High resolution crystal structure of ferricytochrome c′ from Rhodobacter sphaeroides

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作者
Laura M. Ramirez
Herbert L. Axelrod
Steven R. Herron
Bernhard Rupp
James P. Allen
Katherine A. Kantardjieff
机构
[1] California State University,Department of Chemistry and Biochemistry and W.M. Keck Foundation Center for Molecular Structure
[2] Lawrence Livermore National Laboratory,Macromolecular Crystallography and Structural Genomics
[3] Arizona State University,Department of Chemistry and Biochemistry
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关键词
Cytochrome c′; heme protein; four helix bundle;
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摘要
Cytochrome c′ isolated from Rhodobacter sphaeroides strain R26 (RSCP) crystallizes as a dimer of two identical 14-kDa subunits, in trigonal space group P31, with cell parameters a, b = 48.10 Å, c = 115.80 Å. The crystal structure of RSCP has been solved by molecular replacement using cytochrome c′ from Rhodobacter capsulatus (PDB ID: 1CPQ) as a search model. To ensure effective phase bias removal, the RSCP model was iteratively built into maps generated by a modified wARP procedure, Shake&wARP. The 1.8 Å model (PDB ID: 1GQA) has been refined to an R = 0.204 and freeR = 0.254. Each subunit consists of four antiparallel α-helices, with the pentacoordinate heme covalently bound to a C–X–Y–C–H motif near the C-terminus. F14, located on helix A, blocks direct access to what would be the sixth “distal” ligand binding site of the heme. The dimer subunits form a flattened “X” shape, intermediate between the Type 1 and Type 2 cytochromes c′. The presence of the aromatic F14 and a deep channel between helices B and C places RSCP into Group 1 cytochromes c′. Clear electron density has revealed that the amino acid sequences for the cytochrome c′ from strains R26 and 2.4.1 are identical.
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页码:413 / 424
页数:11
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