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2. A Multilaboratory Comparison of Calibration Accuracy and the Performance of External References in Analytical Ultracentrifugation

Author

Langowski, J, Zhao, H, Ghirlando, R, Alfonso, C, Arisaka, F, Attali, I, Bain, DL, Bakhtina, MM, Becker, DF, Bedwell, GJ, Bekdemir, A, Besong, TMD, Birck, C, Brautigam, CA, Brennerman, W, Byron, O, Bzowska, A, Chaires, JB, Chaton, CT, Coelfen, H, Connaghan, KD, Crowley, KA, Curth, U, Daviter, T, Dean, WL, Diez, AI, Ebel, C, Eckert, DM, Eisele, LE, Eisenstein, E, England, P, Escalante, C, Fagan, JA, Fairman, R, Finn, RM, Fischle, W, Garcia de la Torre, J, Gor, J, Gustafsson, H, Hall, D, Harding, SE, Hernandez Cifre, JG, Herr, AB, Howell, EE, Isaac, RS, Jao, S-C, Jose, D, Kim, S-J, Kokona, B, Kornblatt, JA, Kosek, D, Krayukhina, E, Krzizike, D, Kusznir, EA, Kwon, H, Larson, A, Laue, TM, Le Roy, A, Leech, AP, Lilie, H, Luger, K, Luque-Ortega, JR, Ma, J, May, CA, Maynard, EL, Modrak-Wojcik, A, Mok, Y-F, Muecke, N, Nagel-Steger, L, Narlikar, GJ, Noda, M, Nourse, A, Obsil, T, Park, CK, Park, J-K, Pawelek, PD, Perdue, EE, Perkins, SJ, Perugini, MA, Peterson, CL, Peverelli, MG, Piszczek, G, Prag, G, Prevelige, PE, Raynal, BDE, Rezabkova, L, Richter, K, Ringel, AE, Rosenberg, R, Rowe, AJ, Rufer, AC, Scott, DJ, Seravalli, JG, Solovyova, AS, Song, R, Staunton, D, Stoddard, C, Stott, K, Strauss, HM, Streicher, WW, Sumida, JP, Swygert, SG, Szczepanowski, RH, Tessmer, I, Toth, RT, Tripathy, A, Uchiyama, S, Uebel, SFW, Unzai, S, Gruber, AV, von Hippel, PH, Wandrey, C, Wang, S-H, Weitzel, SE, Wielgus-Kutrowska, B, Wolberger, C, Wolff, M, Wright, E, Wu, Y-S, Wubben, JM, Schuck, P, Langowski, J, Zhao, H, Ghirlando, R, Alfonso, C, Arisaka, F, Attali, I, Bain, DL, Bakhtina, MM, Becker, DF, Bedwell, GJ, Bekdemir, A, Besong, TMD, Birck, C, Brautigam, CA, Brennerman, W, Byron, O, Bzowska, A, Chaires, JB, Chaton, CT, Coelfen, H, Connaghan, KD, Crowley, KA, Curth, U, Daviter, T, Dean, WL, Diez, AI, Ebel, C, Eckert, DM, Eisele, LE, Eisenstein, E, England, P, Escalante, C, Fagan, JA, Fairman, R, Finn, RM, Fischle, W, Garcia de la Torre, J, Gor, J, Gustafsson, H, Hall, D, Harding, SE, Hernandez Cifre, JG, Herr, AB, Howell, EE, Isaac, RS, Jao, S-C, Jose, D, Kim, S-J, Kokona, B, Kornblatt, JA, Kosek, D, Krayukhina, E, Krzizike, D, Kusznir, EA, Kwon, H, Larson, A, Laue, TM, Le Roy, A, Leech, AP, Lilie, H, Luger, K, Luque-Ortega, JR, Ma, J, May, CA, Maynard, EL, Modrak-Wojcik, A, Mok, Y-F, Muecke, N, Nagel-Steger, L, Narlikar, GJ, Noda, M, Nourse, A, Obsil, T, Park, CK, Park, J-K, Pawelek, PD, Perdue, EE, Perkins, SJ, Perugini, MA, Peterson, CL, Peverelli, MG, Piszczek, G, Prag, G, Prevelige, PE, Raynal, BDE, Rezabkova, L, Richter, K, Ringel, AE, Rosenberg, R, Rowe, AJ, Rufer, AC, Scott, DJ, Seravalli, JG, Solovyova, AS, Song, R, Staunton, D, Stoddard, C, Stott, K, Strauss, HM, Streicher, WW, Sumida, JP, Swygert, SG, Szczepanowski, RH, Tessmer, I, Toth, RT, Tripathy, A, Uchiyama, S, Uebel, SFW, Unzai, S, Gruber, AV, von Hippel, PH, Wandrey, C, Wang, S-H, Weitzel, SE, Wielgus-Kutrowska, B, Wolberger, C, Wolff, M, Wright, E, Wu, Y-S, Wubben, JM, and Schuck, P

Abstract

Analytical ultracentrifugation (AUC) is a first principles based method to determine absolute sedimentation coefficients and buoyant molar masses of macromolecules and their complexes, reporting on their size and shape in free solution. The purpose of this multi-laboratory study was to establish the precision and accuracy of basic data dimensions in AUC and validate previously proposed calibration techniques. Three kits of AUC cell assemblies containing radial and temperature calibration tools and a bovine serum albumin (BSA) reference sample were shared among 67 laboratories, generating 129 comprehensive data sets. These allowed for an assessment of many parameters of instrument performance, including accuracy of the reported scan time after the start of centrifugation, the accuracy of the temperature calibration, and the accuracy of the radial magnification. The range of sedimentation coefficients obtained for BSA monomer in different instruments and using different optical systems was from 3.655 S to 4.949 S, with a mean and standard deviation of (4.304 ± 0.188) S (4.4%). After the combined application of correction factors derived from the external calibration references for elapsed time, scan velocity, temperature, and radial magnification, the range of s-values was reduced 7-fold with a mean of 4.325 S and a 6-fold reduced standard deviation of ± 0.030 S (0.7%). In addition, the large data set provided an opportunity to determine the instrument-to-instrument variation of the absolute radial positions reported in the scan files, the precision of photometric or refractometric signal magnitudes, and the precision of the calculated apparent molar mass of BSA monomer and the fraction of BSA dimers. These results highlight the necessity and effectiveness of independent calibration of basic AUC data dimensions for reliable quantitative studies.

