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3. Polymorphisms in GDF9 and BMP15 Associated with Fertility and Ovulation Rate in Moghani and Ghezel Sheep in Iran.

Author

Barzegari, A., Atashpaz, S., Ghabili, K., Nemati, Z., Rustaei, M., and Azarbaijani, R.

Subjects
*SHEEP, *ANIMAL breeds, *OVULATION, *GENETIC mutation, *GENETIC polymorphisms
Abstract

Contents The genetic base of fertility and ovulation rate in Moghani and Ghezel sheep in northwestern Iran and northeastern Turkey is important because of their fat-tailed meat and carpet quality wool. The genes encoding bone morphogenetic (BM) protein 15 and growth differentiation (GD) factor 9, respectively BMP15 and GDF9 have been shown to affect female productivity in domesticated sheep. Recently, numerous investigations have been performed on a variety of breeds to determine the association between mutations in these genes and fertility. Thus, in this study, we assessed such mutations in the Moghani and Ghezel breeds using polymerase chain reaction (PCR)-based restriction fragment length polymorphism (RFLP) with appropriate enzymes. Our data were similar to those of the previous studies showing that the genotypes were heterozygous for GD (G →A) and BM (C →T) mutations. These heterozygous genotypes resulted in higher ovulation rates, illustrating that one copy of each of the BMP15 and GDF9 mutations had equivalent effects on the ovulation rate. We demonstrate for the first time that the BM variant may not be sufficient on its own for infertility. In addition, although the previous studies have shown no notable relationship between the GD variant, known as the non-effecting mutation and sterility, we report that this mutation has an important role in the Moghani and Ghezel breeds. [ABSTRACT FROM AUTHOR]

Published
2010
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4. Cloning of taxadiene synthase gene into Arabidopsis thaliana (ecotype Columbia-0)

Author

Khani, S., Sohani, M. M., Mahna, N., Barar, J., Hejazi, M. S., Nazemieh, H., Atashpaz, S., Dadpour, M. R., and Yadollah Omidi

Subjects
chemistry.chemical_classification, Cloning, biology, Taxadiene, Molecular cloning, biology.organism_classification, Applied Microbiology and Biotechnology, chemistry.chemical_compound, Enzyme, chemistry, Biochemistry, Taxadiene synthase, Paclitaxel, arabidopsis, taxadiene synthase, geranylgeranyl diphosphate, Arabidopsis, Genetics, biology.protein, Arabidopsis thaliana, Agronomy and Crop Science, Molecular Biology, Gene, Biotechnology
Abstract

Paclitaxel (Taxol), a complex diterpenoid, produced by yew tree (Taxus sp.) is the most important chemotherapeutic agent that is widely used against a variety of malignancies such as ovarian and breast cancers. However, destructive methods for its production from natural resources together with currently used low-yielding industrial production systems via total synthesis or semi-synthesis have led researchers to invent a robust alternative biological production system usingbiotechnological approaches. The first committed step in taxol biosynthesis pathway is the production of taxadiene from geranylgeranyl diphosphate (GGPP) catalyzed by the plastid-localized enzyme taxadiene synthase (TXS). In this research, an attempt was made to evaluate the effects of the first critical enzyme in the taxol biosynthesis pathway on Arabidopsis plant through the expression of taxadiene synthase gene under the control of a dexamethasone-inducible promoter.To achieve this goal, Arabidopsis plants (ecotype Columbia-0) were transformed with the construct pTA-TXS-His via floral dip method using Agrobacterium tumefaciens AGL1. The transformed plants were confirmed using the PCR reaction amplifying an 800 bp fragment of the cloned gene. Upon these findings, a proposal was made that biotechnological strategies could be utilized for the production of taxol components. Key words: Paclitaxel, arabidopsis, taxadiene synthase, geranylgeranyl diphosphate. ______________________________________________

