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Fluorescence microscopy methods have seen an increase in popularity in recent years for detecting protein crystals in screening trays. The fluorescence-based crystal detection methods have thus far relied on intrinsic UV-inducible tryptophan fluorescence, nonlinear optics or fluorescence in the visible light range dependent on crystals soaked with fluorescent dyes. In this paper data are presented on a novel visible-light-inducible autofluorescence arising from protein crystals as a result of general stabilization of conjugated double-bond systems and increased charge delocalization due to crystal packing. The visible-light-inducible autofluorescence serves as a complementary method to bright-field microscopy in beamline applications where accurate crystal centering about the rotation axis is essential. Owing to temperature-dependent chromophore stabilization, protein crystals exhibit tenfold higher fluorescence intensity at cryogenic temperatures, making the method ideal for experiments where crystals are cooled to 100 K with a cryostream. In addition to the non-damaging excitation wavelength and low laser power required for imaging, the method can also serve a useful role for differentiating protein crystals from salt crystals in screening trays.

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Portable Document Format (PDF) file https://doi.org/10.1107/S160057671502419X/te5008sup1.pdf
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Portable Document Format (PDF) file https://doi.org/10.1107/S160057671502419X/te5008sup2.pdf
Supplementary Fig. 2

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Portable Document Format (PDF) file https://doi.org/10.1107/S160057671502419X/te5008sup3.pdf
Supplementary Fig. 3

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Supplementary Fig. 4

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Macromolecular Crystallographic Information File (mmCIF) https://doi.org/10.1107/S160057671502419X/te5008sup5.mcf
Supplementary material

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Portable Document Format (PDF) file https://doi.org/10.1107/S160057671502419X/te5008sup6.pdf
Supplementary material


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