Published
2015

3. Unraveling the molecular basis of subunit specificity in P pilus assembly by mass spectrometry\ud

Author

Rose, R.J., Verger, D., Daviter, T., Remaut, H., Paci, E., Waksman, G., Ashcroft, A.E., and Radford, S.E.

Abstract

P pili are multisubunit fibers essential for the attachment of uropathogenic Escherichia coli to the kidney. These fibers are formed by the noncovalent assembly of six different homologous subunit types in an array that is strictly defined in terms of both the number and order of each subunit type. Assembly occurs through a mechanism termed “donor-strand exchange (DSE)” in which an N-terminal extension (Nte) of one subunit donates a β-strand to an adjacent subunit, completing its Ig fold. Despite structural determination of the different subunits, the mechanism determining specificity of subunit ordering in pilus assembly remained unclear. Here, we have used noncovalent mass spectrometry to monitor DSE between all 30 possible pairs of P pilus subunits and their Ntes. We demonstrate a striking correlation between the natural order of subunits in pili and their ability to undergo DSE in vitro. The results reveal insights into the molecular mechanism by which subunit ordering during the assembly of this complex is achieved.

Published
2008

9. Structural Determinants of Polymerization Reactivity of the P pilus Adaptor Subunit PapF

Author

Gabriel Waksman, Alison E. Ashcroft, Gregory T. Costakes, R.J. Rose, Scott J. Hultgren, Han Remaut, Tina Daviter, Emanuele Paci, Denis Verger, Sheena E. Radford, Department of Bio-engineering Sciences, Structural Biology Brussels, Verger D., Rose R.J., Paci E., Costakes G., Daviter T., Hultgren S., Remaut H., Ashcroft A.E., Radford S.E., and Waksman G.

Subjects
Models, Molecular, MICROBIO, Protein Conformation, PROTEINS, Protein subunit, Molecular Sequence Data, Molecular Chaperones/chemistry, Sequence alignment, Biology, Periplasmic Proteins/chemistry, Pilus, Fimbriae Proteins/chemistry, 03 medical and health sciences, 0302 clinical medicine, Protein structure, Bacterial Proteins, Bacterial Proteins/chemistry, Structural Biology, Computer Simulation, Amino Acid Sequence, Proton-Translocating ATPases/chemistry, Molecular Biology, Peptide sequence, 030304 developmental biology, 0303 health sciences, Escherichia coli Proteins, Molecular biology, N-terminus, Proton-Translocating ATPases, kinetics, Fimbriae, Bacterial, Escherichia coli Proteins/chemistry, Biophysics, Fimbriae Proteins, Periplasmic Proteins, Bacterial outer membrane, Sequence Alignment, Fimbriae, Bacterial/chemistry, 030217 neurology & neurosurgery, Biogenesis, Molecular Chaperones
Abstract

P pili are important adhesive fibers involved in kidney infection by uropathogenic Escherichia coli. Pilus subunits are characterized by a large groove resulting from lack of a β strand. Polymerization of pilus subunits occurs via the donor-strand exchange (DSE) mechanism initiated when the N terminus of an incoming subunit interacts with the P5 region/pocket of the previously assembled subunit groove. Here, we solve the structure of the PapD:PapF complex in order to understand why PapF undergoes slow DSE. The structure reveals that the PapF P5 pocket is partially obstructed. MD simulations show this region of PapF is flexible compared with its equivalent in PapH, a subunit that also has an obstructed P5 pocket and is unable to undergo DSE. Using electrospray-ionization mass spectrometry, we show that mutations in the P5 region result in increased DSE rates. Thus, partial obstruction of the P5 pocket serves as a modulating mechanism of DSE. © 2008 Elsevier Ltd. All rights reserved.

Published
2008
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10. Unraveling the molecular basis of subunit specificity in P pilus assembly by mass spectrometry

Author

Gabriel Waksman, Tina Daviter, Sheena E. Radford, Denis Verger, Alison E. Ashcroft, Han Remaut, Emanuele Paci, R.J. Rose, Structural Biology Brussels, Rose R.J., Verger D., Daviter T., Remaut H., Paci E., Waksman G., Ashcroft A.E., and Radford S.E.

Subjects
Models, Molecular, Pilus assembly, Spectrometry, Mass, Electrospray Ionization, Specificity factor, Protein subunit, Molecular Sequence Data, Biology, medicine.disease_cause, Peptides/chemistry, Pilus, Electrospray ionization, medicine, Amino Acid Sequence, Escherichia coli, Peptide sequence, Multidisciplinary, Donor strand exchange, Uropathogenic bacteria, Biological Sciences, Protein Subunits, Biochemistry, Noncovalent protein complexe, Protein Subunits/chemistry, Fimbriae, Bacterial, Biophysics, Bacterial outer membrane, Peptides, Biogenesis, Fimbriae, Bacterial/chemistry, Molecular Chaperones
Abstract

P pili are multisubunit fibers essential for the attachment of uropathogenic Escherichia coli to the kidney. These fibers are formed by the noncovalent assembly of six different homologous subunit types in an array that is strictly defined in terms of both the number and order of each subunit type. Assembly occurs through a mechanism termed “donor-strand exchange (DSE)” in which an N-terminal extension (Nte) of one subunit donates a β-strand to an adjacent subunit, completing its Ig fold. Despite structural determination of the different subunits, the mechanism determining specificity of subunit ordering in pilus assembly remained unclear. Here, we have used noncovalent mass spectrometry to monitor DSE between all 30 possible pairs of P pilus subunits and their Ntes. We demonstrate a striking correlation between the natural order of subunits in pili and their ability to undergo DSE in vitro . The results reveal insights into the molecular mechanism by which subunit ordering during the assembly of this complex is achieved.

Published
2008

11. Structural and thermodynamic analyses of the β-to-α transformation in RfaH reveal principles of fold-switching proteins.

