Literatura científica selecionada sobre o tema "Protein N-terminal modifications"
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Artigos de revistas sobre o assunto "Protein N-terminal modifications"
Lai, Zon W., Agnese Petrera e Oliver Schilling. "Protein amino-terminal modifications and proteomic approaches for N-terminal profiling". Current Opinion in Chemical Biology 24 (fevereiro de 2015): 71–79. http://dx.doi.org/10.1016/j.cbpa.2014.10.026.
Texto completo da fonteVoronina, A. I., Yu V. Miroshnichenko e V. S. Skvortsov. "Bioinformatic identification of proteins with altered PTM levels in a mouse line established to study the mechanisms of the development of fibromuscular dysplasia". Biomeditsinskaya Khimiya 70, n.º 4 (2024): 248–55. http://dx.doi.org/10.18097/pbmc20247004248.
Texto completo da fonteYu, Guann-Yi, Ki-Jeong Lee, Lu Gao e Michael M. C. Lai. "Palmitoylation and Polymerization of Hepatitis C Virus NS4B Protein". Journal of Virology 80, n.º 12 (15 de junho de 2006): 6013–23. http://dx.doi.org/10.1128/jvi.00053-06.
Texto completo da fonteDissmeyer, Nico. "Conditional Protein Function via N-Degron Pathway–Mediated Proteostasis in Stress Physiology". Annual Review of Plant Biology 70, n.º 1 (29 de abril de 2019): 83–117. http://dx.doi.org/10.1146/annurev-arplant-050718-095937.
Texto completo da fonteMeinnel, Thierry, e Carmela Giglione. "Tools for analyzing and predicting N-terminal protein modifications". PROTEOMICS 8, n.º 4 (fevereiro de 2008): 626–49. http://dx.doi.org/10.1002/pmic.200700592.
Texto completo da fonteRose, K., P. O. Regamey, R. Anderegg, T. N. C. Wells e A. E. I. Proudfoot. "Human interleukin-5 expressed in Escherichia coli has N-terminal modifications". Biochemical Journal 286, n.º 3 (15 de setembro de 1992): 825–28. http://dx.doi.org/10.1042/bj2860825.
Texto completo da fonteLee, Seon Hwa, e Tomoyuki Oe. "Oxidative stress-mediated N-terminal protein modifications and MS-based approaches for N-terminal proteomics". Drug Metabolism and Pharmacokinetics 31, n.º 1 (fevereiro de 2016): 27–34. http://dx.doi.org/10.1016/j.dmpk.2015.12.002.
Texto completo da fonteOuidir, Tassadit, Frédérique Jarnier, Pascal Cosette, Thierry Jouenne e Julie Hardouin. "Characterization of N-terminal protein modifications in Pseudomonas aeruginosa PA14". Journal of Proteomics 114 (janeiro de 2015): 214–25. http://dx.doi.org/10.1016/j.jprot.2014.11.006.
Texto completo da fonteGiglione, Carmela, Sonia Fieulaine e Thierry Meinnel. "N-terminal protein modifications: Bringing back into play the ribosome". Biochimie 114 (julho de 2015): 134–46. http://dx.doi.org/10.1016/j.biochi.2014.11.008.
Texto completo da fonteVan Damme, Petra. "Charting the N-Terminal Acetylome: A Comprehensive Map of Human NatA Substrates". International Journal of Molecular Sciences 22, n.º 19 (2 de outubro de 2021): 10692. http://dx.doi.org/10.3390/ijms221910692.
Texto completo da fonteTeses / dissertações sobre o assunto "Protein N-terminal modifications"
Xie, Dong. "Uncovering the maturation pathway of plant Rubisco". Electronic Thesis or Diss., université Paris-Saclay, 2024. http://www.theses.fr/2024UPASL080.
Texto completo da fonteDuring photosynthesis, atmospheric carbon dioxide (CO₂), the prevalent anthropogenic greenhouse gas, is assimilated into carbohydrates by the enzyme Rubisco, the most abundant protein on earth. The large subunit of Rubisco (RbcL) undergoes a unique maturation pathway leading to unusual N-terminal modifications. This mechanism is conserved in plants, resulting in an N-terminal acetylated proline at position 3. Unravelling the maturation pathway of Rubisco is therefore a key challenge for CO₂ fixation in the context of climate change and global warming. My PhD project aimed at discovering the machinery leading to Pro3 acetylation and unmasking the associated functional relevance. First, two open reading frames (ORFs) in Arabidopsis thaliana were identified as putative candidates that might contribute to the proteolytic part of this process. The functions of two conserved aminopeptidases were challenged in vitro assay and in knockout Arabidopsis thaliana lines. I showed that one protease is specifically in charge of residue 2 release, while the second does not contribute to N-terminal protein maturation in the plastid. In addition, my data demonstrates that Pro3 acetylation is catalysed by only one acetyltransferase isoform occurring in the plastid. Together, the unique N-terminal modification machinery involved in RbcL processing relies on two enzymes that are dedicated to RbcL processing. I could reconstitute the maturation pathway in E. coli. Finally, I have investigated how the N-terminal modifications of RbcL affect Rubisco assembly, activity, and accumulation
Connor, Rebecca E. Barton Jacqueline K. Tirrell David A. "N-terminal modification and codon reassignment with non-canonical amino acids in proteins /". Diss., Pasadena, Calif. : California Institute of Technology, 2008. http://resolver.caltech.edu/CaltechETD:etd-03052008-065324.
