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1. Applying reservoir geochemistry methods to determine working intervals in multilayered field.

Author

Nevestenko, M. A., Tarasova, Y. S., Sadmanova, M. V., and Ermolovsky, A. V.

Subjects
*ROCK analysis, *HYDROCARBON analysis, *PROBLEM solving, *GEOCHEMISTRY, *PYROLYSIS
Abstract

The article presents some examples of applying complex geochemical studies to determine the working intervals in multilayered deposits. Geochemical complex consists of bitumen-luminescence and pyrolysis (Rock-Eval) analyses of rocks, molecular analysis of extracts from rocks, analysis of hydrocarbon fluids for determination of main physical-chemical characteristics and molecular composition of different fractions. Using these methods, it becomes possible to solve problems related to refinement of oil-saturated intervals and to evaluate the contribution of several productive zones of multilayered field to the commingled production. [ABSTRACT FROM AUTHOR]

Published
2023
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2. Geochemical technologies in the study of technogenic products problematic for field exploitation.

Author

Tarasova, Y. S., Nevestenko, M. A., Sadmanova, M. V., Ermolovsky, A. V., Potemkin, I. P., and Polskaya, N. N.

Subjects
*DRILL core analysis, *CORE drilling, *DRILLING muds, *GEOCHEMICAL surveys, *FLUIDS
Abstract

The article presents some examples of applying geochemical survey to the study of technogenic products problematic for field exploitation and development. It describes how the adaptation of traditional geochemical technologies to the study of technogenic products make it possible to solve quickly and efficiently the problems that took place at the oilfield. The methods of physical-chemical and molecular analyses help to understand the nature of different deposits, to detect the presence or absence of oil hydrocarbons in annulus fluids, to identify technogenic contamination of hydrocarbon-base drilling mud in core samples. [ABSTRACT FROM AUTHOR]

Published
2023
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4. SYMBIONTS OF MOLLUSCS OF THE GENERA LYMNAEA AND THEODOXUS IN RESERVOIRS OF CENTRAL POLISSYA

Author

Astakhova, L., Tarasova, Y., and Andriychuk, T.

Subjects
molluscs, synoikia, ectocommensals, parasitism, Central Polissya, Lymnaea, Theodoxus, молюски, синойкія, ектокоменсали, паразитизм, Центральне Полісся
Abstract

In biocenoses molluscs are connected by complex biotic relationships with other organisms. In case of molluscs of the genera Lymnaea and Theodoxus such relationships are most commonly expressed in the forms of synoikia and parasitism. Synoiks of pond are green and blue-green algae, protozoa, coelentera, round, flat, segmented worms, bryozoa, molluscs, arachnids, insects. All of them are ectocommensals that settle on the surface of a shell, in the extrapallial or mantle cavity of the molluscs. The characteritics of synoikia Theodoxus fluviatilis Linnaeus, 1758 and oligochaetes of Chaetogaster limnaei K. Baer, 1827 were identified.It has been found that oligochaetes-symbionts can be fed both a food, that comes directly into the mantle and extrapallial cavity of mollusks, in which they settle, and food that is located outside of these cavities. The «parasite-host» symbiotic relationship between molluscs and the larval form of trematode was researched. By taking up the role of intermediate and secondary host, T. fluviatilis supports life cycles of 5 species of trematodes from 4 families (Notocotylidae, Plagiorchiidae, Echinostomatidae and Allocreadiidae). Lymnaea, that has greater species diversity (19 species), participates in life cycles of 26 species of trematodes from 10 families: Echinostomatidae, Plagiorchiidae, Notocotylidae, Diplostomatidae, Sanguinicolidae, Strigeidae, Schistosomatidae, Fasciolidae, Psilostomatidae, Monorchiidae. The antagonistic symbiosis in the form of «predator–victim» relationship is manifested between molluscs and organisms, for whom they are objects of nutrition. The complex symbiotic relation- ships of molluscs of the genera Lymnaea and Theodoxus with other organisms can be characterized as positive, negative or neutral., В біоценозах молюски пов’язані складними біотичними взаємовідношеннями з іншими організмами. Такі стосунки у молюсків родів Lymnaea та Theodoxus виражені найчастіше у формі синойкії та паразитизму. Синойками ставковикiв є зеленi та синьо-зеленi водоростi, найпростiшi, кишковопорожниннi, круглi, плоскi та кiльчастi черви, моховатки, молюски, павукоподiбнi, комахи. Усi вони є ектокоменсалами, що поселяються на поверхнi черепашки, в екстрапалiальнiй або мантiйнiй порожнинi молюскiв. З’ясовано особливості синойкії Theodoxus fluviatilis Linnaeus, 1758 та олігохети Chaetogaster limnaei K. Baer, 1827. Виявлено, що олігохети-симбіонти можуть живитись як кормом, який надходить безпосередньо у мантійну і екстрапаліальну порожнини молюсків, в яких вони оселяються, так і кормом, що знаходиться за межами цих порожнин. Досліджено симбіотичні відносини молюсків із личинковими формами трематод за типом «паразит–хазяїн». Виступаючи у ролі проміжного й додаткового хазяїна, T. fluviatilis забезпечує перебіг життєвих циклів 5 видів трематод, що належать до 4 родин (Notocotylidae, Plagiorchiidae, Echinostomatidae і Allocreadiidae). Ставковики, маючи більшу видову різноманітність (19 видів), беруть участь у життєвих циклах 26 видів трематод з 10 родин: Echinostomatidae, Plagiorchiidae, Notocotylidae, Diplostomatidae, Sanguinicolidae, Strigeidae, Schistosomatidae, Fasciolidae, Psilostomatidae, Monorchiidae. Антагоністичний симбіоз у формі «хижак– жертва» проявляється у молюсків із організмами, для яких вони є об’єктами живлення. Складні симбіотичні відносини молюсків родів Lymnaea та Theodoxus з іншими організмами можуть бути охарактеризовані як позитивні, негативні або нейтральні.