Author

Zuber PK, Daviter T, Heißmann R, Persau U, Schweimer K, and Knauer SH

Subjects
Escherichia coli metabolism, Thermodynamics, Transcription Factors metabolism, Escherichia coli Proteins metabolism, Peptide Elongation Factors metabolism, Trans-Activators metabolism, Protein Folding
Abstract

The two-domain protein RfaH, a paralog of the universally conserved NusG/Spt5 transcription factors, is regulated by autoinhibition coupled to the reversible conformational switch of its 60-residue C-terminal Kyrpides, Ouzounis, Woese (KOW) domain between an α-hairpin and a β-barrel. In contrast, NusG/Spt5-KOW domains only occur in the β-barrel state. To understand the principles underlying the drastic fold switch in RfaH, we elucidated the thermodynamic stability and the structural dynamics of two RfaH- and four NusG/Spt5-KOW domains by combining biophysical and structural biology methods. We find that the RfaH-KOW β-barrel is thermodynamically less stable than that of most NusG/Spt5-KOWs and we show that it is in equilibrium with a globally unfolded species, which, strikingly, contains two helical regions that prime the transition toward the α-hairpin. Our results suggest that transiently structured elements in the unfolded conformation might drive the global folding transition in metamorphic proteins in general., Competing Interests: PZ, TD, RH, UP, KS, SK No competing interests declared, (© 2022, Zuber et al.)

Published
2022
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12. An entropic safety catch controls hepatitis C virus entry and antibody resistance.

Author

Stejskal L, Kalemera MD, Lewis CB, Palor M, Walker L, Daviter T, Lees WD, Moss DS, Kremyda-Vlachou M, Kozlakidis Z, Gallo G, Bailey D, Rosenberg W, Illingworth CJR, Shepherd AJ, and Grove J

Subjects
Antibodies, Neutralizing, Entropy, Humans, Viral Envelope Proteins metabolism, Virus Internalization, Hepacivirus genetics, Hepacivirus metabolism, Hepatitis C
Abstract

E1 and E2 (E1E2), the fusion proteins of Hepatitis C Virus (HCV), are unlike that of any other virus yet described, and the detailed molecular mechanisms of HCV entry/fusion remain unknown. Hypervariable region-1 (HVR-1) of E2 is a putative intrinsically disordered protein tail. Here, we demonstrate that HVR-1 has an autoinhibitory function that suppresses the activity of E1E2 on free virions; this is dependent on its conformational entropy. Thus, HVR-1 is akin to a safety catch that prevents premature triggering of E1E2 activity. Crucially, this mechanism is turned off by host receptor interactions at the cell surface to allow entry. Mutations that reduce conformational entropy in HVR-1, or genetic deletion of HVR-1, turn off the safety catch to generate hyper-reactive HCV that exhibits enhanced virus entry but is thermally unstable and acutely sensitive to neutralising antibodies. Therefore, the HVR-1 safety catch controls the efficiency of virus entry and maintains resistance to neutralising antibodies. This discovery provides an explanation for the ability of HCV to persist in the face of continual immune assault and represents a novel regulatory mechanism that is likely to be found in other viral fusion machinery., Competing Interests: LS, MK, CL, MP, LW, TD, WL, DM, MK, GG, DB, WR, CI, AS, JG No competing interests declared, ZK Where authors are identified as personnel of the International Agency for Research on Cancer/WHO, the authors alone are responsible for the views expressed in this article and they do not necessarily represent the decisions, policy or views of the International Agency for Research on Cancer/WHO, (© 2022, Stejskal, Kalemera et al.)

Published
2022
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13. Correction to: Reproducibility and accuracy of microscale thermophoresis in the NanoTemper Monolith: a multi laboratory benchmark study.

Author

López-Méndez B, Baron B, Brautigam CA, Jowitt TA, Knauer SH, Uebel S, Williams MA, Sedivy A, Abian O, Abreu C, Adamczyk M, Bal W, Berger S, Buell AK, Carolis C, Daviter T, Fish A, Garcia-Alai M, Guenther C, Hamacek J, Holková J, Houser J, Johnson C, Kelly S, Leech A, Mas C, Matulis D, McLaughlin SH, Montserret R, Nasreddine R, Nehmé R, Nguyen Q, Ortega-Alarcón D, Perez K, Pirc K, Piszczek G, Podobnik M, Rodrigo N, Rokov-Plavec J, Schaefer S, Sharpe T, Southall J, Staunton D, Tavares P, Vanek O, Weyand M, and Wu D

Published
2021
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14. Design, synthesis, and evaluation of peptide-imidazo[1,2-a]pyrazine bioconjugates as potential bivalent inhibitors of the VirB11 ATPase HP0525.

Author

Sayer JR, Walldén K, Koss H, Allan H, Daviter T, Gane PJ, Waksman G, and Tabor AB

Subjects
Bacterial Proteins, Peptides pharmacology, Pyrazines, Adenosine Triphosphatases, Helicobacter pylori
Abstract

Helicobacter pylori (H. pylori) infections have been implicated in the development of gastric ulcers and various cancers: however, the success of current therapies is compromised by rising antibiotic resistance. The virulence and pathogenicity of H. pylori is mediated by the type IV secretion system (T4SS), a multiprotein macromolecular nanomachine that transfers toxic bacterial factors and plasmid DNA between bacterial cells, thus contributing to the spread of antibiotic resistance. A key component of the T4SS is the VirB11 ATPase HP0525, which is a hexameric protein assembly. We have previously reported the design and synthesis of a series of novel 8-amino imidazo[1,2-a]pyrazine derivatives as inhibitors of HP0525. In order to improve their selectivity, and potentially develop these compounds as tools for probing the assembly of the HP0525 hexamer, we have explored the design and synthesis of potential bivalent inhibitors. We used the structural details of the subunit-subunit interactions within the HP0525 hexamer to design peptide recognition moieties of the subunit interface. Different methods (cross metathesis, click chemistry, and cysteine-malemide) for bioconjugation to selected 8-amino imidazo[1,2-a]pyrazines were explored, as well as peptides spanning larger or smaller regions of the interface. The IC 50 values of the resulting linker-8-amino imidazo[1,2-a]pyrazine derivatives, and the bivalent inhibitors, were related to docking studies with the HP0525 crystal structure and to molecular dynamics simulations of the peptide recognition moieties., (© 2021 The Authors. Journal of Peptide Science published by European Peptide Society and John Wiley & Sons Ltd.)

Published
2021
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15. Reproducibility and accuracy of microscale thermophoresis in the NanoTemper Monolith: a multi laboratory benchmark study.

