6 h with the following cultivation for 18 h in fresh medium prior to fixation exerted no influence on the degree of genotoxicity effect, typical of the separate action of these agents. However a significant decrease in the number of dicentrics occurred. Apparently, e-HSP70 has a protective effect on chromosomal stability mainly at phase 62 of the mitotic cycle. The denaturated e-HSP70 (50, 100 mg/ml) has a genotoxicity effect similar to that of the infact e-HSP70 under above conditions. The joint action of CF and denaturated e-HSP70 (50 mg/ml) during 24 h exerts no influence on the degree of genotoxicity effect, induced by the separate action of these agents or leads to an increase in the number of dicentrics, acting separately or jointly compared to the control. The denaturated e-HSP70 (100 mg/ml) acting jointly with CF for 24 h, increases the degree of genotoxicity effects, induced by separate actions of the agents. Lipopolysacharide (50 mg/ml) exerts no influence on the number of chromosomal aberrations in the control. The sensitivity of individual chromosomes and their regions to agents inducing chromosomal instability is different. The preferential involvement of some chromosomes in dicentric formation was observed. A possible role of dicentrics in adaptation of cells belonging to "markerless" lines to infavourable factors of the environment, and possible mechanisms of protecting effect exerted by e-HSP70 on chromosomes are discussed.

Published
1997

15. Exogenous heat shock protein hsp70 activates potassium channels in U937 cells.

Author

Negulyaev YA, Vedernikova EA, Kinev AV, and Voronin AP

Subjects
Calcium metabolism, Calcium pharmacology, Electric Conductivity, Humans, Kinetics, Lymphoma, Large B-Cell, Diffuse, Patch-Clamp Techniques, Tumor Cells, Cultured, Cell Membrane physiology, HSP70 Heat-Shock Proteins pharmacology, Potassium Channels drug effects, Potassium Channels physiology
Abstract

With the use of patch clamp technique, the effect of exogenous heat shock protein hsp70 on ion channel properties in the plasma membrane of human promonocyte U937 cells has been examined. Cell-attached experiments showed that the addition of 30-100 micrograms/ml hsp70 to the pipette solution resulted in an activation of outward currents through potassium-selective channels of 9 pS unitary conductance. The activity of K(+)-selective channels did not depend on membrane voltage and could be controlled by the intracellular free calcium concentration as revealed in inside-out recordings. K+ channels with similar conductance and kinetic behaviour were found in normal cell-attached patches very rarely. Outside-out experiments showed that the addition of hsp70 to the external solution induced a channel-like stepwise increase of inward current which may provide cation entry from the extracellular medium. The interaction of extracellular hsp70 with the membrane surface of the native cell and of the excised fragment was found to be different. The results suggest that hsp70-induced activation of Ca-dependent K channels in monocyte-macrophage cells may be due to a local increase of free Ca2+ concentration just near the inner membrane side.

Published
1996
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16. The characterization and use of different antibodies against the hsp70 major heat shock protein family for the development of an immunoassay.

Author

Margulis BA, Nacharov PV, Tsvetkova OI, Welsh M, and Kinev AV

Subjects
Enzyme-Linked Immunosorbent Assay, HeLa Cells, Humans, Immunoblotting, Precipitin Tests, Antibody Specificity immunology, Heat-Shock Proteins immunology, Immunoassay
Abstract

The hsp70 family of major stress proteins is composed of several different members exhibiting similar structural and functional properties. In order to obtain an antiserum with wide epitope reactivity, rabbits were immunized with a mixture of native and denatured hsp70 purified from bovine muscle by ATP-affinity chromatography. Screening for antibody specificity was performed by a "sandwich" enzyme linked immunosorbent assay (ELISA). Immunoprecipitation and immunoblotting analyses demonstrated that the polyclonal antiserum obtained by us and a monoclonal antibody raised against a different preparation of antigen recognized the same determinant on the native hsp70 molecule (inducible form). With a different specificity the polyclonal antiserum recognized only the denatured monomers of the other members of the hsp70 family. These results are discussed in relation to the immunological features of the hsp70 molecule and to the development of an immunoassay for the detection of hsp70 in cell and tissue extracts.

Published
1991
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