Published
2019

11. Principles of integrative modelling at studying of plasma and welding processes

Author

Anakhov, S. V., Perminov, E. A., Dzyubich, D. K., Yarushina, M. A., Tarasova, Y. A., Anakhov, S. V., Perminov, E. A., Dzyubich, D. K., Yarushina, M. A., and Tarasova, Y. A.

Abstract

The relevance of the problem subject to the research is conditioned by need for introduction of modern technologies into the educational process and insufficient adaptation of the higher school teachers to the applied information and automated procedures in education and science. The purpose of the publication consists in the analysis of automated procedures efficiency in engineering training and development of structurally functional model of information skills for students and teachers during their teaching in welding and allied technologies. The leading approach to research of this problem is the structurally functional method of the objects studying. This method based on representation of technological structure as hierarchical sequence of the interconnected devices and division of a matter into objects and means of influence that allows to allocate the processes providing functioning between means of influence. In the publication the structurally functional models of information skills formation for students and teachers in engineering and natural-science training are presented. The materials of the publication can be useful for students and teachers at studying of welding and allied technologies and development of scientifically-methodical maintenance for engineering and natural-science disciplines. © 2016 Anakhov et al.

Published
2016

12. The American aid to the Russian reforms at the end of the twentieth century

Author

Tarasova, Y. A., Bolshakova, L. S., Yasenitsky, I. A., Larionova, M. B., Tarasova, Y. A., Bolshakova, L. S., Yasenitsky, I. A., and Larionova, M. B.

Abstract

The importance of the studied problem is caused by the USA’s leading role in the development of modern world order and the economy, its influence in the international economic organizations. The article is aimed at revealing the reasons of choosing neoliberal strategy for Russian reforms, the amount and results of the American financial and technical aid to these reforms. The leading approach of researching this problem is the complex one. It allows finding out economic, internal political, geopolitical and cultural factors which influenced the implementation and the results of the American assistance to the Russian reforms. Authors draw a conclusion about considerable influence of the USA on domestic policy of Russia in the early nineties of the XX century. The amount and the content of the American financial and technical assistance to the Russian government are analyzed. Promises of massive financial aid from the international economic organizations and the USA were realized partially and much later, than it was necessary for economic transformations. The article’s content and conclusions can be used in other scientific works on American-Russian relations history, Modern history of Russia, during elaboration the effective strategy of reforms for the countries which are in a condition of a transitional economy. © 2016 Tarasova et al.

Published
2016

14. Biodegradation of organic compounds in wastewater

Author

Salishcheva Olesya, Burlachenko Anastasia, Tarasova Yuliya, Moldagulova Natalia, and Yustratov Vladimir

Subjects
Microbiology, QR1-502, Physiology, QP1-981, Zoology, QL1-991
Abstract

Biodegradation is a sustainable and efficient method for removing organic pollutants from the aquatic environment. We studied the biological purification of aqueous solutions from betaine organic matter under the action of bacterial strains of the genus Pseudomonas and determined the rate of decomposition in the presence of chloride ions and heavy metal cations. The bacteria showed lower activity in the presence of salts of heavy metals and performed more efficiently in the presence of chloride ions. Almost complete degradation of organic matter was observed on the 21st day. Thus, these strains of microorganisms can be used as decomposers of organic betaine compounds.

Published
2023
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15. Training of judiciaries and the effectiveness of the judicial system in Russia

Author

Dolgopolova Tatyana Anatolyevna, Maiboroda Viktor Aleksandrovich, Maiboroda Elvira Tagirovna, Potapov Yuri Alekseevich, and Tarasova Yulia Nikolaevna

Subjects
judiciary, personnel, career, ideal judge, Social Sciences
Abstract

The article examines the theoretical, legal, social and psychological aspects of the formation of a highly effective judiciary in Russia on the basis of a systematic approach in the preparation and selection of personnel for the judicial system. The authors substantiate the most significant tasks of forming the professional identity of Russian judges based on social and psychological research, practical experience of legal personnel, information educational technologies, and analyze the results of assessing the effectiveness of the Russian judicial system according to European standards. When writing the article, general scientific and special research methods were used: structural and functional analysis, comparative legal and analytical methods. The research carried out by the authors made it possible to obtain the following results: to form a comprehensive idea of the identity of a judge based on the concepts of self-esteem, behavior control, communication characteristics and social abilities. It is possible to use these results in the academic process of educational institutions of secondary vocational education and higher education, in the selection of personnel and social and psychological support for the activities of judges and employees of the judicial apparatus. The importance of such studies is associated with the high social significance of this type of activity, its impact on the level of social trust in law and legality.

Published
2021
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16. Some Aspect of Legal Regulation of Special Economic Zones in Russia

Author

Tarasova Yu.A., Kozhevnikova S.A., Bobkova T.S., and Porunova O.G.

Subjects
special economic zones, legal regulation, direct investments, benefits and preferences, infrastructure, zone of industrial and production type, Social Sciences
Abstract

The authors analyze the Russian and international experience of functioning of territories with special legal status. The multiple advantages of establishing and developing of such territories in the country in the short-term and long term are noted. On the basis of the analysis of the Federal Law “About special economic zones in the Russian Federation” and the other normative legal acts, the advantages and the shortcomings of the legal regulation of the creation, management and closing of the special economic zones are revealed. The factors defining a set of privileges for the foreign investors in various territories with special legal status and also the conditions of the effective work of the special economic zone of industrial and production type are considered. The authors support their analysis of the legislation with the description and comparison of economic indicators of work of two special economic zones of industrial and production type in the Volga Federal District. The authors also consider jurisprudence on the controversial issues arising in the connection with the establishment of special economic zones. The article comes to the end with the consideration of possible prospects of the territories with special legal status transformation.