Author

López-Méndez B, Baron B, Brautigam CA, Jowitt TA, Knauer SH, Uebel S, Williams MA, Sedivy A, Abian O, Abreu C, Adamczyk M, Bal W, Berger S, Buell AK, Carolis C, Daviter T, Fish A, Garcia-Alai M, Guenther C, Hamacek J, Holková J, Houser J, Johnson C, Kelly S, Leech A, Mas C, Matulis D, McLaughlin SH, Montserret R, Nasreddine R, Nehmé R, Nguyen Q, Ortega-Alarcón D, Perez K, Pirc K, Piszczek G, Podobnik M, Rodrigo N, Rokov-Plavec J, Schaefer S, Sharpe T, Southall J, Staunton D, Tavares P, Vanek O, Weyand M, and Wu D

Subjects
Calorimetry, Reproducibility of Results, Temperature, Laboratories
Abstract

Microscale thermophoresis (MST), and the closely related Temperature Related Intensity Change (TRIC), are synonyms for a recently developed measurement technique in the field of biophysics to quantify biomolecular interactions, using the (capillary-based) NanoTemper Monolith and (multiwell plate-based) Dianthus instruments. Although this technique has been extensively used within the scientific community due to its low sample consumption, ease of use, and ubiquitous applicability, MST/TRIC has not enjoyed the unambiguous acceptance from biophysicists afforded to other biophysical techniques like isothermal titration calorimetry (ITC) or surface plasmon resonance (SPR). This might be attributed to several facts, e.g., that various (not fully understood) effects are contributing to the signal, that the technique is licensed to only a single instrument developer, NanoTemper Technology, and that its reliability and reproducibility have never been tested independently and systematically. Thus, a working group of ARBRE-MOBIEU has set up a benchmark study on MST/TRIC to assess this technique as a method to characterize biomolecular interactions. Here we present the results of this study involving 32 scientific groups within Europe and two groups from the US, carrying out experiments on 40 Monolith instruments, employing a standard operation procedure and centrally prepared samples. A protein-small molecule interaction, a newly developed protein-protein interaction system and a pure dye were used as test systems. We characterized the instrument properties and evaluated instrument performance, reproducibility, the effect of different analysis tools, the influence of the experimenter during data analysis, and thus the overall reliability of this method.

Published
2021
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16. The crystal structure of the Sgt1-Skp1 complex: the link between Hsp90 and both SCF E3 ubiquitin ligases and kinetochores.

Author

Willhoft O, Kerr R, Patel D, Zhang W, Al-Jassar C, Daviter T, Millson SH, Thalassinos K, and Vaughan CK

Subjects
Adaptor Proteins, Signal Transducing metabolism, Amino Acid Sequence, Binding Sites, Conserved Sequence, F-Box Proteins metabolism, HSP90 Heat-Shock Proteins metabolism, Kinetochores metabolism, Protein Binding, Protein Interaction Domains and Motifs, Protein Multimerization, Recombinant Proteins, SKP Cullin F-Box Protein Ligases metabolism, Saccharomyces cerevisiae Proteins metabolism, Adaptor Proteins, Signal Transducing chemistry, F-Box Proteins chemistry, HSP90 Heat-Shock Proteins chemistry, Kinetochores chemistry, Models, Molecular, Protein Conformation, SKP Cullin F-Box Protein Ligases chemistry, Saccharomyces cerevisiae Proteins chemistry
Abstract

The essential cochaperone Sgt1 recruits Hsp90 chaperone activity to a range of cellular factors including SCF E3 ubiquitin ligases and the kinetochore in eukaryotes. In these pathways Sgt1 interacts with Skp1, a small protein that heterodimerizes with proteins containing the F-box motif. We have determined the crystal structure of the interacting domains of Saccharomyces cerevisiae Sgt1 and Skp1 at 2.8 Å resolution and validated the interface in the context of the full-length proteins in solution. The BTB/POZ domain of Skp1 associates with Sgt1 via the concave surface of its TPR domain using residues that are conserved in humans. Dimerization of yeast Sgt1 occurs via an insertion that is absent from monomeric human Sgt1. We identify point mutations that disrupt dimerization and Skp1 binding in vitro and find that the interaction with Skp1 is an essential function of Sgt1 in yeast. Our data provide a structural rationale for understanding the phenotypes of temperature-sensitive Sgt1 mutants and for linking Skp1-associated proteins to Hsp90-dependent pathways., Competing Interests: The authors declare no competing financial interests.

Published
2017
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17. Repression of RNA polymerase by the archaeo-viral regulator ORF145/RIP.

Author

Sheppard C, Blombach F, Belsom A, Schulz S, Daviter T, Smollett K, Mahieu E, Erdmann S, Tinnefeld P, Garrett R, Grohmann D, Rappsilber J, and Werner F

Subjects
Promoter Regions, Genetic, Sulfolobus, Transcription Initiation, Genetic, Transcription, Genetic, Acidianus metabolism, DNA-Directed RNA Polymerases metabolism, Viral Proteins metabolism
Abstract

Little is known about how archaeal viruses perturb the transcription machinery of their hosts. Here we provide the first example of an archaeo-viral transcription factor that directly targets the host RNA polymerase (RNAP) and efficiently represses its activity. ORF145 from the temperate Acidianus two-tailed virus (ATV) forms a high-affinity complex with RNAP by binding inside the DNA-binding channel where it locks the flexible RNAP clamp in one position. This counteracts the formation of transcription pre-initiation complexes in vitro and represses abortive and productive transcription initiation, as well as elongation. Both host and viral promoters are subjected to ORF145 repression. Thus, ORF145 has the properties of a global transcription repressor and its overexpression is toxic for Sulfolobus. On the basis of its properties, we have re-named ORF145 RNAP Inhibitory Protein (RIP).

Published
2016
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18. A multilaboratory comparison of calibration accuracy and the performance of external references in analytical ultracentrifugation.

