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1

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Structure of (2R)-2-(1-aziridinyl)-3-(2-choroethyl)-2-oxo-1,3,2λ5-oxazaphosphorinane (1990)

Brzozowski, A. M. ; Stępien, A. ; Dauter, Z. ; [et al.]

Oxford [u.a.] : International Union of Crystallography (IUCr)

Acta crystallographica 46 (1990), S. 618-621

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ISSN: 1600-5759

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Chemistry and Pharmacology , Geosciences , Physics

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0108270189003677

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2

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Refinement of rubredoxin from Desulfovibrio vulgaris at 1.0 Å with and without restraints (1992)

Dauter, Z. ; Sieker, L. C. ; Wilson, K. S.

Copenhagen : International Union of Crystallography (IUCr)

Acta crystallographica 48 (1992), S. 42-59

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ISSN: 1600-5740

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Chemistry and Pharmacology , Geosciences , Physics

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0108768191010613

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3

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Refinement of hexamethylenetetramine based on diffractometer and imaging-plate data (1994)

Grochowski, J. ; Serda, P. ; Wilson, K. S. ; [et al.]

Copenhagen : International Union of Crystallography (IUCr)

Applied crystallography online 27 (1994), S. 722-726

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ISSN: 1600-5767

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Geosciences , Physics

Notes: Two data sets were collected on single crystals of hexamethylenetetramine (urotropin) using a four-circle diffractometer with Cu Kα radiation and an imaging-plate two-dimensional detector with Mo Kα source using the rotation method. Both data sets extend to the same limit of sin θ/λ = 0.62 Å−1, corresponding to a resolution of 0.81 Å. Different processing protocols were employed for the two sets of data. Structure refinements carried out separately with each data set led to equivalent results of comparable accuracy. The imaging-plate scanner was able to provide X-ray data of high quality in a significantly shorter time than the diffractometer.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0021889894002116

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4

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Crystallization and preliminary diffraction studies of the chemically synthesized domain A of Thermus flavus 5S rRNA: an RNA dodecamer double helix (1993)

Lorenz, S. ; Fürste, J. P. ; Bald, R. ; [et al.]

Copenhagen : International Union of Crystallography (IUCr)

Acta crystallographica 49 (1993), S. 418-420

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ISSN: 1399-0047

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Chemistry and Pharmacology , Geosciences , Physics

Notes: Crystals of domain A of Thermus flavus 5S rRNA have been obtained. The space group was found to be P43 with unit-cell dimensions a = b = 30.10 and c = 86.80 Å. Data to 2.3 Å have been recorded and solution of the structure is currently underway by means of molecular-replacement techniques.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0907444993001520

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5

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Crystallographic analyses of an active HIV-1 ribonuclease H domain show structural features that distinguish it from the inactive form (1993)

Chattopadhyay, D. ; Finzel, B. C. ; Munson, S. H. ; [et al.]

Copenhagen : International Union of Crystallography (IUCr)

Acta crystallographica 49 (1993), S. 423-427

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ISSN: 1399-0047

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Chemistry and Pharmacology , Geosciences , Physics

Notes: . An active recombinant preparation of the carboxy-terminal ribonuclease H (RNase H) domain of HIV-I reverse transcriptase has produced crystals of several different forms, including a trigonal prism form (P31; a = b = 52.03, c = 113.9 Å with two molecules per asymmetric unit) and a hexagonal tablet form (P6222 or P6422; a = b = 93.5, c = 74.1 Å with one molecule per asymmetric unit). The former appears to be isomorphous with crystals of a similar, but inactive, version of the enzyme that was used for a prior crystal structure determination [Davies, Hostomska, Hostomsky, Jordan & Matthews (1991). Science, 252, 88–95]. We have also obtained a structure solution for this crystal form and have refined it with 2.8 Å resolution data (R = 0.216). We report here details of our crystallization studies and some initial structural results that verify that the preparation of active HIV-1 RNase H yields a protein that is not just enzymatically, but also structurally, distinguishable from the inactive form. Evidence suggests that region 538–542, which may be involved in the catalytic site and which is disordered in both molecules in the prior structure determination, is ordered in the crystal structure of the active enzyme, although the ordering may include more than one conformation for this loop. It should also be noted that, in the crystal structure of the trigonal form, RNase H monomers associate to form noncrystallographic twofold-symmetric dimers by fusing five-stranded mixed β sheets into a single ten-stranded dimerwide sheet, an assembly that was not remarked upon by previous investigators.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0907444993002409

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6

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The application of direct methods and Patterson interpretation to high-resolution native protein data (1993)

Sheldrick, G. M. ; Dauter, Z. ; Wilson, K. S. ; [et al.]

