Academic literature on the topic 'Transcriptions, Tamil'
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Journal articles on the topic "Transcriptions, Tamil"
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Ito, Jun, Hidehiro Fukaki, Makoto Onoda, et al. "Auxin-dependent compositional change in Mediator in ARF7- and ARF19-mediated transcription." Proceedings of the National Academy of Sciences 113, no. 23 (2016): 6562–67. http://dx.doi.org/10.1073/pnas.1600739113.
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Mediator is a multiprotein complex that integrates the signals from transcription factors binding to the promoter and transmits them to achieve gene transcription. The subunits of Mediator complex reside in four modules: the head, middle, tail, and dissociable CDK8 kinase module (CKM). The head, middle, and tail modules form the core Mediator complex, and the association of CKM can modify the function of Mediator in transcription. Here, we show genetic and biochemical evidence that CKM-associated Mediator transmits auxin-dependent transcriptional repression in lateral root (LR) formation. The AUXIN/INDOLE 3-ACETIC ACID 14 (Aux/IAA14) transcriptional repressor inhibits the transcriptional activity of its binding partners AUXIN RESPONSE FACTOR 7 (ARF7) and ARF19 by making a complex with the CKM-associated Mediator. In addition, TOPLESS (TPL), a transcriptional corepressor, forms a bridge between IAA14 and the CKM component MED13 through the physical interaction. ChIP assays show that auxin induces the dissociation of MED13 but not the tail module component MED25 from the ARF7 binding region upstream of its target gene. These findings indicate that auxin-induced degradation of IAA14 changes the module composition of Mediator interacting with ARF7 and ARF19 in the upstream region of their target genes involved in LR formation. We suggest that this regulation leads to a quick switch of signal transmission from ARFs to target gene expression in response to auxin.
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Georges, Sara A., W. Lee Kraus, Karolin Luger, Jennifer K. Nyborg, and Paul J. Laybourn. "p300-Mediated Tax Transactivation from Recombinant Chromatin: Histone Tail Deletion Mimics Coactivator Function." Molecular and Cellular Biology 22, no. 1 (2002): 127–37. http://dx.doi.org/10.1128/mcb.22.1.127-137.2002.
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ABSTRACT Efficient transcription of the human T-cell leukemia virus type 1 (HTLV-1) genome requires Tax, a virally encoded oncogenic transcription factor, in complex with the cellular transcription factor CREB and the coactivators p300/CBP. To examine Tax transactivation in vitro, we used a chromatin assembly system that included recombinant core histones. The addition of Tax, CREB, and p300 to the HTLV-1 promoter assembled into chromatin activated transcription several hundredfold. Chromatin templates selectively lacking amino-terminal histone tails demonstrated enhanced transcriptional activation by Tax and CREB, with significantly reduced dependence on p300 and acetyl coenzyme A (acetyl-CoA). Interestingly, Tax/CREB activation from the tailless chromatin templates retained a substantial requirement for acetyl-CoA, indicating a role for acetyl-CoA beyond histone acetylation. These data indicate that during Tax transcriptional activation, the amino-terminal histone tails are the major targets of p300 and that tail deletion and acetylation are functionally equivalent.
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Liu, Zhongle, and Lawrence C. Myers. "Fungal Mediator Tail Subunits Contain Classical Transcriptional Activation Domains." Molecular and Cellular Biology 35, no. 8 (2015): 1363–75. http://dx.doi.org/10.1128/mcb.01508-14.
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Classical activation domains within DNA-bound eukaryotic transcription factors make weak interactions with coactivator complexes, such as Mediator, to stimulate transcription. How these interactions stimulate transcription, however, is unknown. The activation of reporter genes by artificial fusion of Mediator subunits to DNA binding domains that bind to their promoters has been cited as evidence that the primary role of activators is simply to recruit Mediator. We have identified potent classical transcriptional activation domains in the C termini of several tail module subunits ofSaccharomyces cerevisiae,Candida albicans, andCandida dubliniensisMediator, while their N-terminal domains are necessary and sufficient for their incorporation into Mediator but do not possess the ability to activate transcription when fused to a DNA binding domain. This suggests that Mediator fusion proteins actually are functioning in a manner similar to that of a classical DNA-bound activator rather than just recruiting Mediator. Our finding that deletion of the activation domains ofS. cerevisiaeMed2 and Med3, as well asC. dubliniensisTlo1 (a Med2 ortholog), impairs the induction of certain genes shows these domains function at native promoters. Activation domains within coactivators are likely an important feature of these complexes and one that may have been uniquely leveraged by a common fungal pathogen.