8. ATR expands embryonic stem cell fate potential in response to replication stress

Author

Sara Samadi Shams, Endre Sebestyén, Sina Atashpaz, Valeria Cancila, Negar Arghavanifard, Eliene Albers, Javier Martin Gonzalez, Oscar Fernandez-Capetillo, Giovanni Faga, Angela Bachi, Vincenzo Costanzo, Elisa Allievi, Francesco Ferrari, Andrea Gnocchi, Paolo Soffientini, Simone Minardi, Claudio Tripodo, Andrés J. López-Contreras, Atashpaz S., Shams S.S., Gonzalez J.M., Sebestyen E., Arghavanifard N., Gnocchi A., Albers E., Minardi S., Faga G., Soffientini P., Allievi E., Cancila V., Bachi A., Fernandez-Capetillo O., Tripodo C., Ferrari F., Lopez-Contreras A.J., Costanzo V., Italian Association for Cancer Research, Giovanni Armenise-Harvard Foundation, European Research Council, Danish Cancer Society, Det Frie Forskningsrad (DFF), Danish National Research Foundation, Associazione Italiana per la Ricerca sul Cancro (AIRC), European Research Council (ERC), and Danmarks Grundforskningsfond

Subjects
0301 basic medicine, Endogeny, Ataxia Telangiectasia Mutated Proteins, Mice, 0302 clinical medicine, Tandem Mass Spectrometry, Transcription (biology), GENE ATR, cell biology, Cloning, Molecular, Biology (General), Cells, Cultured, 0303 health sciences, General Neuroscience, Totipotent, Cell Differentiation, Embryo, General Medicine, Cell biology, Medicine, biological phenomena, cell phenomena, and immunity, Research Article, QH301-705.5, replication stress, DNA damage, Science, Settore MED/08 - Anatomia Patologica, Biology, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Animals, RNA, Messenger, Gene, Embryonic Stem Cells, mouse, Cell Proliferation, 030304 developmental biology, Messenger RNA, General Immunology and Microbiology, Chimera, Sequence Analysis, RNA, Embryogenesis, TELOMERE ELONGATION, EPIGENETIC RESTRICTION, embryonic stem cell, Embryonic stem cell, ATR, 030104 developmental biology, Gene Expression Regulation, DNA-DAMAGE, Checkpoint Kinase 1, GENOMIC STABILITY, 030217 neurology & neurosurgery, Chromatography, Liquid, DNA Damage
Abstract

Fondazione Italiana per la Ricerca sul Cancro FIRC 18112 Sina Atashpaz.Fondazione Umberto Veronesi Sina Atashpaz Associazione Italiana per la Ricerca sul Cancro AIRC 5xmille METAMECH program Vincenzo Costanzo Giovanni Armenise-Harvard Foundation Vincenzo Costanzo European Research Council Consolidator grant 614541 Vincenzo Costanzo Associazione Italiana per la Ricerca sul Cancro Fellowship 23961 Negar ArghavanifarDanish Cancer Society KBVU-2014 Andres Joaquin Lopez-Contreras Danish Council for Independent Research Sapere Aude, DFF Starting Grant 2014 Andres Joaquin Lopez-Contreras European Research Council ERC-2015-STG-679068 Andres Joaquin Lopez-Contreras Danish National Research Foundation DNRF115 Andres Joaquin Lopez-Contreras The funders had no role in study design, data collection and interpretation, or the decision to submit the work for publication. Unrepaired DNA damage during embryonic development can be potentially inherited by a large population of cells. However, the quality control mechanisms that minimize the contribution of damaged cells to developing embryos remain poorly understood. Here, we uncovered an ATR- and CHK1-mediated transcriptional response to replication stress (RS) in mouse embryonic stem cells (ESCs) that induces genes expressed in totipotent two-cell (2C) stage embryos and 2C-like cells. This response is mediated by Dux, a multicopy retrogene defining the cleavage-specific transcriptional program in placental mammals. In response to RS, DUX triggers the transcription of 2C-like markers such as murine endogenous retrovirus-like elements (MERVL) and Zscan4. This response can also be elicited by ETAA1-mediated ATR activation in the absence of RS. ATR-mediated activation of DUX requires GRSF1-dependent post-transcriptional regulation of Dux mRNA. Strikingly, activation of ATR expands ESCs fate potential by extending their contribution to both embryonic and extra-embryonic tissues. These findings define a novel ATR dependent pathway involved in maintaining genome stability in developing embryos by controlling ESCs fate in response to RS. Sí

