Observation of substrate diffusion and ligand binding in enzyme crystals using high-repetition-rate mix-and-inject serial crystallography

Pandey, S.; Calvey, G.; Katz, A.M.; Malla, T.N.; Koua, F.H.M.; Martin-Garcia, J.M.; Poudyal, I.; Yang, J.-H.; Vakili, M.; Yefanov, O.; Zielinski, K.A.; Bajt, S.; Awel, S.; Doerner, K.; Frank, M.; Gelisio, L.; Jernigan, R.; Kirkwood, H.; Kloos, M.; Koliyadu, J.; Mariani, V.; Miller, M.D.; Mills, G.; Nelson, G.; Olmos Jr., J.L.; Sadri, A.; Sato, T.; Tolstikova, A.; Xu, W.; Ourmazd, A.; Spence, J.H.C.; Schwander, P.; Barty, A.; Chapman, H.N.; Fromme, P.; Mancuso, A.P.; Phillips Jr, G.N.; Bean, R.; Pollack, L.; Schmidt, M.

doi:10.1107/S2052252521008125

research papers

IUCrJ

Volume 8| Part 6| November 2021| Pages 878-895

ISSN: 2052-2525

https://doi.org/10.1107/S2052252521008125

BIOLOGY | MEDICINE

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Observation of substrate diffusion and ligand binding in enzyme crystals using high-repetition-rate mix-and-inject serial crystallography

^aPhysics Department, University of Wisconsin-Milwaukee, 3135 North Maryland Avenue, Milwaukee, WI 53211, USA, ^bSchool of Applied and Engineering Physics, Cornell University, 254 Clark Hall, Ithaca, NY 14853, USA, ^cCenter for Free-Electron Laser Science, Deutsches Elektronen-Synchrotron DESY, Notkestrasse 85, 22607 Hamburg, Germany, ^dSchool of Molecular Sciences and Biodesign Center for Applied Structural Discovery, Arizona State University, Tempe, AZ 85287-1604, USA, ^eInstitute of Physical Chemistry Rocasolano, Spanish National Research Council, Calle de Serrano 119, 28006 Madrid, Spain, ^fEuropean XFEL, Holzkoppel 4, 22869 Schenefeld, Germany, ^gDeutsches Elektronen-Synchrotron DESY, Notkestrasse 85, 22607 Hamburg, Germany, ^hThe Hamburg Centre for Ultrafast Imaging, Luruper Chaussee 149, 22761 Hamburg, Germany, ⁱLawrence Livermore National Laboratory, 7000 East Avenue, Livermore, CA 94550, USA, ^jSLAC National Accelerator Laboratory, 2575 Sand Hill Rd, Menlo Park, California 94025, USA, ^kDepartment of BioSciences, Rice University, 6100 Main Street, Houston, TX 77005, USA, ^lDepartment of Physics, Arizona State University, Tempe, AZ 85287, USA, ^mDepartment of Bioengineering and Therapeutic Sciences, University of California San Francisco, San Francisco, CA 94158, USA, ⁿDepartment of Physics, Universität Hamburg, Luruper Chaussee 149, 22761 Hamburg, Germany, ^oDepartment of Chemistry and Physics, La Trobe Institute for Molecular Science, La Trobe University, Melbourne, Victoria 3086, Australia, and ^pDepartment of Chemistry, Rice University, 6100 Main Street, Houston, TX 77005, USA
^*Correspondence e-mail: m-schmidt@uwm.edu

Edited by K. Moffat, University of Chicago, USA (Received 21 June 2021; accepted 6 August 2021; online 9 September 2021)

In memoriam of John Spence.

Here, we illustrate what happens inside the catalytic cleft of an enzyme when substrate or ligand binds on single-millisecond timescales. The initial phase of the enzymatic cycle is observed with near-atomic resolution using the most advanced X-ray source currently available: the European XFEL (EuXFEL). The high repetition rate of the EuXFEL combined with our mix-and-inject technology enables the initial phase of ceftriaxone binding to the Mycobacterium tuberculosis β-lactamase to be followed using time-resolved crystallography in real time. It is shown how a diffusion coefficient in enzyme crystals can be derived directly from the X-ray data, enabling the determination of ligand and enzyme–ligand concentrations at any position in the crystal volume as a function of time. In addition, the structure of the irreversible inhibitor sulbactam bound to the enzyme at a 66 ms time delay after mixing is described. This demonstrates that the EuXFEL can be used as an important tool for biomedically relevant research.