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McCulloch, Vicki, and Gerald S. Shadel. "Human Mitochondrial Transcription Factor B1 Interacts with the C-Terminal Activation Region of h-mtTFA and Stimulates Transcription Independently of Its RNA Methyltransferase Activity." Molecular and Cellular Biology 23, no. 16 (2003): 5816–24. http://dx.doi.org/10.1128/mcb.23.16.5816-5824.2003.
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ABSTRACT A significant advancement in understanding mitochondrial gene expression is the recent identification of two new human mitochondrial transcription factors, h-mtTFB1 and h-mtTFB2. Both proteins stimulate transcription in collaboration with the high-mobility group box transcription factor, h-mtTFA, and are homologous to rRNA methyltransferases. In fact, the dual-function nature of h-mtTFB1 was recently demonstrated by its ability to methylate a conserved rRNA substrate. Here, we demonstrate that h-mtTFB1 binds h-mtTFA both in HeLa cell mitochondrial extracts and in direct-binding assays via an interaction that requires the C-terminal tail of h-mtTFA, a region necessary for transcriptional activation. In addition, point mutations in conserved methyltransferase motifs of h-mtTFB1 revealed that it stimulates transcription in vitro independently of S-adenosylmethionine binding and rRNA methyltransferase activity. Furthermore, one mutation (G65A) eliminated the ability of h-mtTFB1 to bind DNA yet did not affect transcriptional activation. These results, coupled with the observation that h-mtTFB1 and human mitochondrial RNA (h-mtRNA) polymerase can also be coimmunoprecipitated, lead us to propose a model in which h-mtTFA demarcates mitochondrial promoter locations and where h-mtTFB proteins bridge an interaction between the C-terminal tail of h-mtTFA and mtRNA polymerase to facilitate specific initiation of transcription. Altogether, these data provide important new insight into the mechanism of transcription initiation in human mitochondria and indicate that the dual functions of h-mtTFB1 can be separated.
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Alff, Peter J., Nandini Sen, Elena Gorbunova, Irina N. Gavrilovskaya, and Erich R. Mackow. "The NY-1 Hantavirus Gn Cytoplasmic Tail Coprecipitates TRAF3 and Inhibits Cellular Interferon Responses by Disrupting TBK1-TRAF3 Complex Formation." Journal of Virology 82, no. 18 (2008): 9115–22. http://dx.doi.org/10.1128/jvi.00290-08.
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ABSTRACT Pathogenic hantaviruses replicate within human endothelial cells and cause two diseases, hemorrhagic fever with renal syndrome and hantavirus pulmonary syndrome. In order to replicate in endothelial cells pathogenic hantaviruses inhibit the early induction of beta interferon (IFN-β). Expression of the cytoplasmic tail of the pathogenic NY-1 hantavirus Gn protein is sufficient to inhibit RIG-I- and TBK1-directed IFN responses. The formation of TBK1-TRAF3 complexes directs IRF-3 phosphorylation, and both IRF-3 and NF-κB activation are required for transcription from the IFN-β promoter. Here we report that the NY-1 virus (NY-1V) Gn tail inhibits both TBK1-directed NF-κB activation and TBK1-directed transcription from promoters containing IFN-stimulated response elements. The NY-1V Gn tail coprecipitated TRAF3 from cellular lysates, and analysis of TRAF3 deletion mutants demonstrated that the TRAF3 N terminus is sufficient for interacting with the NY-1V Gn tail. In contrast, the Gn tail of the nonpathogenic hantavirus Prospect Hill virus (PHV) failed to coprecipitate TRAF3 or inhibit NF-κB or IFN-β transcriptional responses. Further, expression of the NY-1V Gn tail blocked TBK1 coprecipitation of TRAF3 and infection by NY-1V, but not PHV, blocked the formation of TBK1-TRAF3 complexes. These findings indicate that the NY-1V Gn cytoplasmic tail forms a complex with TRAF3 which disrupts the formation of TBK1-TRAF3 complexes and downstream signaling responses required for IFN-β transcription.
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Talbert, Paul B., and Steven Henikoff. "The Yin and Yang of Histone Marks in Transcription." Annual Review of Genomics and Human Genetics 22, no. 1 (2021): 147–70. http://dx.doi.org/10.1146/annurev-genom-120220-085159.