Published
2020

9. ATR expands embryonic stem cell fate potential in response to replication stress.

Author

Atashpaz S, Samadi Shams S, Gonzalez JM, Sebestyén E, Arghavanifard N, Gnocchi A, Albers E, Minardi S, Faga G, Soffientini P, Allievi E, Cancila V, Bachi A, Fernández-Capetillo Ó, Tripodo C, Ferrari F, López-Contreras AJ, and Costanzo V

Subjects
Animals, Ataxia Telangiectasia Mutated Proteins genetics, Ataxia Telangiectasia Mutated Proteins metabolism, Cell Differentiation, Cell Proliferation physiology, Cells, Cultured, Checkpoint Kinase 1 genetics, Chimera, Chromatography, Liquid, Cloning, Molecular, DNA Damage, Embryonic Stem Cells, Gene Expression Regulation, Mice, RNA, Messenger genetics, RNA, Messenger metabolism, Sequence Analysis, RNA, Tandem Mass Spectrometry, Checkpoint Kinase 1 metabolism
Abstract

Unrepaired DNA damage during embryonic development can be potentially inherited by a large population of cells. However, the quality control mechanisms that minimize the contribution of damaged cells to developing embryos remain poorly understood. Here, we uncovered an ATR- and CHK1-mediated transcriptional response to replication stress (RS) in mouse embryonic stem cells (ESCs) that induces genes expressed in totipotent two-cell (2C) stage embryos and 2C-like cells. This response is mediated by Dux , a multicopy retrogene defining the cleavage-specific transcriptional program in placental mammals. In response to RS, DUX triggers the transcription of 2C-like markers such as murine endogenous retrovirus-like elements (MERVL) and Zscan4 . This response can also be elicited by ETAA1-mediated ATR activation in the absence of RS. ATR-mediated activation of DUX requires GRSF1-dependent post-transcriptional regulation of Dux mRNA. Strikingly, activation of ATR expands ESCs fate potential by extending their contribution to both embryonic and extra-embryonic tissues. These findings define a novel ATR dependent pathway involved in maintaining genome stability in developing embryos by controlling ESCs fate in response to RS., Competing Interests: SA, SS, JG, ES, NA, AG, EA, SM, GF, PS, EA, VC, AB, ÓF, CT, FF, AL, VC No competing interests declared, (© 2020, Atashpaz et al.)

Published
2020
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10. KMT2B Is Selectively Required for Neuronal Transdifferentiation, and Its Loss Exposes Dystonia Candidate Genes.

Author

Barbagiovanni G, Germain PL, Zech M, Atashpaz S, Lo Riso P, D'Antonio-Chronowska A, Tenderini E, Caiazzo M, Boesch S, Jech R, Haslinger B, Broccoli V, Stewart AF, Winkelmann J, and Testa G

Subjects
Animals, Cell Differentiation genetics, Embryo, Mammalian cytology, Epigenesis, Genetic, Fibroblasts cytology, Histones metabolism, Humans, Lysine metabolism, Methylation, Mice, Knockout, Neurons metabolism, Transcriptome genetics, Cell Transdifferentiation genetics, Dystonia genetics, Genetic Association Studies, Histone-Lysine N-Methyltransferase metabolism, Myeloid-Lymphoid Leukemia Protein metabolism, Neurons pathology
Abstract