Published
2019
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17. Author Correction: A genomic mutational constraint map using variation in 76,156 human genomes.

Author

Chen S, Francioli LC, Goodrich JK, Collins RL, Kanai M, Wang Q, Alföldi J, Watts NA, Vittal C, Gauthier LD, Poterba T, Wilson MW, Tarasova Y, Phu W, Grant R, Yohannes MT, Koenig Z, Farjoun Y, Banks E, Donnelly S, Gabriel S, Gupta N, Ferriera S, Tolonen C, Novod S, Bergelson L, Roazen D, Ruano-Rubio V, Covarrubias M, Llanwarne C, Petrillo N, Wade G, Jeandet T, Munshi R, Tibbetts K, O'Donnell-Luria A, Solomonson M, Seed C, Martin AR, Talkowski ME, Rehm HL, Daly MJ, Tiao G, Neale BM, MacArthur DG, and Karczewski KJ

Published
2024
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18. A genomic mutational constraint map using variation in 76,156 human genomes.

Author

Chen S, Francioli LC, Goodrich JK, Collins RL, Kanai M, Wang Q, Alföldi J, Watts NA, Vittal C, Gauthier LD, Poterba T, Wilson MW, Tarasova Y, Phu W, Grant R, Yohannes MT, Koenig Z, Farjoun Y, Banks E, Donnelly S, Gabriel S, Gupta N, Ferriera S, Tolonen C, Novod S, Bergelson L, Roazen D, Ruano-Rubio V, Covarrubias M, Llanwarne C, Petrillo N, Wade G, Jeandet T, Munshi R, Tibbetts K, O'Donnell-Luria A, Solomonson M, Seed C, Martin AR, Talkowski ME, Rehm HL, Daly MJ, Tiao G, Neale BM, MacArthur DG, and Karczewski KJ

Subjects
Humans, Access to Information, Databases, Genetic, Datasets as Topic, Gene Frequency, Selection, Genetic, Genome, Human genetics, Genomics, Models, Genetic, Mutation genetics
Abstract

The depletion of disruptive variation caused by purifying natural selection (constraint) has been widely used to investigate protein-coding genes underlying human disorders 1-4 , but attempts to assess constraint for non-protein-coding regions have proved more difficult. Here we aggregate, process and release a dataset of 76,156 human genomes from the Genome Aggregation Database (gnomAD)-the largest public open-access human genome allele frequency reference dataset-and use it to build a genomic constraint map for the whole genome (genomic non-coding constraint of haploinsufficient variation (Gnocchi)). We present a refined mutational model that incorporates local sequence context and regional genomic features to detect depletions of variation. As expected, the average constraint for protein-coding sequences is stronger than that for non-coding regions. Within the non-coding genome, constrained regions are enriched for known regulatory elements and variants that are implicated in complex human diseases and traits, facilitating the triangulation of biological annotation, disease association and natural selection to non-coding DNA analysis. More constrained regulatory elements tend to regulate more constrained protein-coding genes, which in turn suggests that non-coding constraint can aid the identification of constrained genes that are as yet unrecognized by current gene constraint metrics. We demonstrate that this genome-wide constraint map improves the identification and interpretation of functional human genetic variation., (© 2023. The Author(s), under exclusive licence to Springer Nature Limited.)

Published
2024
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19. Two clinical case reports of embryonic mosaicism identified with PGT-A persisting during pregnancy as true fetal mosaicism.

Author

Greco E, Yakovlev P, Kornilov N, Vyatkina S, Bogdanova D, Ermakova M, Tarasova Y, Tikhonov A, Pendina A, Biricik A, Sessa MT, Listorti I, Ronsini C, Greco PF, Victor A, Barnes F, Zouves C, Spinella F, and Viotti M

Subjects
Pregnancy, Female, Humans, Male, Prospective Studies, Chromosomes, Human, Y, Blastocyst pathology, Genetic Testing methods, Aneuploidy, Fetus, Mosaicism, Preimplantation Diagnosis methods
Abstract

The health risks associated with transferring embryos classified as mosaic by preimplantation genetic testing for aneuploidies (PGT-A) are currently unknown. Such embryos produce PGT-A results indicating the presence of both euploid and aneuploid cells and have historically been deselected from transfer and grouped with uniformly aneuploid embryos as 'abnormal'. In recent years, numerous groups have reported the intentional transfer of mosaic embryos in the absence of uniformly euploid embryos, largely observing births of seemingly healthy babies. However, it remains to be understood whether the embryonic mosaicism invariably becomes resolved during the ensuing pregnancy, or whether the placenta and/or fetal tissues retain aneuploid cells, and if so to what potential clinical effect. Here, we report two cases of mosaicism persisting from the embryonic stage to the established pregnancy. Case 1 involved an embryonic low-level segmental mosaic loss in Chromosome (Chr) 1, which was confirmed in amniocentesis as well as in brain tissue of the products of conception. This pregnancy was terminated due to the chromosomal pathologies associated with 1p36 deletion syndrome, such as severe intellectual disability. Case 2 involved a low-level mosaic Chr 21 trisomy, which was confirmed with chorionic villus sampling and amniocentesis. The ensuing pregnancy was terminated after ultrasound identification of severe abnormalities in the placenta and fetus. Together, these two cases should be taken into account for risk-benefit assessments of prospective mosaic embryo transfers., (© The Author(s) 2023. Published by Oxford University Press on behalf of European Society of Human Reproduction and Embryology. All rights reserved. For permissions, please email: journals.permissions@oup.com.)