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Nucleosomes wrap DNA and impede access for the machinery of transcription. The core histones that constitute nucleosomes are subject to a diversity of posttranslational modifications, or marks, that impact the transcription of genes. Their functions have sometimes been difficult to infer because the enzymes that write and read them are complex, multifunctional proteins. Here, we examine the evidence for the functions of marks and argue that the major marks perform a fairly small number of roles in either promoting transcription or preventing it. Acetylations and phosphorylations on the histone core disrupt histone–DNA contacts and/or destabilize nucleosomes to promote transcription. Ubiquitylations stimulate methylations that provide a scaffold for either the formation of silencing complexes or resistance to those complexes, and carry a memory of the transcriptional state. Tail phosphorylations deconstruct silencing complexes in particular contexts. We speculate that these fairly simple roles form the basis of transcriptional regulation by histone marks.
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Sims, Jennifer K., and Judd C. Rice. "PR-Set7 Establishes a Repressive trans-Tail Histone Code That Regulates Differentiation." Molecular and Cellular Biology 28, no. 14 (2008): 4459–68. http://dx.doi.org/10.1128/mcb.00410-08.
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ABSTRACT Posttranslational modifications of the DNA-associated histone proteins play fundamental roles in eukaryotic transcriptional regulation. We previously discovered a novel trans-tail histone code involving monomethylated histone H4 lysine 20 (H4K20) and H3 lysine 9 (H3K9); however, the mechanisms that establish this code and its function in transcription were unknown. In this report, we demonstrate that H3K9 monomethylation is dependent upon the PR-Set7 H4K20 monomethyltransferase but independent of its catalytic function, indicating that PR-Set7 recruits an H3K9 monomethyltransferase to establish the trans-tail histone code. We determined that this histone code is involved in a transcriptional regulatory pathway in vivo whereby monomethylated H4K20 binds the L3MBTL1 repressor protein to repress specific genes, including RUNX1, a critical regulator of hematopoietic differentiation. The selective loss of monomethylated H4K20 at the RUNX1 promoter resulted in the displacement of L3MBTL1 and a concomitant increase in RUNX1 transcription. Importantly, the lack of monomethylated H4K20 in the human K562 multipotent cell line was specifically associated with spontaneous megakaryocytic differentiation, in part, by activating RUNX1. Our findings demonstrate that this newly described repression pathway is required for regulating proper megakaryopoiesis and suggests that it is likely to function similarly in other multipotent cell types to regulate specific differentiation pathways.
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WANG, Guannan, Jianyin LONG, Isao MATSUURA, Dongming HE, and Fang LIU. "The Smad3 linker region contains a transcriptional activation domain." Biochemical Journal 386, no. 1 (2005): 29–34. http://dx.doi.org/10.1042/bj20041820.
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Transforming growth factor-β (TGF-β)/Smads regulate a wide variety of biological responses through transcriptional regulation of target genes. Smad3 plays a key role in TGF-β/Smad-mediated transcriptional responses. Here, we show that the proline-rich linker region of Smad3 contains a transcriptional activation domain. When the linker region is fused to a heterologous DNA-binding domain, it activates transcription. We show that the linker region physically interacts with p300. The adenovirus E1a protein, which binds to p300, inhibits the transcriptional activity of the linker region, and overexpression of p300 can rescue the linker-mediated transcriptional activation. In contrast, an adenovirus E1a mutant, which cannot bind to p300, does not inhibit the linker-mediated transcription. The native Smad3 protein lacking the linker region is unable to mediate TGF-β transcriptional activation responses, although it can be phosphorylated by the TGF-β receptor at the C-terminal tail and has a significantly increased ability to form a heteromeric complex with Smad4. We show further that the linker region and the C-terminal domain of Smad3 synergize for transcriptional activation in the presence of TGF-β. Thus our findings uncover an important function of the Smad3 linker region in Smad-mediated transcriptional control.
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Ryu, Hong-Yeoul, Dejian Zhao, Jianhui Li, Dan Su, and Mark Hochstrasser. "Histone sumoylation promotes Set3 histone-deacetylase complex-mediated transcriptional regulation." Nucleic Acids Research 48, no. 21 (2020): 12151–68. http://dx.doi.org/10.1093/nar/gkaa1093.
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Abstract Histones are substrates of the SUMO (small ubiquitin-like modifier) conjugation pathway. Several reports suggest histone sumoylation affects transcription negatively, but paradoxically, our genome-wide analysis shows the modification concentrated at many active genes. We find that trans-tail regulation of histone-H2B ubiquitylation and H3K4 di-methylation potentiates subsequent histone sumoylation. Consistent with the known control of the Set3 histone deacetylase complex (HDAC) by H3K4 di-methylation, histone sumoylation directly recruits the Set3 complex to both protein-coding and noncoding RNA (ncRNA) genes via a SUMO-interacting motif in the HDAC Cpr1 subunit. The altered gene expression profile caused by reducing histone sumoylation matches well to the profile in cells lacking Set3. Histone H2B sumoylation and the Set3 HDAC coordinately suppress cryptic ncRNA transcription initiation internal to mRNA genes. Our results reveal an elaborate co-transcriptional histone crosstalk pathway involving the consecutive ubiquitylation, methylation, sumoylation and deacetylation of histones, which maintains transcriptional fidelity by suppressing spurious transcription.