Transdifferentiation of fibroblasts into induced neuronal cells (iNs) by the neuron-specific transcription factors Brn2, Myt1l, and Ascl1 is a paradigmatic example of inter-lineage conversion across epigenetically distant cells. Despite tremendous progress regarding the transcriptional hierarchy underlying transdifferentiation, the enablers of the concomitant epigenome resetting remain to be elucidated. Here, we investigated the role of KMT2A and KMT2B, two histone H3 lysine 4 methylases with cardinal roles in development, through individual and combined inactivation. We found that Kmt2b, whose human homolog's mutations cause dystonia, is selectively required for iN conversion through suppression of the alternative myocyte program and induction of neuronal maturation genes. The identification of KMT2B-vulnerable targets allowed us, in turn, to expose, in a cohort of 225 patients, 45 unique variants in 39 KMT2B targets, which represent promising candidates to dissect the molecular bases of dystonia., (Copyright © 2018 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2018
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11. Polycomb dysregulation in gliomagenesis targets a Zfp423-dependent differentiation network.

Author

Signaroldi E, Laise P, Cristofanon S, Brancaccio A, Reisoli E, Atashpaz S, Terreni MR, Doglioni C, Pruneri G, Malatesta P, and Testa G

Subjects
Animals, Base Sequence, Cells, Cultured, Down-Regulation, Epigenesis, Genetic, Female, Gene Silencing, Histones, Humans, Mice, Mice, Inbred Strains, Polycomb-Group Proteins genetics, Promoter Regions, Genetic, Protein Binding, Transcription Factors, Gene Expression Regulation, Neoplastic physiology, Glioma metabolism, Polycomb-Group Proteins metabolism
Abstract

Malignant gliomas constitute one of the most significant areas of unmet medical need, owing to the invariable failure of surgical eradication and their marked molecular heterogeneity. Accumulating evidence has revealed a critical contribution by the Polycomb axis of epigenetic repression. However, a coherent understanding of the regulatory networks affected by Polycomb during gliomagenesis is still lacking. Here we integrate transcriptomic and epigenomic analyses to define Polycomb-dependent networks that promote gliomagenesis, validating them both in two independent mouse models and in a large cohort of human samples. We find that Polycomb dysregulation in gliomagenesis affects transcriptional networks associated with invasiveness and de-differentiation. The dissection of these networks uncovers Zfp423 as a critical Polycomb-dependent transcription factor whose silencing negatively impacts survival. The anti-gliomagenic activity of Zfp423 requires interaction with the SMAD proteins within the BMP signalling pathway, pointing to a novel synergic circuit through which Polycomb inhibits BMP signalling.

Published
2016
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12. 7q11.23 dosage-dependent dysregulation in human pluripotent stem cells affects transcriptional programs in disease-relevant lineages.

Author

Adamo A, Atashpaz S, Germain PL, Zanella M, D'Agostino G, Albertin V, Chenoweth J, Micale L, Fusco C, Unger C, Augello B, Palumbo O, Hamilton B, Carella M, Donti E, Pruneri G, Selicorni A, Biamino E, Prontera P, McKay R, Merla G, and Testa G

Subjects
Cell Differentiation, Cell Lineage, Cohort Studies, Comparative Genomic Hybridization, Gene Dosage, Gene Duplication, Gene Expression Profiling, Histone Demethylases genetics, Humans, Oligonucleotide Array Sequence Analysis, Phenotype, Pluripotent Stem Cells pathology, Sequence Analysis, RNA, Chromosomes, Human, Pair 7 genetics, DNA Copy Number Variations, Gene Expression Regulation genetics, Pluripotent Stem Cells physiology, Transcription Factors, TFII genetics, Williams Syndrome genetics
Abstract