Published
2023
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20. The Validation of the Sample6 DETECT TM HT/L for AOAC Research Institute.

Author

Banerjee K, Peirson B, Hu C, Carrier E, Malsick L, Tarasova Y, Daudenarde S, Brownell D, Koeris M, Klass N, Bird P, Benzinger MJ, Agin J, and Goins D

Subjects
Environmental Monitoring methods, Food Contamination analysis, Food Microbiology, Humans, Limit of Detection, Listeria classification, Listeria monocytogenes classification, Listeria monocytogenes isolation & purification, Listeriosis microbiology, Bacterial Typing Techniques methods, Listeria isolation & purification, Reagent Kits, Diagnostic, Stainless Steel analysis
Abstract

Background: Listeria spp. are an important foodborne human pathogen because of their ability to cause disease and high mortality in individuals, particularly pregnant women, neonates, the elderly, immunocompromised individuals, and children. The Sample6 DETECTTM HT/L Kit is a semi-automated qualitative pathogen detection system designed to detect Listeria spp. (L. monocytogenes, L. innocua, L. ivanovii, L. seeligeri, L. welshimeri, and L. marthii) in environmental samples using the Sample6 BioIlluminationTM technology., Objective: The study was done to evaluate the Sample6 DETECT HT/L Kit. The assay was evaluated for inclusivity, exclusivity, robustness, product consistency, and stability, and a matrix study of one environmental surface., Methods: The performance of the Sample6 DETECT HT/L was compared with U.S. Food and Drug Administration reference culture method for Listeria using an unpaired study design., Results: The Sample6 DETECT HT/L assay correctly identified all 50 inclusivity isolates and correctly excluded all 30 nontarget strains evaluated. The assay was not affected by minor variations in incubation temperature and time, or sample volume. Results across three production lots spanning the shelf life of the assay were consistent. In the matrix study, the Sample6 DETECT HT/L for Listeria correctly identified each test portion for the presence or absence of Listeria, and there were no statistically significant differences between candidate and reference method results., Conclusions: The data collected in this study demonstrate that the Sample6 DETECT HT/L assay is a reliable method for the detection of Listeria spp. on stainless-steel environmental surfaces after 22 h of enrichment.

Published
2018
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21. Rational design of thiolase substrate specificity for metabolic engineering applications.

Author

Bonk BM, Tarasova Y, Hicks MA, Tidor B, and Prather KLJ

Subjects
Escherichia coli genetics, Escherichia coli metabolism, Megasphaera elsdenii enzymology, Megasphaera elsdenii genetics, Substrate Specificity, Acetyl-CoA C-Acetyltransferase genetics, Acetyl-CoA C-Acetyltransferase metabolism, Metabolic Engineering methods, Mutant Proteins genetics, Mutant Proteins metabolism
Abstract

Metabolic engineering efforts require enzymes that are both highly active and specific toward the synthesis of a desired output product to be commercially feasible. The 3-hydroxyacid (3HA) pathway, also known as the reverse β-oxidation or coenzyme-A-dependent chain-elongation pathway, can allow for the synthesis of dozens of useful compounds of various chain lengths and functionalities. However, this pathway suffers from byproduct formation, which lowers the yields of the desired longer chain products, as well as increases downstream separation costs. The thiolase enzyme catalyzes the first reaction in this pathway, and its substrate specificity at each of its two catalytic steps sets the chain length and composition of the chemical scaffold upon which the other downstream enzymes act. However, there have been few attempts reported in the literature to rationally engineer thiolase substrate specificity. In this study, we present a model-guided, rational design study of ordered substrate binding applied to two biosynthetic thiolases, with the goal of increasing the ratio of C6/C4 products formed by the 3HA pathway, 3-hydroxy-hexanoic acid and 3-hydroxybutyric acid. We identify thiolase mutants that result in nearly 10-fold increases in C6/C4 selectivity. Our findings can extend to other pathways that employ the thiolase for chain elongation, as well as expand our knowledge of sequence-structure-function relationship for this important class of enzymes., (© 2018 Wiley Periodicals, Inc.)

Published
2018
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22. Ascorbic acid promotes cardiomyogenesis through SMAD1 signaling in differentiating mouse embryonic stem cells.

Author

Perino MG, Yamanaka S, Riordon DR, Tarasova Y, and Boheler KR

Subjects
Animals, Embryonic Stem Cells cytology, Mice, Myocytes, Cardiac cytology, Myocytes, Cardiac metabolism, Ascorbic Acid pharmacology, Cell Differentiation drug effects, Embryonic Stem Cells drug effects, Myocytes, Cardiac drug effects, Signal Transduction drug effects, Smad1 Protein metabolism
Abstract

Numerous groups have documented that Ascorbic Acid (AA) promotes cardiomyocyte differentiation from both mouse and human ESCs and iPSCs. AA is now considered indispensable for the routine production of hPSC-cardiomyocytes (CMs) using defined media; however, the mechanisms involved with the inductive process are poorly understood. Using a genetically modified mouse embryonic stem cell (mESC) line containing a dsRED transgene driven by the cardiac-restricted portion of the ncx1 promoter, we show that AA promoted differentiation of mESCs to CMs in a dose- and time-dependent manner. Treatment of mPSCs with AA did not modulate total SMAD content; however, the phosphorylated/active forms of SMAD2 and SMAD1/5/8 were significantly elevated. Co-administration of the SMAD2/3 activator Activin A with AA had no significant effect, but the addition of the nodal co-receptor TDGF1 (Cripto) antagonized AA's cardiomyogenic-promoting ability. AA could also reverse some of the inhibitory effects on cardiomyogenesis of ALK/SMAD2 inhibition by SB431542, a TGFβ pathway inhibitor. Treatment with BMP2 and AA strongly amplified the positive cardiomyogenic effects of SMAD1/5/8 in a dose-dependent manner. AA could not, however, rescue dorsomorphin-mediated inhibition of ALK/SMAD1 activity. Using an inducible model system, we found that SMAD1, but not SMAD2, was essential for AA to promote the formation of TNNT2+-CMs. These data firmly demonstrate that BMP receptor-activated SMADs, preferential to TGFβ receptor-activated SMADs, are necessary to promote AA stimulated cardiomyogenesis. AA-enhanced cardiomyogenesis thus relies on the ability of AA to modulate the ratio of SMAD signaling among the TGFβ-superfamily receptor signaling pathways.