Copenhagen : International Union of Crystallography (IUCr)

Acta crystallographica 49 (1993), S. 18-23

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ISSN: 1399-0047

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Chemistry and Pharmacology , Geosciences , Physics

Notes: Conventional small-molecule methods of solving the phase problem from native data alone, without the use of heavy-atom derivatives, known fragment geometries or anomalous dispersion, have been tested on 0.9 Å resolution data for two small proteins: rubredoxin, from Desulfovibrio vulgaris, and crambin. The presence of three disulfide bridges in crambin and an FeS4 unit in rubredoxin enabled automated Patterson interpretation as well as direct methods to be tried. Although both structures were already well established, the known structures were not used in the phasing attempts, except for identifying successful solutions. Direct methods were not successful for crambin, although the correct phases were stable to phase refinement and gave figures of merit clearly superior to any obtained in the ca 500 000 random starting phase sets that were refined. It appears that the presence of an iron atom in rubredoxin reduces the scale of the search problem by many orders of magnitude, but at the cost of producing `over-consistent' phase sets that overemphasize the iron atom and involve partial loss of enantiomorph information. However, about 1% of direct-methods trials were successful for rubredoxin, giving mean phase errors of about 56° (for all E 〉 1.2) that could be reduced to about 20° by standard E-Fourier recycling methods. Limiting the resolution of the data degraded the quality of the solutions and suggested that the limiting resolution for routine direct-methods solution of rubredoxin is about 1.2 Å. With the 0.9 Å data, automated Patterson interpretation convincingly finds the three disulfide bridges in crambin and the FeS4 unit in rubredoxin, and in both cases E-Fourier recycling starting from these `heavier' atoms yields almost the complete structure. Whereas crambin could only be solved in this way at very high resolution, rubredoxin could be solved by Patterson interpretation down to 1.6 Å. These results emphasize the benefits of collecting protein data to the highest possible resolution, and indicate that when a few `heavier' atoms are present, it may prove possible in favorable cases to solve the phase problem from a single native data set collected to `atomic resolution'.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0907444992007364

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7

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Structure of the ADP complex of the 3-phosphoglycerate kinase from Bacillus stearothermophilus at 1.65 Å (1994)

Davies, G. J. ; Gamblin, S. J. ; Littlechild, J. A. ; [et al.]

Copenhagen : International Union of Crystallography (IUCr)

Acta crystallographica 50 (1994), S. 202-209

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ISSN: 1399-0047

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Chemistry and Pharmacology , Geosciences , Physics

Notes: The structure of the ADP complex of the enzyme 3-phosphoglycerate kinase (PGK, E.C. 2.7.2.3) from Bacillus stearothermophilus NCA-1503 has been determined by the method of molecular replacement. The structure has been refined to an R factor of 0.16 for all data between 10.0 and 1.65 Å resolution, using data collected on the Hendrix–Lentfer imaging plate at the EMBL outstation in Hamburg. The r.m.s. deviations from stereochemical ideality are 0.010 and 0.011 Å for bonds and planes, respectively. Although crystallized in the presence of the nucleotide product MgATP, the high-resolution structure reveals the bound nucleotide to be MgADP reflecting the low intrinsic ATPase activity of PGK. Although the two domains of this enzyme are found to be some 4.5° closer together than is found in the yeast and horse-muscle apo-enzyme structures, this structure represents the `open' rather than the `closed', catalytically competent form, of the enzyme.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0907444993011138

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8

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High-resolution structures of single-metal-substituted concanavalin A: the Co,Ca-protein at 1.6 Å and the Ni,Ca-protein at 2.0 Å (1994)

Emmerich, C. ; Helliwell, J. R. ; Redshaw, M. ; [et al.]