Cell reprogramming promises to make characterization of the impact of human genetic variation on health and disease experimentally tractable by enabling the bridging of genotypes to phenotypes in developmentally relevant human cell lineages. Here we apply this paradigm to two disorders caused by symmetrical copy number variations of 7q11.23, which display a striking combination of shared and symmetrically opposite phenotypes--Williams-Beuren syndrome and 7q-microduplication syndrome. Through analysis of transgene-free patient-derived induced pluripotent stem cells and their differentiated derivatives, we find that 7q11.23 dosage imbalance disrupts transcriptional circuits in disease-relevant pathways beginning in the pluripotent state. These alterations are then selectively amplified upon differentiation of the pluripotent cells into disease-relevant lineages. A considerable proportion of this transcriptional dysregulation is specifically caused by dosage imbalances in GTF2I, which encodes a key transcription factor at 7q11.23 that is associated with the LSD1 repressive chromatin complex and silences its dosage-sensitive targets.

Published
2015
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13. Highly effective DNA extraction method from fresh, frozen, dried and clotted blood samples.

Author

Samadi Shams S, Zununi Vahed S, Soltanzad F, Kafil V, Barzegari A, Atashpaz S, and Barar J

Abstract

Introduction: Today, with the tremendous potential of genomics and other recent advances in science, the role of science to improve reliable DNA extraction methods is more relevant than ever before. The ideal process for genomic DNA extraction demands high quantities of pure, integral and intact genomic DNA (gDNA) from the sample with minimal co-extraction of inhibitors of downstream processes. Here, we report the development of a very rapid, less-hazardous, and high throughput protocol for extracting of high quality DNA from blood samples., Methods: Dried, clotted and ethylene diamine tetra-acetic acid (EDTA) treated fresh and frozen blood samples were extracted using this method in which the quality and integrity of the extracted DNA were corroborated by agarose gel electrophoresis, PCR reaction and DNA digestion using restricted enzyme. The UV spectrophotometric and gel electrophoresis analysis resulted in high A260/A280 ratio (>1.8) with high intactness of DNA., Results: PCR and DNA digestion experiments indicated that the final solutions of extracted DNA contained no inhibitory substances, which confirms that the isolated DNA is of good quality., Conclusion: The high quality and quantity of current method, no enzymatic processing and accordingly its low cost, make it appropriate for DNA extraction not only from human but also from animal blood samples in any molecular biology labs.

Published
2011
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14. Microsurgeon Hirudo medicinalis as a Natural Bioshuttle for Spontaneous Mass Vaccination against Influenza A Virus.

Author

Samadi-Shams S, Atashpaz S, and Khani S

Abstract

Introduction: Recent report on existence of a stem region of hemagglutinin has arisen new hopes for vaccination of influenza A as it consist of a conserve fusion peptide shared across several influenza subtypes and can be targeted by human immune system., Methods: Given that traditional vaccination based on live attenuated viruses often fails to surpass such viral infection, a great deal of attention has been devoted to develop a safe yet efficient system for vaccination influenza A. We believe that a natural bioshuttle can be recruited for spontaneous mass vaccination., Results: Thus, here, we hypothesize that a bioengineered transgenic Hirudo medicinalis can be considered as an alive bioshuttle for in-situ vaccination against influenza A virus. By introducing the designated gene(s) encoding the target fragment (i.e., stem region of hemagglutinin), this microsurgeon can act as a rapid microproducer of viral proteins for in-house mass vaccination through imparting the necessary proteins such as those, naturally presented in leech's saliva., Conclusion: This peculiar bioshuttle can be easily exploited as a medical modality choice at home resulting in greater patient compliance.

Published
2011
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15. A robust universal method for extraction of genomic DNA from bacterial species.