Published
2017
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23. Adaptive Evolution of Thermotoga maritima Reveals Plasticity of the ABC Transporter Network.

Author

Latif H, Sahin M, Tarasova J, Tarasova Y, Portnoy VA, Nogales J, and Zengler K

Subjects
Carbon metabolism, Gene Expression Profiling, Genome, Bacterial, Glucose metabolism, Metabolic Networks and Pathways genetics, Molecular Sequence Data, Sequence Analysis, DNA, Thermotoga maritima growth & development, Thermotoga maritima metabolism, ATP-Binding Cassette Transporters genetics, ATP-Binding Cassette Transporters metabolism, Adaptation, Biological, Mutation, Thermotoga maritima physiology
Abstract

Thermotoga maritima is a hyperthermophilic anaerobe that utilizes a vast network of ABC transporters to efficiently metabolize a variety of carbon sources to produce hydrogen. For unknown reasons, this organism does not metabolize glucose as readily as it does glucose di- and polysaccharides. The leading hypothesis implicates the thermolability of glucose at the physiological temperatures at which T. maritima lives. After a 25-day laboratory evolution, phenotypes were observed with growth rates up to 1.4 times higher than and glucose utilization rates exceeding 50% those of the wild type. Genome resequencing revealed mutations in evolved cultures related to glucose-responsive ABC transporters. The native glucose ABC transporter, GluEFK, has more abundant transcripts either as a result of gene duplication-amplification or through mutations to the operator sequence regulating this operon. Conversely, BglEFGKL, a transporter of beta-glucosides, is substantially downregulated due to a nonsense mutation to the solute binding protein or due to a deletion of the upstream promoter. Analysis of the ABC2 uptake porter families for carbohydrate and peptide transport revealed that the solute binding protein, often among the transcripts detected at the highest levels, is predominantly downregulated in the evolved cultures, while the membrane-spanning domain and nucleotide binding components are less varied. Similar trends were observed in evolved strains grown on glycerol, a substrate that is not dependent on ABC transporters. Therefore, improved growth on glucose is achieved through mutations favoring GluEFK expression over BglEFGKL, and in lieu of carbon catabolite repression, the ABC transporter network is modulated to achieve improved growth fitness., (Copyright © 2015, American Society for Microbiology. All Rights Reserved.)

Published
2015
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24. Engineering E. coli for the biosynthesis of 3-hydroxy-γ-butyrolactone (3HBL) and 3,4-dihydroxybutyric acid (3,4-DHBA) as value-added chemicals from glucose as a sole carbon source.

Author

Dhamankar H, Tarasova Y, Martin CH, and Prather KL

Subjects
4-Butyrolactone biosynthesis, Cell Proliferation physiology, Computer Simulation, Models, Biological, 4-Butyrolactone analogs & derivatives, Butylene Glycols metabolism, Butyrates metabolism, Escherichia coli physiology, Escherichia coli Proteins physiology, Genetic Enhancement methods, Glucose metabolism, Metabolic Engineering methods
Abstract

3-hydroxy-γ-butyrolactone (3HBL) is a versatile chiral synthon, deemed a top value-added chemical from biomass by the DOE. We recently reported the first biosynthetic pathway towards 3HBL and its hydrolyzed form, 3,4-dihydroxybutyric acid (3,4-DHBA) in recombinant Escherichia coli using glucose and glycolic acid as feedstocks and briefly described their synthesis solely from glucose. Synthesis from glucose requires integration of the endogenous glyoxylate shunt with the 3,4-DHBA/3HBL pathway and co-overexpression of seven genes, posing challenges with respect to expression, repression of the glyoxylate shunt and optimal carbon distribution between the two pathways. Here we discuss engineering this integration. While appropriate media and over-expression of glyoxylate shunt enzymes helped overcome repression, two orthogonal expression systems were employed to address the expression and carbon distribution challenge. Synthesis of up to 0.3g/L of 3HBL and 0.7g/L of 3,4-DHBA solely from glucose was demonstrated, amounting to 24% of the theoretical maximum., (Copyright © 2014 International Metabolic Engineering Society. Published by Elsevier Inc. All rights reserved.)

Published
2014
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25. Synthesis and accumulation of aromatic aldehydes in an engineered strain of Escherichia coli.

