Mix-and-diffuse serial synchrotron crystallography

Author:

Beyerlein Kenneth R.ORCID,Dierksmeyer Dennis,Mariani ValerioORCID,Kuhn Manuela,Sarrou Iosifina,Ottaviano AngelicaORCID,Awel Salah,Knoska JurajORCID,Fuglerud SiljeORCID,Jönsson OlofORCID,Stern Stephan,Wiedorn Max O.ORCID,Yefanov OleksandrORCID,Adriano Luigi,Bean RichardORCID,Burkhardt Anja,Fischer Pontus,Heymann MichaelORCID,Horke Daniel A.ORCID,Jungnickel Katharina E. J.ORCID,Kovaleva ElenaORCID,Lorbeer Olga,Metz MarkusORCID,Meyer Jan,Morgan AndrewORCID,Pande KanupriyaORCID,Panneerselvam SaravananORCID,Seuring CarolinORCID,Tolstikova Aleksandra,Lieske JuliaORCID,Aplin Steve,Roessle Manfred,White Thomas A.,Chapman Henry N.ORCID,Meents AlkeORCID,Oberthuer DominikORCID

Abstract

Unravelling the interaction of biological macromolecules with ligands and substrates at high spatial and temporal resolution remains a major challenge in structural biology. The development of serial crystallography methods at X-ray free-electron lasers and subsequently at synchrotron light sources allows new approaches to tackle this challenge. Here, a new polyimide tape drive designed for mix-and-diffuse serial crystallography experiments is reported. The structure of lysozyme bound by the competitive inhibitor chitotriose was determined using this device in combination with microfluidic mixers. The electron densities obtained from mixing times of 2 and 50 s show clear binding of chitotriose to the enzyme at a high level of detail. The success of this approach shows the potential for high-throughput drug screening and even structural enzymology on short timescales at bright synchrotron light sources.

Funder

European Research Council

Deutsche Forschungsgemeinschaft

Helmholtz-Gemeinschaft

Publisher

International Union of Crystallography (IUCr)

Subject

Condensed Matter Physics,General Materials Science,Biochemistry,General Chemistry

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