Author

Atashpaz S, Khani S, Barzegari A, Barar J, Vahed SZ, Azarbaijani R, and Omidi Y

Subjects
Bacteria genetics, Bacteria chemistry, DNA, Bacterial isolation & purification, Genome, Bacterial
Abstract

The intactness of DNA is the keystone of genome-based clinical investigations, where rapid molecular detection of life-threatening bacteria is largely dependent on the isolation of high-quality DNA. Various protocols have been so far developed for genomic DNA isolation from bacteria, most of which have been claimed to be reproducible with relatively good yields of high-quality DNA. Nonetheless, they are not fully applicable to various types of bacteria, their processing cost is relatively high, and some toxic reagents are used. The routine protocols for DNA extraction appear to be sensitive to species diversity, and may fail to produce high-quality DNA from different species. Such protocols remain time-consuming and tedious, thus to resolve some of these impediments, we report development of a very simple, rapid, and high-throughput protocol for extracting of high-quality DNA from different bacterial species. Based upon our protocol, interfering phenolic compounds were removed from extraction using polyvinylpyrrolidone (PVP) and RNA contamination was precipitated using LiCI. The UV spectrophotometric and gel electrophoresis analysis resulted in high A260/A280 ratio (>1.8) with high intactness of DNA. Subsequent evaluations were performed using some quality-dependent techniques (e.g., RAPD marker and restriction digestions). The isolated DNA from 9 different bacterial species confirmed the accuracy of this protocol which requires no enzymatic processing and accordingly its low-cost making it an appropriate method f r large-scale DNA isolation fromvarious bacterial species.

Published
2010

16. Rapid and simple methodology for isolation of high quality genomic DNA from coniferous tissues (Taxus baccata).

Author

Barzegari A, Vahed SZ, Atashpaz S, Khani S, and Omidi Y

Subjects
DNA, Plant genetics, Genome, Plant, Nucleic Acid Amplification Techniques, Quality Control, Taxus chemistry, Time Factors, Tracheophyta chemistry, Tracheophyta genetics, Cell Fractionation methods, Cloning, Molecular methods, DNA, Plant isolation & purification, Taxus genetics
Abstract

Various investigations have been so far performed for extraction of genomic DNA from plant tissues, in which the extracted intact DNA can be exploited for a diverse range of biological studies. Extraction of high quality DNA from leathery plant tissues (e.g., coniferous organs) appears to be a critical stage. Moreover, for some species such as Taxus trees, bioprocess engineering and biosynthesis of secondary metabolites (e.g., paclitaxel) is a crucial step due to the restrictions associated with extinction of these species. However, extraction of intact genomic DNA from these plants still demands a rapid, easy and efficient protocol. To pursue such aim, in the current work, we report on the development of a simple and highly efficient method for the extraction of DNA from Taxus baccata. Based upon our protocol, interfering phenolic compounds were removed from extraction using polyvinylpyrrolidone and RNA contamination was resolved using LiCl. By employing this method, high quality genomic DNA was successfully extracted from leaves of T. baccata. The quality of extracted DNA was validated by various techniques such as RAPD marker, restriction digestions and pre-AFLP. Upon our findings, we propose this simple method to be considered for extraction of DNA from leathery plant tissues.

Published
2010
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17. Rapid virulence typing of Pasteurella multocida by multiplex PCR.

Author

Atashpaz S, Shayegh J, and Hejazi MS

Subjects
Genes, Bacterial, Pasteurella multocida genetics, Virulence, Pasteurella multocida classification, Pasteurella multocida pathogenicity, Polymerase Chain Reaction methods
Abstract

The gram-negative bacterium Pasteurella multocida constitutes a heterogeneous species associated with wide range of disease in many animals. Isolates are classified into five groups based on capsular antigen (capA, B, D, E and F). Recently, a new valuable PCR-based method was introduced to determine the epidemiological correlation between P. multocida infection and existence of virulence genes including tbpA, pfhA, toxA and hgbB. However, this method is tedious and laborious. Thus, in the current study, we designed a reliable multiplex PCR method for rapid detection of virulence genes in P. multocida. Eighty seven strains of P. multocida isolated from various clinically healthy and infected hosts were examined by uniplex PCR method for each virulence associated genes. Based on our improved and simplified multiplex PCR method, rapid detection of four virulence genes was accomplished. It is proposed that its implementation may benefit the epidemiological investigations.

Published
2009
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