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Merrick, David, Kavita Mistry, Jingshing Wu, et al. "Polycystin-1 regulates bone development through an interaction with the transcriptional coactivator TAZ." Human Molecular Genetics 28, no. 1 (2018): 16–30. http://dx.doi.org/10.1093/hmg/ddy322.
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Abstract Polycystin-1 (PC1), encoded by the PKD1 gene that is mutated in the autosomal dominant polycystic kidney disease, regulates a number of processes including bone development. Activity of the transcription factor RunX2, which controls osteoblast differentiation, is reduced in Pkd1 mutant mice but the mechanism governing PC1 activation of RunX2 is unclear. PC1 undergoes regulated cleavage that releases its C-terminal tail (CTT), which translocates to the nucleus to modulate transcriptional pathways involved in proliferation and apoptosis. We find that the cleaved CTT of PC1 (PC1-CTT) stimulates the transcriptional coactivator TAZ (Wwtr1), an essential coactivator of RunX2. PC1-CTT physically interacts with TAZ, stimulating RunX2 transcriptional activity in pre-osteoblast cells in a TAZ-dependent manner. The PC1-CTT increases the interaction between TAZ and RunX2 and enhances the recruitment of the p300 transcriptional co-regulatory protein to the TAZ/RunX2/PC1-CTT complex. Zebrafish injected with morpholinos directed against pkd1 manifest severe bone calcification defects and a curly tail phenotype. Injection of messenger RNA (mRNA) encoding the PC1-CTT into pkd1-morphant fish restores bone mineralization and reduces the severity of the curly tail phenotype. These effects are abolished by co-injection of morpholinos directed against TAZ. Injection of mRNA encoding a dominant-active TAZ construct is sufficient to rescue both the curly tail phenotype and the skeletal defects observed in pkd1-morpholino treated fish. Thus, TAZ constitutes a key mechanistic link through which PC1 mediates its physiological functions.
Dissertations / Theses on the topic "Transcriptions, Tamil"
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Enikanolaiye, Adebola. "The Role of the Claudin 6 Cytoplasmic Tail In Epidermal Differentiation and the Role of Cdx In Endodermal Development." Thesis, Université d'Ottawa / University of Ottawa, 2015. http://hdl.handle.net/10393/32354.
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The mammalian skin provides a necessary barrier between the organism and the environment, defending against loss of water and solutes, preventing the invasion of pathogens as well as protecting against chemical and physical assault. Claudin (Cldn)-based Tight Junctions (TJs) are the main functional part of the skin barrier. In particular, Cldn6 through its cytoplasmic tail has been shown to be important for barrier function. In other to further investigate the role of the Cldn6 tail in TJ-function, we developed Cldn6 mouse mutants carrying varying truncations of the Cldn6 tail. Both of these mice present with epidermal differentiation perturbations and delayed barrier function that is repaired later in life. These studies support the importance of the tail portion of the Cldn molecules in epidermal differentiation and barrier function. In addition, both of these mouse models are useful for the study of barrier function in preterm infants and in aging, with the hope of developing novel therapeutics for the alleviation of barrier dysfunction.
Cdx is a family of homeodomain (HD) transcription factors (TFs) essential for many key developmental processes. In particular, Cdx2 is important for the establishment and maintenance of posterior identity in the developing endoderm. In spite of this, only a few Cdx targets in the developing endoderm have been discovered. In addition, the interplay between Cdx and its targets within the endoderm is poorly understood. In this study, we show that the forkhead box transcription factor, Foxa2 is a Cdx2 target. We also show that Foxa2 and Cdx2 physically and genetically interact to regulate a subset of genes that are implicated in endodermal development. These studies help to further our understanding of endoderm biology with the goal of developing new strategies to diagnose and treat diseases associated with defective endoderm development.
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Su, Yu-Lun, and 蘇昱倫. "Part I: Tristetraprolin (TTP) inhibits poly(A)-tail synthesis in nuclearmRNA that contains AU-rich elements by interacting with poly(A)-bindingprotein nuclear 1 (PABPN1)Part II: Transcriptional regulation of mitogen-activated protein kinasephosphatase-1 (Mkp-1) expression in LPS-stimulated mouse macrophageRAW264.7 cells." Thesis, 2012. http://ndltd.ncl.edu.tw/handle/12755275548414566611.
