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Nowakowski, J., Shim, P.J., Joyce, G.F., & Sout, C.D.
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"Crystallization of the
10-23 DNA enzyme using a combinatorial
screen of paired oligonucleotides"
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Acta. Cryst., D55,
1885-1892
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One of the most difficult steps in the X-ray crystallography
of nucleic acids is obtaining crystals that diffract to high
resolution. The choice of the nucleotide sequence has proven
to be more important in producing high quality crystals than
the composition of the crystallization solution. This manuscript
describes a systematic procedure for identifying the optimal
sizes of a multi-stranded nucleic acid complex which provide
high-quality crystals. This approach was used to crystallize
the in vitro evolved 10-23 DNA enzyme complexed with its
RNA substrate. In less than two months, 81 different enzyme-substrate
complexes were generated by combinatorial mixing and annealing
of complementary oligonucleotides which differed in length, resulting
in duplexes of varying length, with ot without nucleotide overhangs.
Each of these complexes was screened against a standard set of
48 crystallization conditions and evaluated for crystal formation.
The screen resulted in over 40 crystal forms, the best of which
diffracted to 2.8 A resolution when exposed to a synchotron X-ray
source.
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