Author

Kunjapur AM, Tarasova Y, and Prather KL

Subjects
Aldehydes chemistry, Escherichia coli chemistry, Molecular Structure, Aldehydes metabolism, Escherichia coli genetics, Escherichia coli metabolism, Metabolic Engineering
Abstract

Aromatic aldehydes are useful in numerous applications, especially as flavors, fragrances, and pharmaceutical precursors. However, microbial synthesis of aldehydes is hindered by rapid, endogenous, and redundant conversion of aldehydes to their corresponding alcohols. We report the construction of an Escherichia coli K-12 MG1655 strain with reduced aromatic aldehyde reduction (RARE) that serves as a platform for aromatic aldehyde biosynthesis. Six genes with reported activity on the model substrate benzaldehyde were rationally targeted for deletion: three genes that encode aldo-keto reductases and three genes that encode alcohol dehydrogenases. Upon expression of a recombinant carboxylic acid reductase in the RARE strain and addition of benzoate during growth, benzaldehyde remained in the culture after 24 h, with less than 12% conversion of benzaldehyde to benzyl alcohol. Although individual overexpression results demonstrated that all six genes could contribute to benzaldehyde reduction in vivo, additional experiments featuring subset deletion strains revealed that two of the gene deletions were dispensable under the conditions tested. The engineered strain was next investigated for the production of vanillin from vanillate and succeeded in preventing formation of the byproduct vanillyl alcohol. A pathway for the biosynthesis of vanillin directly from glucose was introduced and resulted in a 55-fold improvement in vanillin titer when using the RARE strain versus the wild-type strain. Finally, synthesis of the chiral pharmaceutical intermediate L-phenylacetylcarbinol (L-PAC) was demonstrated from benzaldehyde and glucose upon expression of a recombinant mutant pyruvate decarboxylase in the RARE strain. Beyond allowing accumulation of aromatic aldehydes as end products in E. coli, the RARE strain expands the classes of chemicals that can be produced microbially via aldehyde intermediates.

Published
2014
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26. Transcriptional regulation of the carbohydrate utilization network in Thermotoga maritima.

Author

Rodionov DA, Rodionova IA, Li X, Ravcheev DA, Tarasova Y, Portnoy VA, Zengler K, and Osterman AL

Abstract

Hyperthermophilic bacteria from the Thermotogales lineage can produce hydrogen by fermenting a wide range of carbohydrates. Previous experimental studies identified a large fraction of genes committed to carbohydrate degradation and utilization in the model bacterium Thermotoga maritima. Knowledge of these genes enabled comprehensive reconstruction of biochemical pathways comprising the carbohydrate utilization network. However, transcriptional factors (TFs) and regulatory mechanisms driving this network remained largely unknown. Here, we used an integrated approach based on comparative analysis of genomic and transcriptomic data for the reconstruction of the carbohydrate utilization regulatory networks in 11 Thermotogales genomes. We identified DNA-binding motifs and regulons for 19 orthologous TFs in the Thermotogales. The inferred regulatory network in T. maritima contains 181 genes encoding TFs, sugar catabolic enzymes and ABC-family transporters. In contrast to many previously described bacteria, a transcriptional regulation strategy of Thermotoga does not employ global regulatory factors. The reconstructed regulatory network in T. maritima was validated by gene expression profiling on a panel of mono- and disaccharides and by in vitro DNA-binding assays. The observed upregulation of genes involved in catabolism of pectin, trehalose, cellobiose, arabinose, rhamnose, xylose, glucose, galactose, and ribose showed a strong correlation with the UxaR, TreR, BglR, CelR, AraR, RhaR, XylR, GluR, GalR, and RbsR regulons. Ultimately, this study elucidated the transcriptional regulatory network and mechanisms controlling expression of carbohydrate utilization genes in T. maritima. In addition to improving the functional annotations of associated transporters and catabolic enzymes, this research provides novel insights into the evolution of regulatory networks in Thermotogales.

Published
2013
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27. The genome organization of Thermotoga maritima reflects its lifestyle.

Author

Latif H, Lerman JA, Portnoy VA, Tarasova Y, Nagarajan H, Schrimpe-Rutledge AC, Smith RD, Adkins JN, Lee DH, Qiu Y, and Zengler K

Subjects
5' Untranslated Regions, Life Style, Molecular Sequence Data, Transcription Initiation Site, Gene Expression Profiling, Thermotoga maritima genetics
Abstract

The generation of genome-scale data is becoming more routine, yet the subsequent analysis of omics data remains a significant challenge. Here, an approach that integrates multiple omics datasets with bioinformatics tools was developed that produces a detailed annotation of several microbial genomic features. This methodology was used to characterize the genome of Thermotoga maritima--a phylogenetically deep-branching, hyperthermophilic bacterium. Experimental data were generated for whole-genome resequencing, transcription start site (TSS) determination, transcriptome profiling, and proteome profiling. These datasets, analyzed in combination with bioinformatics tools, served as a basis for the improvement of gene annotation, the elucidation of transcription units (TUs), the identification of putative non-coding RNAs (ncRNAs), and the determination of promoters and ribosome binding sites. This revealed many distinctive properties of the T. maritima genome organization relative to other bacteria. This genome has a high number of genes per TU (3.3), a paucity of putative ncRNAs (12), and few TUs with multiple TSSs (3.7%). Quantitative analysis of promoters and ribosome binding sites showed increased sequence conservation relative to other bacteria. The 5'UTRs follow an atypical bimodal length distribution comprised of "Short" 5'UTRs (11-17 nt) and "Common" 5'UTRs (26-32 nt). Transcriptional regulation is limited by a lack of intergenic space for the majority of TUs. Lastly, a high fraction of annotated genes are expressed independent of growth state and a linear correlation of mRNA/protein is observed (Pearson r = 0.63, p<2.2 × 10(-16) t-test). These distinctive properties are hypothesized to be a reflection of this organism's hyperthermophilic lifestyle and could yield novel insights into the evolutionary trajectory of microbial life on earth., Competing Interests: The authors have declared that no competing interests exist.

Published
2013
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28. The extracellular matrix Component Psl provides fast-acting antibiotic defense in Pseudomonas aeruginosa biofilms.