Author

Zhao H, Ghirlando R, Alfonso C, Arisaka F, Attali I, Bain DL, Bakhtina MM, Becker DF, Bedwell GJ, Bekdemir A, Besong TM, Birck C, Brautigam CA, Brennerman W, Byron O, Bzowska A, Chaires JB, Chaton CT, Cölfen H, Connaghan KD, Crowley KA, Curth U, Daviter T, Dean WL, Díez AI, Ebel C, Eckert DM, Eisele LE, Eisenstein E, England P, Escalante C, Fagan JA, Fairman R, Finn RM, Fischle W, de la Torre JG, Gor J, Gustafsson H, Hall D, Harding SE, Cifre JG, Herr AB, Howell EE, Isaac RS, Jao SC, Jose D, Kim SJ, Kokona B, Kornblatt JA, Kosek D, Krayukhina E, Krzizike D, Kusznir EA, Kwon H, Larson A, Laue TM, Le Roy A, Leech AP, Lilie H, Luger K, Luque-Ortega JR, Ma J, May CA, Maynard EL, Modrak-Wojcik A, Mok YF, Mücke N, Nagel-Steger L, Narlikar GJ, Noda M, Nourse A, Obsil T, Park CK, Park JK, Pawelek PD, Perdue EE, Perkins SJ, Perugini MA, Peterson CL, Peverelli MG, Piszczek G, Prag G, Prevelige PE, Raynal BD, Rezabkova L, Richter K, Ringel AE, Rosenberg R, Rowe AJ, Rufer AC, Scott DJ, Seravalli JG, Solovyova AS, Song R, Staunton D, Stoddard C, Stott K, Strauss HM, Streicher WW, Sumida JP, Swygert SG, Szczepanowski RH, Tessmer I, Toth RT 4th, Tripathy A, Uchiyama S, Uebel SF, Unzai S, Gruber AV, von Hippel PH, Wandrey C, Wang SH, Weitzel SE, Wielgus-Kutrowska B, Wolberger C, Wolff M, Wright E, Wu YS, Wubben JM, and Schuck P

Subjects
Calibration, Reproducibility of Results, Ultracentrifugation methods, Ultracentrifugation standards
Abstract

Analytical ultracentrifugation (AUC) is a first principles based method to determine absolute sedimentation coefficients and buoyant molar masses of macromolecules and their complexes, reporting on their size and shape in free solution. The purpose of this multi-laboratory study was to establish the precision and accuracy of basic data dimensions in AUC and validate previously proposed calibration techniques. Three kits of AUC cell assemblies containing radial and temperature calibration tools and a bovine serum albumin (BSA) reference sample were shared among 67 laboratories, generating 129 comprehensive data sets. These allowed for an assessment of many parameters of instrument performance, including accuracy of the reported scan time after the start of centrifugation, the accuracy of the temperature calibration, and the accuracy of the radial magnification. The range of sedimentation coefficients obtained for BSA monomer in different instruments and using different optical systems was from 3.655 S to 4.949 S, with a mean and standard deviation of (4.304 ± 0.188) S (4.4%). After the combined application of correction factors derived from the external calibration references for elapsed time, scan velocity, temperature, and radial magnification, the range of s-values was reduced 7-fold with a mean of 4.325 S and a 6-fold reduced standard deviation of ± 0.030 S (0.7%). In addition, the large data set provided an opportunity to determine the instrument-to-instrument variation of the absolute radial positions reported in the scan files, the precision of photometric or refractometric signal magnitudes, and the precision of the calculated apparent molar mass of BSA monomer and the fraction of BSA dimers. These results highlight the necessity and effectiveness of independent calibration of basic AUC data dimensions for reliable quantitative studies.

Published
2015
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19. Nanofiber-based delivery of therapeutic peptides to the brain.

Author

Mazza M, Notman R, Anwar J, Rodger A, Hicks M, Parkinson G, McCarthy D, Daviter T, Moger J, Garrett N, Mead T, Briggs M, Schätzlein AG, and Uchegbu IF

Subjects
Blood-Brain Barrier metabolism, Drug Carriers metabolism, Enkephalin, Leucine-2-Alanine metabolism, Enkephalin, Leucine-2-Alanine therapeutic use, Models, Molecular, Nanomedicine, Peptides metabolism, Protein Conformation, Brain metabolism, Drug Carriers chemistry, Enkephalin, Leucine-2-Alanine analogs & derivatives, Nanofibers chemistry, Peptides chemistry
Abstract

The delivery of therapeutic peptides and proteins to the central nervous system is the biggest challenge when developing effective neuropharmaceuticals. The central issue is that the blood-brain barrier is impermeable to most molecules. Here we demonstrate the concept of employing an amphiphilic derivative of a peptide to deliver the peptide into the brain. The key to success is that the amphiphilic peptide should by design self-assemble into nanofibers wherein the active peptide epitope is tightly wrapped around the nanofiber core. The nanofiber form appears to protect the amphiphilic peptide from degradation while in the plasma, and the amphiphilic nature of the peptide promotes its transport across the blood-brain barrier. Therapeutic brain levels of the amphiphilic peptide are achieved with this strategy, compared with the absence of detectable peptide in the brain and the consequent lack of a therapeutic response when the underivatized peptide is administered.

Published
2013
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20. Archaeology of RNA polymerase: factor swapping during the transcription cycle.

Author

Blombach F, Daviter T, Fielden D, Grohmann D, Smollett K, and Werner F

Subjects
DNA-Directed RNA Polymerases genetics, Evolution, Molecular, Models, Molecular, Promoter Regions, Genetic, Protein Biosynthesis, DNA-Directed RNA Polymerases metabolism, Transcription Factors metabolism
Abstract

All RNAPs (RNA polymerases) repeatedly make use of their DNA template by progressing through the transcription cycle multiple times. During transcription initiation and elongation, distinct sets of transcription factors associate with multisubunit RNAPs and modulate their nucleic-acid-binding and catalytic properties. Between the initiation and elongation phases of the cycle, the factors have to be exchanged by a largely unknown mechanism. We have shown that the binding sites for initiation and elongation factors are overlapping and that the binding of the factors to RNAP is mutually exclusive. This ensures an efficient exchange or 'swapping' of factors and could furthermore assist RNAP during promoter escape, enabling robust transcription. A similar mechanism applies to the bacterial RNAP system. The elongation factors are evolutionarily conserved between the bacterial (NusG) and archaeo-eukaryotic (Spt5) systems; however, the initiation factors [σ and TBP (TATA-box-binding protein)/TF (transcription factor) B respectively] are not. Therefore we propose that this factor-swapping mechanism, operating in all three domains of life, is the outcome of convergent evolution.

Published
2013
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21. Measurement of protein-ligand complex formation.

