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Past work has shown that it is feasible to mutate surface residues of soluble proteins and to a lesser extent membrane proteins in order to improve their crystallization behavior. Described here is a successful application of this approach to the integral membrane protein Thermus thermophilus cytochrome ba3 oxidase. Two mutant forms of this enzyme (I-K258R and I-K258R/II-E4Q) were created in which symmetrical crystal contacts within crystals of wild-type enzyme were modified. These mutant proteins had greatly shortened crystallization times, decreasing from ∼30 d for the wild type to 1–3 d for the mutants, and crystallization was highly reproducible. Native-like proteins crystallize in space group P43212, whereas the mutant proteins crystallize in space group P41212 with a different packing arrangement. Crystals of the P43212 form occasionally diffracted to 2.4–2.3 Å resolution following controlled dehydration, while those of the P41212 form routinely diffracted to between 3.0 and 2.6 Å for crystals that had been cryoprotected but not dehydrated.

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Portable Document Format (PDF) file https://doi.org/10.1107/S1744309107054176/bw5212sup1.pdf
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