Author

Billings N, Millan M, Caldara M, Rusconi R, Tarasova Y, Stocker R, and Ribbeck K

Subjects
Anti-Bacterial Agents pharmacology, Drug Resistance, Bacterial drug effects, Escherichia coli genetics, Escherichia coli metabolism, Polysaccharides, Bacterial genetics, Pseudomonas aeruginosa genetics, Staphylococcus aureus genetics, Staphylococcus aureus metabolism, Anti-Bacterial Agents metabolism, Biofilms, Drug Resistance, Bacterial physiology, Polysaccharides, Bacterial metabolism, Pseudomonas aeruginosa metabolism
Abstract

Bacteria within biofilms secrete and surround themselves with an extracellular matrix, which serves as a first line of defense against antibiotic attack. Polysaccharides constitute major elements of the biofilm matrix and are implied in surface adhesion and biofilm organization, but their contributions to the resistance properties of biofilms remain largely elusive. Using a combination of static and continuous-flow biofilm experiments we show that Psl, one major polysaccharide in the Pseudomonas aeruginosa biofilm matrix, provides a generic first line of defense toward antibiotics with diverse biochemical properties during the initial stages of biofilm development. Furthermore, we show with mixed-strain experiments that antibiotic-sensitive "non-producing" cells lacking Psl can gain tolerance by integrating into Psl-containing biofilms. However, non-producers dilute the protective capacity of the matrix and hence, excessive incorporation can result in the collapse of resistance of the entire community. Our data also reveal that Psl mediated protection is extendible to E. coli and S. aureus in co-culture biofilms. Together, our study shows that Psl represents a critical first bottleneck to the antibiotic attack of a biofilm community early in biofilm development.

Published
2013
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29. A cell surfaceome map for immunophenotyping and sorting pluripotent stem cells.

Author

Gundry RL, Riordon DR, Tarasova Y, Chuppa S, Bhattacharya S, Juhasz O, Wiedemeier O, Milanovich S, Noto FK, Tchernyshyov I, Raginski K, Bausch-Fluck D, Tae HJ, Marshall S, Duncan SA, Wollscheid B, Wersto RP, Rao S, Van Eyk JE, and Boheler KR

Subjects
Animals, Cells, Cultured, Cytokine Receptor gp130 analysis, Embryo, Mammalian cytology, Embryonic Stem Cells cytology, Embryonic Stem Cells metabolism, Embryonic Stem Cells transplantation, Fibroblasts cytology, Fibroblasts metabolism, Flow Cytometry, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Induced Pluripotent Stem Cells cytology, Induced Pluripotent Stem Cells metabolism, Induced Pluripotent Stem Cells transplantation, Mass Spectrometry, Mice, Mice, 129 Strain, Mice, Transgenic, Microscopy, Confocal, Octamer Transcription Factor-3 genetics, Octamer Transcription Factor-3 metabolism, Pluripotent Stem Cells cytology, Teratoma metabolism, Teratoma pathology, Cell Separation methods, Glycoproteins analysis, Immunophenotyping methods, Membrane Proteins analysis, Pluripotent Stem Cells metabolism, Proteomics methods
Abstract

Induction of a pluripotent state in somatic cells through nuclear reprogramming has ushered in a new era of regenerative medicine. Heterogeneity and varied differentiation potentials among induced pluripotent stem cell (iPSC) lines are, however, complicating factors that limit their usefulness for disease modeling, drug discovery, and patient therapies. Thus, there is an urgent need to develop nonmutagenic rapid throughput methods capable of distinguishing among putative iPSC lines of variable quality. To address this issue, we have applied a highly specific chemoproteomic targeting strategy for de novo discovery of cell surface N-glycoproteins to increase the knowledge-base of surface exposed proteins and accessible epitopes of pluripotent stem cells. We report the identification of 500 cell surface proteins on four embryonic stem cell and iPSCs lines and demonstrate the biological significance of this resource on mouse fibroblasts containing an oct4-GFP expression cassette that is active in reprogrammed cells. These results together with immunophenotyping, cell sorting, and functional analyses demonstrate that these newly identified surface marker panels are useful for isolating iPSCs from heterogeneous reprogrammed cultures and for isolating functionally distinct stem cell subpopulations.

Published
2012
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30. Deletion of genes encoding cytochrome oxidases and quinol monooxygenase blocks the aerobic-anaerobic shift in Escherichia coli K-12 MG1655.

Author

Portnoy VA, Scott DA, Lewis NE, Tarasova Y, Osterman AL, and Palsson BØ

Subjects
Aerobiosis, Anaerobiosis, Carbon Isotopes metabolism, Citric Acid Cycle, Electron Transport Complex IV metabolism, Escherichia coli K12 genetics, Escherichia coli Proteins metabolism, Glycolysis, Lactic Acid metabolism, Mixed Function Oxygenases metabolism, Oxygen metabolism, Staining and Labeling methods, Ubiquinone metabolism, Vitamin K 2 metabolism, Bacterial Outer Membrane Proteins biosynthesis, Electron Transport Complex IV genetics, Escherichia coli K12 metabolism, Escherichia coli Proteins biosynthesis, Gene Deletion, Gene Expression Regulation, Bacterial, Mixed Function Oxygenases deficiency, Repressor Proteins biosynthesis
Abstract