Author

Lowe PN, Vaughan CK, and Daviter T

Subjects
Autoradiography, Binding Sites, Binding, Competitive, Catalysis, Fluorescence Resonance Energy Transfer, Humans, Kinetics, Luminescent Measurements, Protein Binding, Thermodynamics, Ligands, Molecular Dynamics Simulation, Proteins chemistry
Abstract

Experimental approaches to detect, measure, and quantify protein-ligand binding, along with their theoretical bases, are described. A range of methods for detection of protein-ligand interactions is summarized. Specific protocols are provided for a nonequilibrium procedure pull-down assay, for an equilibrium direct binding method and its modification into a competition-based measurement and for steady-state measurements based on the effects of ligands on enzyme catalysis.

Published
2013
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22. Protein sample characterization.

Author

Daviter T and Fronzes R

Subjects
Chromatography, Gel, Circular Dichroism, Electrophoresis, Polyacrylamide Gel, Light, Membrane Proteins isolation & purification, Protein Stability, Scattering, Radiation, Solubility, Ultracentrifugation, Membrane Proteins chemistry
Abstract

Most biophysical experiments require protein samples of high quality and accurately determined concentration. This chapter attempts to compile basic information on the most common methods to assess the purity, dispersity, and stability of protein samples. It also reminds of methods to measure protein concentration and of their limits. The idea is to make aware and remind of the range of methods available and of commonly overlooked pitfalls. The aim is to enable experimenters to fully characterize their preparations of soluble or membrane proteins and gain reliable and reproducible results from their experimental work.

Published
2013
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23. Circular and linear dichroism spectroscopy for the study of protein-ligand interactions.

Author

Daviter T, Chmel N, and Rodger A

Subjects
Calibration, Circular Dichroism, Kinetics, Protein Binding, Protein Structure, Secondary, Signal-To-Noise Ratio, Stereoisomerism, Thermodynamics, Amino Acids chemistry, Ligands, Protein Subunits chemistry, Proteins chemistry
Abstract

Circular dichroism (CD) is the difference in absorption of left and right circularly polarized light, usually by a solution containing the molecules of interest. A non-zero signal for solutions is only measured for chiral molecules such as proteins whose mirror image is not superposable on the original molecule. A CD spectrum provides information about the bonds and structures responsible for the chirality. When a small molecule (or ligand) binds to a protein, it acquires an induced CD (ICD) spectrum through chiral perturbation to its structure or electron rearrangements (transitions). The wavelengths of this ICD are determined by the ligand's own absorption spectrum, and the intensity of the ICD spectrum is determined by the strength and geometry of its interaction with the protein. Thus, ICD can be used to probe the binding of ligands to proteins. This chapter contains an outline of how to perform protein CD and ICD experiments, together with some of the issues relating to experimental design and implementation. Addition of a quarter wave plate to a CD spectropolarimeter converts it to a linear dichroism (LD) spectrometer. When protein samples are aligned either in flow (as for fibers or membrane proteins in liposomes) or on surfaces the orientations of ligands with respect to the protein backbone or other subunits can be determined.

Published
2013
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24. Crystal structure of reduced MsAcg, a putative nitroreductase from Mycobacterium smegmatis and a close homologue of Mycobacterium tuberculosis Acg.

Author

Chauviac FX, Bommer M, Yan J, Parkin G, Daviter T, Lowden P, Raven EL, Thalassinos K, and Keep NH

Subjects
Binding Sites, Crystallography, X-Ray, Flavin Mononucleotide metabolism, Models, Molecular, Mycobacterium smegmatis chemistry, Mycobacterium smegmatis genetics, Mycobacterium tuberculosis chemistry, Mycobacterium tuberculosis genetics, NAD metabolism, NADP metabolism, Nitroreductases genetics, Nitroreductases metabolism, Mycobacterium smegmatis enzymology, Mycobacterium tuberculosis enzymology, Nitroreductases chemistry
Abstract

This paper presents the structure of MsAcg (MSMEG_5246), a Mycobacterium smegmatis homologue of Mycobacterium tuberculosis Acg (Rv2032) in its reduced form at 1.6 Å resolution using x-ray crystallography. Rv2032 is one of the most induced genes under the hypoxic model of tuberculosis dormancy. The Acg family turns out to be unusual flavin mononucleotide (FMN)-binding proteins that have probably arisen by gene duplication and fusion from a classical homodimeric nitroreductase such that the monomeric protein resembles a classical nitroreductase dimer but with one active site deleted and the other active site covered by a unique lid. The FMN cofactor is not reduced by either NADH or NADPH, but the chemically reduced enzyme is capable of reduction of nitro substrates, albeit at no kinetic advantage over free FMN. The reduced enzyme is rapidly oxidized by oxygen but without any evidence for a radical state commonly seen in oxygen-sensitive nitroreductases. The presence of the unique lid domain, the lack of reduction by NAD(P)H, and the slow rate of reaction of the chemically reduced protein raises a possible alternative function of Acg proteins in FMN storage or sequestration from other biochemical pathways as part of the bacteria's adaptation to a dormancy state.

Published
2012
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25. In silico assessment of potential druggable pockets on the surface of α1-antitrypsin conformers.

Author

Patschull AO, Gooptu B, Ashford P, Daviter T, and Nobeli I

Subjects
Humans, Protein Structure, Quaternary, Protein Structure, Tertiary, alpha 1-Antitrypsin genetics, Molecular Dynamics Simulation, Protein Multimerization, alpha 1-Antitrypsin chemistry
Abstract

The search for druggable pockets on the surface of a protein is often performed on a single conformer, treated as a rigid body. Transient druggable pockets may be missed in this approach. Here, we describe a methodology for systematic in silico analysis of surface clefts across multiple conformers of the metastable protein α(1)-antitrypsin (A1AT). Pathological mutations disturb the conformational landscape of A1AT, triggering polymerisation that leads to emphysema and hepatic cirrhosis. Computational screens for small molecule inhibitors of polymerisation have generally focused on one major druggable site visible in all crystal structures of native A1AT. In an alternative approach, we scan all surface clefts observed in crystal structures of A1AT and in 100 computationally produced conformers, mimicking the native solution ensemble. We assess the persistence, variability and druggability of these pockets. Finally, we employ molecular docking using publicly available libraries of small molecules to explore scaffold preferences for each site. Our approach identifies a number of novel target sites for drug design. In particular one transient site shows favourable characteristics for druggability due to high enclosure and hydrophobicity. Hits against this and other druggable sites achieve docking scores corresponding to a K(d) in the µM-nM range, comparing favourably with a recently identified promising lead. Preliminary ThermoFluor studies support the docking predictions. In conclusion, our strategy shows considerable promise compared with the conventional single pocket/single conformer approach to in silico screening. Our best-scoring ligands warrant further experimental investigation.