Texto completo da fonteLiu, Li. "Purification and characterization of a protein palmitoyltransferase that acts on H-Ras protein and on a C-terminal N-Ras peptide /". Thesis, Connect to this title online; UW restricted, 1996. http://hdl.handle.net/1773/8664.
Texto completo da fonteLavecchia, Francesco. "Integrative Approaches to Decode the Co-translational Role of the Phage Vp16 Peptide Deformylase and how it Compromises Host Viability". Thesis, Université Paris-Saclay (ComUE), 2019. http://www.theses.fr/2019SACLS004/document.
Texto completo da fonteN-terminal Methionine Excision (NME) is the first occurring N-terminal Protein Modification (NPMs). Peptide deformylases (PDFs) are the enzymes involved in this essential and conserved co-translational process. PDFs remove the formyl group bound to the iMet present at the beginning of all prokaryotic nascent chains. PDFs act on the nascent chain at the level of the ribosome exit tunnel, a central hub for a number of Ribosome-associated Protein Biogenesis factors (RPBs) involved not only on NPMs but also in protein folding and translocation. Deformylation involves 95% of bacterial proteome and it is suggested to directly contribute to protein stability. Recent high-throughput sequencing of thousands of genomes has strongly contributed to revolutionizing our perception of the distribution of PDFs among kingdoms, revealing putative PDFs in all organisms, including viruses. In particular, studies of viruses within oceanic microbial samples retrieved unusual PDFs genes as the most abundant family in most of phage genomes. Sequence comparisons reveal that viral PDFs show high conservation in the three motifs that build the catalytic site; however, viral PDFs do not display a C-terminal extension when compared to the different active PDFs from other organisms. Since this C-terminal extension was shown to be important for PDF-ribosome binding and is required for the in vivo deformylase activity of E. coli PDF, it was unclear whether the discovered phage PDFs might support a classical deformylase activity. Thus, the discovery of these viral PDFs raises a number of questions among which: a) Have these viral PDFs a classical deformylase activity? b) Are these PDFs able to still bind to the ribosomes? c) Why so many viruses carry a peptide deformylase? In this context, the objective of my thesis was to undertake the characterization of these marine phage PDFs and particularly Vp16 PDF derived from the bacteriophages originally isolated from Vibrio Parahaemolyticus strain 16. Our studies reveal that phage PDFs display deformylase activity both in vitro and in vivo with a substrate specificity similar to that of other bacterial PDFs. On the other hand, we showed by biochemical and structural data, combined with site-directed mutagenesis analyses, that Vp16 PDF significantly differs from previously characterized PDFs in terms of their properties, which can be related to its few uncommon peculiarities. Interestingly, expression of Vp16 PDF in E. coli strains, even at low concentrations, exhibited a severe bactericidal effect at temperature lower than 37 °C. This bactericidal effect of Vp16 PDF was independent of the presence of the bacterial endogenous PDF and strictly relied on its PDF activity. Characterization of this phenotype revealed that Vp16 PDF-induced lethality showed a strong genetic link with genes encoding cellular factors involved in nascent pre-secretory protein targeting and folding (Trigger Factor and Sec). Differently from bacterial PDF, I could show that Vp16 PDF has strong affinity for ribosomes with a specific nascent chain, interacting with a ribosomal region overlapping that of factors involved in pre-secretory protein targeting. A competition between Vp16 PDF and these RPBs at the level of the ribosome may contribute to the host lysis, revealing a possible new unrecognized mechanism developed by viruses to control host viability
Kshetri, Man B. "N-TERMINAL DOMAIN OF rRNA METHYLTRANSFERASE ENZYME RsmC IS IMPORTANT FOR ITS BINDING TO RNA AND RNA CHAPERON ACTIVITY". Kent State University Honors College / OhioLINK, 2021. http://rave.ohiolink.edu/etdc/view?acc_num=ksuhonors1621007414429417.
Texto completo da fonteEl, Barbry Houssam. "Découverte du rôle crucial du résidu en position 2 des séquences MTS d’adressage mitochondrial". Electronic Thesis or Diss., Sorbonne université, 2023. http://www.theses.fr/2023SORUS035.