The constitutive activation of the anoxic redox control transcriptional regulator (ArcA) in Escherichia coli during aerobic growth, with the consequent production of a strain that exhibits anaerobic physiology even in the presence of air, is reported in this work. Removal of three terminal cytochrome oxidase genes (cydAB, cyoABCD, and cbdAB) and a quinol monooxygenase gene (ygiN) from the E. coli K-12 MG1655 genome resulted in the activation of ArcA aerobically. These mutations resulted in reduction of the oxygen uptake rate by nearly 98% and production of d-lactate as a sole by-product under oxic and anoxic conditions. The knockout strain exhibited nearly identical physiological behaviors under both conditions, suggesting that the mutations resulted in significant metabolic and regulatory perturbations. In order to fully understand the physiology of this mutant and to identify underlying metabolic and regulatory reasons that prevent the transition from an aerobic to an anaerobic phenotype, we utilized whole-genome transcriptome analysis, (13)C tracing experiments, and physiological characterization. Our analysis showed that the deletions resulted in the activation of anaerobic respiration under oxic conditions and a consequential shift in the content of the quinone pool from ubiquinones to menaquinones. An increase in menaquinone concentration resulted in the activation of ArcA. The activation of the ArcB/ArcA regulatory system led to a major shift in the metabolic flux distribution through the central metabolism of the mutant strain. Flux analysis indicated that the mutant strain had undetectable fluxes around the tricarboxylic acid (TCA) cycle and elevated flux through glycolysis and anaplerotic input to oxaloacetate. Flux and transcriptomics data were highly correlated and showed similar patterns.

Published
2010
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31. Expanding the mouse embryonic stem cell proteome: combining three proteomic approaches.

Author

Gundry RL, Tchernyshyov I, Sheng S, Tarasova Y, Raginski K, Boheler KR, and Van Eyk JE

Subjects
Animals, Cell Line, Databases, Protein, Mice, Pluripotent Stem Cells metabolism, Embryonic Stem Cells metabolism, Proteome metabolism, Proteomics methods
Abstract

The current study used three different proteomic strategies, which differed by their extent of intact protein separation, to examine the proteome of a pluripotent mouse embryonic stem cell line, R1. Proteins from whole-cell lysates were subjected either to 2-D-LC, or 1-DE, or were unfractionated prior to enzymatic digestion and subsequent analysis by MS. The results yielded 1895 identified non-redundant proteins and, for 128 of these, the specific isoform could be determined based on detection of an isoform-specific peptide. When compared with two previously published proteomic studies that used the same cell line, the current study reveals 612 new proteins.

Published
2010
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32. The mouse C2C12 myoblast cell surface N-linked glycoproteome: identification, glycosite occupancy, and membrane orientation.

Author

Gundry RL, Raginski K, Tarasova Y, Tchernyshyov I, Bausch-Fluck D, Elliott ST, Boheler KR, Van Eyk JE, and Wollscheid B

Subjects
Animals, Aquaporin 1 chemistry, Binding Sites, Cell Differentiation, Cell Membrane metabolism, Glycoproteins chemistry, Glycosylation, Mice, Models, Biological, Sarcoglycans chemistry, Membrane Proteins metabolism, Myoblasts metabolism, Proteome chemistry, Proteomics methods
Abstract

Endogenous regeneration and repair mechanisms are responsible for replacing dead and damaged cells to maintain or enhance tissue and organ function, and one of the best examples of endogenous repair mechanisms involves skeletal muscle. Although the molecular mechanisms that regulate the differentiation of satellite cells and myoblasts toward myofibers are not fully understood, cell surface proteins that sense and respond to their environment play an important role. The cell surface capturing technology was used here to uncover the cell surface N-linked glycoprotein subproteome of myoblasts and to identify potential markers of myoblast differentiation. 128 bona fide cell surface-exposed N-linked glycoproteins, including 117 transmembrane, four glycosylphosphatidylinositol-anchored, five extracellular matrix, and two membrane-associated proteins were identified from mouse C2C12 myoblasts. The data set revealed 36 cluster of differentiation-annotated proteins and confirmed the occupancy for 235 N-linked glycosylation sites. The identification of the N-glycosylation sites on the extracellular domain of the proteins allowed for the determination of the orientation of the identified proteins within the plasma membrane. One glycoprotein transmembrane orientation was found to be inconsistent with Swiss-Prot annotations, whereas ambiguous annotations for 14 other proteins were resolved. Several of the identified N-linked glycoproteins, including aquaporin-1 and beta-sarcoglycan, were found in validation experiments to change in overall abundance as the myoblasts differentiate toward myotubes. Therefore, the strategy and data presented shed new light on the complexity of the myoblast cell surface subproteome and reveal new targets for the clinically important characterization of cell intermediates during myoblast differentiation into myotubes.

Published
2009
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33. Cardiomyocytes derived from embryonic stem cells.

Author

Boheler KR, Crider DG, Tarasova Y, and Maltsev VA

Subjects
Animals, Base Sequence, Cell Differentiation, Cells, Cultured, DNA Primers, Fluorescent Antibody Technique, Mice, Embryo, Mammalian cytology, Myocardium cytology, Stem Cells cytology
Abstract

Self-renewing embryonic stem (ES) cells have been established from early mouse embryos as permanent cell lines. By cultivation in vitro as three-dimensional aggregates called embryoid bodies (EBs), ES cells can differentiate into derivatives of all three primary germ layers, including cardiomyocytes. ES cells thus represent a useful model system for studying cardiomyocyte developmental paradigms. This chapter describes techniques and protocols for the cultivation and maintenance of ES cell lines, and the differentiation of ES cell lines into all specialized cell types of the heart, including atrial-, ventricular-, sinus nodal- and Purkinje-like cardiomyocytes. We also include protocols for the isolation and evaluation (morphological, molecular, and functional) of in vitro-generated cardiomyocytes. We consider these latter techniques to be prerequisites for the successful use of this model system to study cardiomyocyte differentiation. Finally, our objective in writing this chapter is to provide sufficient detail and explanation so that any competent scientist who is new to the field will be able to successfully establish and employ this model system for the analysis of ES cell-derived cardiomyocytes.

Published
2005
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