Published
2012
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26. Characterization of an oxidoreductase from the arylamine N-acetyltransferase operon in Mycobacterium smegmatis.

Author

Evangelopoulos D, Cronin N, Daviter T, Sim E, Keep NH, and Bhakta S

Subjects
Arylamine N-Acetyltransferase chemistry, Crystallography, X-Ray, Humans, Models, Molecular, Mycobacterium smegmatis enzymology, NADP metabolism, Operon, Oxidoreductases metabolism, Recombinant Proteins genetics, Recombinant Proteins metabolism, Tetrahydrofolate Dehydrogenase metabolism, Arylamine N-Acetyltransferase genetics, Oxidoreductases genetics
Abstract

Mycobacterium tuberculosis, the most successful bacterial pathogen, causes tuberculosis, a disease that still causes more than 2 million deaths per year. Arylamine N-acetyltransferase is an enzyme that is conserved in most Mycobacterium spp. The nat gene belongs to an operon that is important for the intracellular survival of M. tuberculosis within macrophages. The nat operon in Mycobacterium smegmatis and other fast-growing mycobacterial species has a unique organization containing genes with uncharacterized function. Here, we describe the biochemical, biophysical and structural characterization of the MSMEG_0308 gene product (MS0308) of the M. smegmatis nat operon. While characterizing the function of MS0308, we validated the oxidoreductase property; however, we found that the enzyme was not utilizing dihydrofolate as its substrate, hence we first report that MS0308 is not a dihydrofolate reductase, as annotated in the genome. The structure of this oxidoreductase was solved at 2.0 Å in complex with the cofactor NADPH and has revealed the hydrophobic pocket where the endogenous substrate binds., (© 2011 The Authors Journal compilation © 2011 FEBS.)

Published
2011
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27. An undecided coiled coil: the leucine zipper of Nek2 kinase exhibits atypical conformational exchange dynamics.

Author

Croasdale R, Ivins FJ, Muskett F, Daviter T, Scott DJ, Hardy T, Smerdon SJ, Fry AM, and Pfuhl M

Subjects
Base Sequence, Circular Dichroism, DNA Primers, Humans, Mutagenesis, Site-Directed, NIMA-Related Kinases, Nuclear Magnetic Resonance, Biomolecular, Protein Conformation, Protein Serine-Threonine Kinases genetics, Ultracentrifugation, Leucine Zippers, Protein Serine-Threonine Kinases chemistry
Abstract

Leucine zippers are oligomerization domains used in a wide range of proteins. Their structure is based on a highly conserved heptad repeat sequence in which two key positions are occupied by leucines. The leucine zipper of the cell cycle-regulated Nek2 kinase is important for its dimerization and activation. However, the sequence of this leucine zipper is most unusual in that leucines occupy only one of the two hydrophobic positions. The other position, depending on the register of the heptad repeat, is occupied by either acidic or basic residues. Using NMR spectroscopy, we show that this leucine zipper exists in two conformations of almost equal population that exchange with a rate of 17 s(-1). We propose that the two conformations correspond to the two possible registers of the heptad repeat. This hypothesis is supported by a cysteine mutant that locks the protein in one of the two conformations. NMR spectra of this mutant showed the predicted 2-fold reduction of peaks in the (15)N HSQC spectrum and the complete removal of cross peaks in exchange spectra. It is possible that interconversion of these two conformations may be triggered by external signals in a manner similar to that proposed recently for the microtubule binding domain of dynein and the HAMP domain. As a result, the leucine zipper of Nek2 kinase is the first example where the frameshift of coiled-coil heptad repeats has been directly observed experimentally.

Published
2011
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28. Unraveling the molecular basis of subunit specificity in P pilus assembly by mass spectrometry.

Author

Rose RJ, Verger D, Daviter T, Remaut H, Paci E, Waksman G, Ashcroft AE, and Radford SE

Subjects
Amino Acid Sequence, Models, Molecular, Molecular Chaperones, Molecular Sequence Data, Peptides chemistry, Fimbriae, Bacterial chemistry, Protein Subunits chemistry, Spectrometry, Mass, Electrospray Ionization
Abstract

P pili are multisubunit fibers essential for the attachment of uropathogenic Escherichia coli to the kidney. These fibers are formed by the noncovalent assembly of six different homologous subunit types in an array that is strictly defined in terms of both the number and order of each subunit type. Assembly occurs through a mechanism termed "donor-strand exchange (DSE)" in which an N-terminal extension (Nte) of one subunit donates a beta-strand to an adjacent subunit, completing its Ig fold. Despite structural determination of the different subunits, the mechanism determining specificity of subunit ordering in pilus assembly remained unclear. Here, we have used noncovalent mass spectrometry to monitor DSE between all 30 possible pairs of P pilus subunits and their Ntes. We demonstrate a striking correlation between the natural order of subunits in pili and their ability to undergo DSE in vitro. The results reveal insights into the molecular mechanism by which subunit ordering during the assembly of this complex is achieved.

Published
2008
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29. A uniform response to mismatches in codon-anticodon complexes ensures ribosomal fidelity.

Author

Gromadski KB, Daviter T, and Rodnina MV

Subjects
Animals, Enzyme Activation, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, GTP Phosphohydrolases metabolism, Macromolecular Substances, Nucleic Acid Conformation, Peptide Elongation Factor Tu metabolism, RNA, Transfer, Amino Acid-Specific metabolism, Thermodynamics, Anticodon, Base Pair Mismatch, Codon, Protein Biosynthesis, Ribosomes metabolism
Abstract

Ribosomes take an active part in aminoacyl-tRNA selection by distinguishing correct and incorrect codon-anticodon pairs. Correct codon-anticodon complexes are recognized by a network of ribosome contacts that are specific for each position of the codon-anticodon duplex and involve A-minor RNA interactions. Here, we show by kinetic analysis that single mismatches at any position of the codon-anticodon complex result in slower forward reactions and a uniformly 1000-fold faster dissociation of the tRNA from the ribosome. This suggests that high-fidelity tRNA selection is achieved by a conformational switch of the decoding site between accepting and rejecting modes, regardless of the thermodynamic stability of the respective codon-anticodon complexes or their docking partners at the decoding site. The forward reactions on mismatched codons were particularly sensitive to the disruption of the A-minor interactions with 16S rRNA and determined the variations in the misreading efficiency of near-cognate codons.