Texto completo da fonteMitochondria are complex organelles involving a thousand proteins, most of which are encoded in the nuclear genome. Their biogenesis has required the evolutionary development of efficient protein addressing and import systems, and failures of these systems are associated with serious pathologies, neuropathies, cardiovascular disorders, myopathies, neurodegenerative diseases and cancers.Many mitochondrial proteins have an N-terminal addressing sequence called MTS (Mitochondrial Targeting Sequence) which forms an amphiphilic alpha helix essential for their mitochondrial import. However, the sequence of the various MTSs is highly variable and their critical characteristics are not yet well understood. The starting point of my thesis was the discovery in yeast of an overrepresentation of 4 hydrophobic amino acids (F, L, I, W) at position 2 of the MTSs sequences. During my thesis, I was able to confirm the critical role of the nature of the residue in position 2 of the MTSs through directed mutagenesis experiments. Indeed, thanks to the development of an innovative system for screening import defects based on the functional rescue of the toxicity of a mitochondrial protein, I was able to observe that only residues overrepresented at position 2 of mitochondrial proteins allowed efficient import. My work has thus demonstrated the existence of strong evolutionary constraints at position 2 of MTSs, the understanding of which could ultimately be useful for optimising the mitochondrial addressing of therapeutic proteins in patients suffering from mitochondrial diseases
Zákoucká, Eva. "Proteomická a bioinformatická charakterizace N-terminálních sekvencí proteinů modifikovaných po importu do hydrogenosomu Trichomonas vaginalis". Master's thesis, 2014. http://www.nusl.cz/ntk/nusl-337356.
Texto completo da fonteConnor, Rebecca Elizabeth. "N-Terminal Modification and Codon Reassignment with Non-Canonical Amino Acids in Proteins". Thesis, 2008. https://thesis.library.caltech.edu/878/8/ConnorTOC.pdf.
Texto completo da fonteLivros sobre o assunto "Protein N-terminal modifications"
Wetzel, Ronald, e Rakesh Mishra. Structural Biology. Oxford University Press, 2014. http://dx.doi.org/10.1093/med/9780199929146.003.0012.
Texto completo da fonteCapítulos de livros sobre o assunto "Protein N-terminal modifications"
Ciechanover, Aaron. "N-terminal Ubiquitination: No Longer Such a Rare Modification". In Protein Degradation, 10–20. Weinheim, FRG: Wiley-VCH Verlag GmbH & Co. KGaA, 2005. http://dx.doi.org/10.1002/352760586x.ch2.
Texto completo da fonteAcikalin Coskun, Kubra, Nazlıcan Yurekli, Elif Cansu Abay, Merve Tutar, Mervenur Al e Yusuf Tutar. "Structure- and Design-Based Difficulties in Recombinant Protein Purification in Bacterial Expression". In Protein Detection [Working Title]. IntechOpen, 2022. http://dx.doi.org/10.5772/intechopen.103958.
Texto completo da fonteArnesen, Thomas. "Preface – The impact of protein N- and C-terminal modifications". In Methods in Enzymology, xv—xviii. Elsevier, 2023. http://dx.doi.org/10.1016/s0076-6879(23)00248-3.
Texto completo da fonteBarlowe, Charles, Randy Schekman e Aki Nakano. "Sarlp". In Guidebook to the Sinall GTPases, 450–51. Oxford University PressOxford, 1995. http://dx.doi.org/10.1093/oso/9780198599456.003.0150.
Texto completo da fonteLahnstein, Jelle, Shanny L. Dyer, Neil H. Goss, Mark Duncan e Raymond S. Norton. "N-TERMINAL MODIFICATION OF MALARIAL ANTIGENS FROM E. coli". In Techniques in Protein Chemistry IV, 83–90. Elsevier, 1993. http://dx.doi.org/10.1016/b978-0-12-058757-5.50014-7.
Texto completo da fonteWu, Pengguang, e Ludwig Brand. "[15] N-terminal modification of proteins for fluorescence measurements". In Methods in Enzymology, 321–30. Elsevier, 1997. http://dx.doi.org/10.1016/s0076-6879(97)78017-0.
Texto completo da fonteRelatórios de organizações sobre o assunto "Protein N-terminal modifications"
Ehrlich, Marcelo, John S. Parker e Terence S. Dermody. Development of a Plasmid-Based Reverse Genetics System for the Bluetongue and Epizootic Hemorrhagic Disease Viruses to Allow a Comparative Characterization of the Function of the NS3 Viroporin in Viral Egress. United States Department of Agriculture, setembro de 2013. http://dx.doi.org/10.32747/2013.7699840.bard.
Texto completo da fonte