Full textAbstract:
博士<br>國立臺灣大學<br>生化科學研究所<br>100<br>Part I
Tristetraprolin (TTP) binds mRNA AU-rich elements (ARE) and thereby facilitates the destabilization of mature mRNA. To understand how TTP mechanistically functions, previously our lab biopanned with a phage-display library for proteins that interact with TTP and retrieved, among others, poly(A) binding protein nuclear 1 (PABPN1). PABPN1 assists in the 3’-polyadenylation of mRNA by binding to an immature poly(A) tail and increasing the affinity of poly(A) polymerase, which is directly responsible for polyadenylation. The poly(A) tail is important for mRNA export from the nucleus, mRNA stabilization, and translation efficiency. The TTP/PABPN1 interaction was characterized using co-immunoprecipitation assays. Although TTP and PABPN1 are located in both the cytoplasm and the nucleus, they interacted in vivo only in the nucleus. Expression of a TTP mutant restricted to the nucleus resulted in the downregulation of a TNFα ARE-containing luciferase activity .Interestingly, we found that TTP binds PABPN1 and thereby inhibits polyadenylation of ARE-containing mRNA in vitro. When TNFα mRNA was induced in mouse RAW264.7 cells by lipopolysaccharide treatment, synthesis of a shorter poly(A) tail in nuclear TNFα mRNA and an increased expression of TTP occurred. Consequently, in addition to its known cytosolic mRNA-degrading function, TTP inhibits poly(A) tail synthesis by interacting with PABPN1 in the nucleus to regulate expression of ARE-containing mRNA.
Part II
Innate immune responses rely on the MAPK signaling pathway, especially p38 and Jnk. These kinases are activated by pro-inflammatory agonists, and lead to inflammatory or innate immune responses by regulating the expression of several effector genes. Both p38 and Jnk are negatively regulated through their dephosphorylation by MAPK phosphatase 1 (Mkp-1), a member of dual specificity protein phosphatase (DUSP). Recent reports supported that Mkp-1 is a critical regulator of innate immunity. Previously, we have demonstrated that the mRNA of Mkp-1 was rapidly elevated around 30 to 60 minutes and soon decreased less than half after LPS stimulation for 2 h in RAW264.7 cells. Here we concerned with the molecular mechanism in control of the growth and decline of Mkp-1 mRNA at transcriptional level. Creb1 and Atf3, members of the Atf/Creb family protein, were shown to associate with the Mkp-1 promoter and increase the activity of luciferase reporter that carrying the Mkp-1 promoter. Knockdown of Atf3 in RAW264.7 cells resulted in Mkp-1 mRNA downregulation. Therefore, Creb1 and Atf3 regulate Mkp-1 expression positively. The PI3K signaling pathway, which was activated after LPS stimulation for 2 h, was suggested to play an opposite role to restrict the TLR4 signaling. The Mkp-1 mRNA level was increased in the presence of the PI3K signaling inhibitor, Wortmannin. Using the microarray analysis and real time PCR, the Id3 was identified and confirmed for the candidates that downstream of PI3K signaling to regulate Mkp-1 expression. Further studies are needed to examine the function of Id3 and the molecular mechanism of regulating Mkp-1 expression in LPS-stimulated RAW264.7 cells.
Books on the topic "Transcriptions, Tamil"
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Taṅkēsvari, Ka. Kuḷakkōṭṭan̲ tarican̲am: Ōr āyvu nōkku. An̲pu Veḷiyīṭu, 1993.
Find full textBook chapters on the topic "Transcriptions, Tamil"
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Carley, Paul, and Inger M. Mees. "Nucleus and tail." In American English Phonetic Transcription. Routledge, 2021. http://dx.doi.org/10.4324/9781003008088-21.
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Carley, Paul, and Inger M. Mees. "Nucleus and tail." In British English Phonetic Transcription. Routledge, 2021. http://dx.doi.org/10.4324/9781003007890-21.
Full textConference papers on the topic "Transcriptions, Tamil"
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Behrens, Michelle, Paul Grandgenett, Jennifer Bailey, Pankaj Singh, Chun-Hui Yi, and Michael Hollingsworth. "Abstract 5077: Signaling through the cytoplasmic tail of MUC1 directly activates transcription of the metastasis promoting growth factor CTGF in pancreatic adenocarcinoma." In Proceedings: AACR 101st Annual Meeting 2010‐‐ Apr 17‐21, 2010; Washington, DC. American Association for Cancer Research, 2010. http://dx.doi.org/10.1158/1538-7445.am10-5077.
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