Published
2006
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30. Essential role of histidine 84 in elongation factor Tu for the chemical step of GTP hydrolysis on the ribosome.

Author

Daviter T, Wieden HJ, and Rodnina MV

Subjects
Binding Sites, Guanosine 5'-O-(3-Thiotriphosphate) metabolism, Guanosine Triphosphate chemistry, Histidine genetics, Hydrogen-Ion Concentration, Hydrolysis, Kinetics, Macromolecular Substances, Peptide Elongation Factor Tu genetics, Peptides chemistry, Peptides metabolism, Protein Biosynthesis, RNA, Transfer, Phe metabolism, Ribosomes chemistry, Ribosomes genetics, Guanosine Triphosphate metabolism, Histidine chemistry, Peptide Elongation Factor Tu chemistry, Peptide Elongation Factor Tu metabolism, Ribosomes metabolism
Abstract

Elongation factor Tu (EF-Tu) is a GTP-binding protein that delivers aminoacyl-tRNA to the A site of the ribosome during protein synthesis. The mechanism of GTP hydrolysis in EF-Tu on the ribosome is poorly understood. It is known that mutations of a conserved histidine residue in the switch II region of the factor, His84 in Escherichia coli EF-Tu, impair GTP hydrolysis. However, the partial reaction which is directly affected by mutations of His84 was not identified and the effect on GTP hydrolysis was not quantified. Here, we show that the replacement of His84 with Ala reduces the rate constant of GTP hydrolysis more than 10(6)-fold, whereas the preceding steps of ternary complex binding to the ribosome, codon recognition and, most importantly, the GTPase activation step are affected only slightly. These results show that His84 plays a key role in the chemical step of GTP hydrolysis. Rate constants of GTP hydrolysis by wild-type EF-Tu, measured using the slowly hydrolyzable GTP analog, GTPgammaS, showed no dependence on pH, indicating that His84 does not act as a general base. We propose that the catalytic role of His84 is to stabilize the transition state of GTP hydrolysis by hydrogen bonding to the attacking water molecule or, possibly, the gamma-phosphate group of GTP.

Published
2003
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31. Structural dynamics of ribosomal RNA during decoding on the ribosome.

Author

Rodnina MV, Daviter T, Gromadski K, and Wintermeyer W

Subjects
Anticodon genetics, Binding Sites, Codon genetics, Crystallography, X-Ray, Guanosine Triphosphate metabolism, Kinetics, Models, Molecular, Nucleic Acid Conformation, Peptide Elongation Factor Tu metabolism, Protein Biosynthesis, Protein Conformation, RNA, Ribosomal chemistry, RNA, Ribosomal metabolism, Ribosomes metabolism, RNA, Ribosomal genetics, Ribosomes genetics
Abstract

Decoding is a multistep process by which the ribosome accurately selects aminoacyl-tRNA (aa-tRNA) that matches the mRNA codon in the A site. The correct geometry of the codon-anticodon complex is monitored by the ribosome, resulting in conformational changes in the decoding center of the small (30S) ribosomal subunit by an induced-fit mechanism. The recognition of aa-tRNA is modulated by changes of the ribosome conformation in regions other than the decoding center that may either affect the architecture of the latter or alter the communication of the 30S subunit with the large (50S) subunit where the GTPase and peptidyl transferase centers are located. Correct codon-anticodon complex formation greatly accelerates the rates of GTP hydrolysis and peptide bond formation, indicating the importance of crosstalk between the subunits and the role of the 50S subunit in aa-tRNA selection. In the present review, recent results of the ribosome crystallography, cryoelectron microscopy (cryo-EM), genetics, rapid kinetics and biochemical approaches are reviewed which show that the dynamics of the structure of ribosomal RNA (rRNA) play a crucial role in decoding.

Published
2002
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32. Late events of translation initiation in bacteria: a kinetic analysis.

Author

Tomsic J, Vitali LA, Daviter T, Savelsbergh A, Spurio R, Striebeck P, Wintermeyer W, Rodnina MV, and Gualerzi CO

Subjects
Codon genetics, Dipeptides biosynthesis, Dipeptides metabolism, Escherichia coli metabolism, Fluorescence, Guanosine Diphosphate metabolism, Guanosine Triphosphate metabolism, Hydrolysis, Kinetics, N-Formylmethionine metabolism, Peptide Elongation Factor Tu metabolism, Peptide Initiation Factors metabolism, Phenylalanine metabolism, Phosphates metabolism, Prokaryotic Initiation Factor-2, Protein Binding, RNA, Transfer, Met genetics, RNA, Transfer, Met metabolism, RNA, Transfer, Phe genetics, RNA, Transfer, Phe metabolism, Ribosomes chemistry, Ribosomes genetics, Ribosomes metabolism, Escherichia coli genetics, Peptide Chain Elongation, Translational, Peptide Chain Initiation, Translational, Protein Biosynthesis genetics
Abstract

Binding of the 50S ribosomal subunit to the 30S initiation complex and the subsequent transition from the initiation to the elongation phase up to the synthesis of the first peptide bond represent crucial steps in the translation pathway. The reactions that characterize these transitions were analyzed by quench-flow and fluorescence stopped-flow kinetic techniques. IF2-dependent GTP hydrolysis was fast (30/s) followed by slow P(i) release from the complex (1.5/s). The latter step was rate limiting for subsequent A-site binding of EF-Tu small middle dotGTP small middle dotPhe-tRNA(Phe) ternary complex. Most of the elemental rate constants of A-site binding were similar to those measured on poly(U), with the notable exception of the formation of the first peptide bond which occurred at a rate of 0.2/s. Omission of GTP or its replacement with GDP had no effect, indicating that neither the adjustment of fMet-tRNA(fMet) in the P site nor the release of IF2 from the ribosome required GTP hydrolysis.

Published
2000
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