Copenhagen : International Union of Crystallography (IUCr)

Acta crystallographica 50 (1994), S. 749-756

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ISSN: 1399-0047

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Chemistry and Pharmacology , Geosciences , Physics

Notes: The molecular structures of cobalt- and nickel-substituted concanavalin A have been refined at 1.6 and 2.0 Å resolution, respectively. Both metal derivatives crystallize in space group I222 with approximate cell dimensions a = 89, b = 87 and c = 63 Å and one monomer in the asymmetric unit. The final R factor for Co-substituted concanavalin A is 17.8% for 29 211 reflections with F 〉 1.0σ(F) between 8.0 and 1.6 Å. For Ni-substituted concanavalin A the final R factor is 15.9% for 16 128 reflections with F 〉 1.0σ(F) between 8.0 and 2.0 Å resolution. Both structures contain a transition-metal binding site and a calcium-binding site but, unlike Cd-substituted concanavalin A, do not have a third metal-binding site. The Co-substituted concanavalin A structure diffracts to the highest resolution of any concanavalin A structure reported to date. A comparison of the structures of Ni-, Co-, Cd-substituted and native concanavalin A gives an indication of coordinate errors, which is a useful baseline for comparisons with saccharide complexes of concanavalin A described in other work. We also give a detailed account of multiple conformations which were found for five side-chain residues.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0907444994002143

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9

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Complex of ribonuclease from Streptomyces aureofaciens with 2'-GMP at 1.7 Å resolution (1993)

Sevcik, J. ; Hill, C. P. ; Dauter, Z. ; [et al.]

Copenhagen : International Union of Crystallography (IUCr)

Acta crystallographica 49 (1993), S. 257-271

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ISSN: 1399-0047

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Chemistry and Pharmacology , Geosciences , Physics

Notes: The crystal structure of a complex of ribonuclease from Streptomyces aureofaciens (RNase Sa) with guanosine-2′-monophosphate (2′-GMP) has been refined against synchrotron data recorded from a single crystal using radiation from beamline X31 at EMBL, Hamburg, and an imaging plate scanner. The crystals are in space group P212121 with cell dimensions a = 64.7, b = 78.8 and c = 39.1 Å. The structure has two enzyme molecules in the asymmetric unit, complexed with 2′-GMP inhibitor with occupancies of 1 and {2 \over 3} (different to the 3′-GMP complex crystal structure where only one of the two independent RNase Sa molecules binds nucleotide), 492 associated water molecules and one sulfate ion, and was refined using all data between 10.0 and 1.7 Å to a final crystallographic R factor of 13.25%. Binding of the base to the enzyme confirms the basis for the guanine specificity but the structural results still do not provide direct evidence of the identity and role of the particular residues involved in the catalytic process. New native RNase Sa data to 1.8 Å were recorded to provide a reference set measured under comparable experimental conditions. The crystals are in the same space group and have the same lattice as those of the 2′-GMP complex. The native structure with 423 water molecules was refined in a similar manner to the complex to a final R factor of 13.87%. 1.77 Å resolution data were independently measured on a 2′-GMP complex crystal at UCLA using an R-AXIS II image plate scanner mounted on a conventional source. The cell dimensions were essentially the same as above. 2′-GMP was bound more fully to molecule A than to molecule B of the RNase Sa. The structure was refined to an R factor of 14.64% with 388 water molecules. This work follows on from the structure determination of native RNase Sa and its complex with 3′-GMP [Sevcik, Dodson & Dodson (1991). Acta Cryst. B47, 240–253].

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0907444992007261

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Refinement of glucose isomerase from Streptomyces albus at 1.65 Å with data from an imaging plate (1990)

Dauter, Z. ; Terry, H. ; Witzel, H. ; [et al.]

Copenhagen : International Union of Crystallography (IUCr)

Acta crystallographica 46 (1990), S. 833-841

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ISSN: 1600-5740

Source: Crystallography Journals Online : IUCR Backfile Archive 1948-2001

Topics: Chemistry and Pharmacology , Geosciences , Physics

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1107/S0108768190008059

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