Keywords: substrate diffusion in crystals; antibiotic resistance; β-lactamases; enzyme kinetics; irreversible inhibition; mix-and-inject serial crystallography; serial femtosecond crystallography; European X-ray Free-Electron Laser; megahertz pulse-repetition rate; protein structure determination; drug discovery; ceftriaxone; sulbactam; X-ray crystallography; enzyme mechanisms.

PDB references: BlaC, unmixed, 7k8l; mixed with ceftriaxone, 5 ms, 7k8e; 10 ms, 7k8f; 50 ms, 7k8h; mixed with sulbactam, 66 ms, 7k8k

1. Introduction

Combatting the rise of infectious diseases requires a collaborative and interdisciplinary approach. Structural biologists can contribute by investigating the reaction mechanisms of biomedically significant enzymes as a structural basis to develop cures for diseases. Bacterial infections with strains that are resistant to currently available antibiotics are on the rise (Cassini et al., 2019 ). A study sponsored by the British government projected that in the near future more people will die from untreatable bacterial infections than from cancer (https://amr-review.org/). Bacterial enzymes that inactivate currently available drugs are central to antibiotic resistance (Fair & Tor, 2014 ), and unraveling the catalytic mechanism of these enzymes will be beneficial for the development of novel antibiotics (Imming et al., 2006 ). β-Lactamases such as the Mycobacterium tuberculosis β-lactamase [BlaC; Fig. 1(a)] catalytically inactivate β-lactam antibiotics. β-Lactamases are responsible for the emergence of multidrug- and extensively drug-resistant bacterial strains (Smith et al., 2013 ). Infectious diseases that could be treated with antibiotics in the past may become untreatable. This warrants the investigation of the structure and function of these enzymes.

Figure 1
The structures of BlaC and the ligands investigated here. (a) Structure of BlaC in the orthorhombic crystal form. The four subunits of BlaC are shown in red (A), green (B), blue (C) and yellow (D). The red dotted box shows the position of the active site. A phosphate (P_i) is present in all active sites. The catalytically active Ser70 is marked in subunits B and D. (b) The chemical structure of ceftriaxone (CEF). The leaving group (dioxotriazine; the double tilde shows the cleaved bond) and the thiazole ring are marked. (c) The chemical structure of sulbactam (SUB). (d) The covalently bound trans-EN. Ser70 of BlaC opens the β-lactam ring of SUB. The structure rearranges to a trans-enamine. This inactivates BlaC.

Using time-resolved crystallography, structures of intermediates and kinetic mechanisms can be extracted simultaneously from the same set of X-ray data (Moffat, 2001 ; Schmidt, 2008 ). At free-electron lasers (XFELs) small, micrometre- and submicrometre-sized, crystals can be examined due to the immense X-ray pulse intensity (Chapman et al., 2011 ). The microcrystals are destroyed by the pulses, and new crystals must be delivered to the X-ray interaction point in a serial fashion. This method has been termed serial femtosecond crystallography (SFX; Chapman et al., 2011; Boutet et al., 2012 ). Since the XFEL pulses are of femtosecond duration, diffraction patterns are collected before the crystals suffer significant radiation damage, resulting in X-ray structures that are essentially damage-free (Lomb et al., 2011 ; Nass, 2019 ; Neutze et al., 2000 ) and are suspended in their current reaction state. Most time-resolved crystallographic experiments at XFELs are of the pump–probe type. An optical laser pulse triggers a reaction in the crystallized molecules. Structures are probed by X-ray pulses after a controlled delay (Tenboer et al., 2014 ; Barends et al., 2015 ; Coquelle et al., 2018 ; Nogly et al., 2018 ; Kern et al., 2018 ; Pandey et al., 2019 ; Skopintsev et al., 2020 ; Dods et al., 2021 ; Yun et al., 2021 ). Due to the ultrashort nature of both X-ray and optical laser pulses, the experiments can reach subpicosecond time resolutions (Hartmann et al., 2014 ; Barends et al., 2015; Pande et al., 2016 ; Skopintsev et al., 2020). Photoactivation requires a light-sensitive cofactor, a chromophore, located in the protein to absorb the light. Light absorption must trigger a reaction that either promotes catalysis directly (Holtorf et al., 1995 ; Li et al., 2010 ; Sorigué et al., 2017 , 2021 ) or regulates the activity of the enzyme (Takala et al., 2014 ; Gourinchas et al., 2017 ; Carrillo et al., 2021 ). Most enzymes, however, are neither activated nor regulated by light, meaning that the technique can only be directly applied in a narrow range of cases. Broader application requires great effort and chemical expertise to either engineer photoactive enzymes or to design photoactive compounds that can by soaked into, and activated in, enzyme crystals (Šrajer & Schmidt, 2017 ; Zaitsev-Doyle et al., 2019 ; Mehrabi, Schulz, Dsouza et al., 2019 ).

With the `mix-and-inject' technique (Schmidt, 2013 ; Stagno et al., 2017 ; Kupitz et al., 2017 ; Olmos et al., 2018 ; Mehrabi, Schulz, Agthe et al., 2019 ) photoactivation is not necessary. The substrate is rapidly mixed with small enzyme crystals during sample delivery (Calvey et al., 2019 ). Mixing occurs at a well controlled location `en route' to the X-ray beam. During the time delay Δt_m that occurs between mixing and injection, the substrate diffuses into the crystals and binds to the enzyme. The complex formed by the substrate and the enzyme then initiates the enzymatic cycle. Variation of Δt_m allows the measurement of rate coefficients together with atomic resolution structures which can be associated with intermediate states of the protein reactions (Kupitz et al., 2017; Olmos et al., 2018; Mehrabi, Schulz, Agthe et al., 2019). This can reveal the mechanism of enzyme action at the molecular level or the binding of a drug molecule. The combination of serial femtosecond crystallography with mixing before injection has been denoted `mix-and-inject serial crystallography' (MISC; Kupitz et al., 2017; Olmos et al., 2018). The feasibility of MISC has previously been demonstrated with BlaC on longer millisecond timescales (Kupitz et al., 2017; Olmos et al., 2018). The observation of intermediate-state structures, and the maximization of the potential time resolution in both photoactivation and mix-and-inject techniques, relies on an accurately gauged start time of the reaction inside the crystals. In photoactivation experiments this requires a sufficient penetration of optical laser light into the crystal to ensure that a reaction is simultaneously triggered in a significant fraction of the molecules. In mix-and-inject experiments, the diffusion time of the substrate into the crystal may limit the ability to discriminate diffusion and kinetics, including substrate binding. To overcome this limitation, micrometre or submicrometre crystal sizes are required that ensure that the substrate diffuses rapidly into the crystals and the reaction is triggered swiftly and much faster than the lifetime of the reaction intermediates of interest (Schmidt, 2013).

The reaction of the cephalosporin antibiotic ceftriaxone [CEF; Fig. 1(b)] with BlaC is an excellent candidate for exploration with MISC. Previously, this reaction was investigated for Δt_m of longer than 30 ms (Kupitz et al., 2017; Olmos et al., 2018). At 30 ms, however, the CEF binding sites in BlaC were essentially fully occupied (Olmos et al., 2018), a state also reached on similar timescales for other proteins and enzymes (Stagno et al., 2017; Mehrabi, Schulz, Agthe et al., 2019; Ishigami et al., 2019 ). The substrate-binding phase and the formation of the enzyme–substrate complex, however, remain elusive. Here, we aim to characterize the early phase of substrate binding with single-millisecond time delays by using the megahertz X-ray pulse-repetition rate of the European XFEL (EuXFEL; Decking et al., 2020 ).

In addition, we aim to investigate the reaction of BlaC with an inhibitor, sulbactam [SUB; Fig. 1(c)], on a millisecond timescale. The biochemistry of SUB and its application in combination with β-lactam antibiotics have been described in detail elsewhere (Totir et al., 2007 ). SUB binds to the active site of BlaC and reacts with the catalytically active serine of β-lactamases to form a covalently bound species. Most abundant is the so-called trans-enamine (trans-EN) species [Fig. 1(d)] that inhibits β-lactamases and helps to eliminate β-lactamase-induced antibiotic resistance. Static structures of trans-ENs with β-lactamases, including BlaC, have recently been characterized (Cheng et al., 2020 ; Tassoni et al., 2019 ), but structures of the early species that form during SUB binding remain elusive.

2. Methods

2.1. BlaC crystals

Platelet-shaped crystals of BlaC with approximate dimensions of 10 × 10 × 2 µm (Appendix A) were produced by a stirring method on site in the XBI facility of the EuXFEL (Han et al., 2021 ) using ammonium phosphate (AP) as described by Olmos et al. (2018). The crystals belonged to space group P2₁ (Table 1), with four BlaC subunits in the asymmetric unit [Fig. 1(a)] (Olmos et al., 2018). Only two subunits bind CEF in their catalytic cleft, as demonstrated previously (Olmos et al., 2018). The concentration of BlaC subunits in the crystals is 15.5 mM, so that the concentration of active subunits is 7.8 mM. When this concentration is matched by substrate, the substrate concentration is called `stoichiometric' in the following description.

Table 1
Data-collection statistics [30 ms data from Olmos et al. (2018)]

	Water (reference)	5 ms CEF	10 ms CEF	50 ms CEF	66 ms SUB	30 ms CEF (LCLS)
Temperature (K)	293	293	293	293	293	293
Space group	P2₁	P2₁	P2₁	P2₁	P2₁	P2₁
EuXFEL train pulse rate (kHz)	564	564	564	564	564	564
a, b, c (Å)	80.9, 99.5, 112.6	80.6, 98.7, 113.1	80.6, 98.5, 113.5	80.4, 98.2, 115.2	81.0, 99.5, 112.6	78.7, 96.8, 112.6
α, β, γ (°)	90, 108.4, 90	90, 108.6, 90	90, 108.8, 90	90, 110.0, 90	90, 108.4, 90	90, 109.7, 90
Resolution (Å)	2.8	2.4	2.6	2.6	2.7	2.7
Hits	51980	110698	85775	85914	35886	35065
Indexed patterns	31812	105495	52323	36256	25013	24397
Hit/indexing rate (%)	2.98/61.2	0.65/95.3	1.33/61.0	2.26/42.2	0.78/69.7	3.87/69.5
Observed reflections	31572191	114717921	49576617	38055135	21034155	14588166
Unique reflections	41870	65232	51595	50760	45344	40340
Multiplicity	754 (236)	1758 (1246)	966.3 (580.4)	749.7 (449.4)	463.8 (307.4)	526 (142)
Completeness (%)	100 (100)	100 (100)	100 (100)	100 (100)	100 (100)	100 (100)
R_split (%)	20.6 (988)	15.6 (303.7)	17.8 (334)	20.9 (198.1)	21.4 (459.2)	14.2 (121.1)
CC_1/2 (%)	96.5 (22.9)	99.2 (26.9)	99.6 (58.4)	99.5 (58.4)	96.9 (20.5)	98.6 (34.5)

2.2. Data collection at the EuXFEL

The platelets were mixed with ceftriaxone [CEF; Fig. 1(b); molecular mass 554.6 g mol⁻¹; 200 mM in 0.8 M AP] or sulbactam (SUB) inhibitor [Fig. 1(c), molecular mass 223.2 g mol⁻¹, 100 mM in 0.8 M AP] using optimized mixing injectors (Calvey et al., 2019) which were adapted to operate at the SPB/SFX instrument (Mancuso, 2019 ) of the EuXFEL. Flow rates and mixer geometries are shown in Table 2. The mixture was intercepted after a delay Δt_m by X-ray pulses from the EuXFEL. The EuXFEL delivers X-ray pulses in pulse trains that repeat ten times per second (Fig. 2). Each train contained 202 X-ray pulses with approximately 40 fs full-width at half-maximum (FWHM) pulse duration and about 1.5 mJ pulse energy. The pulse-repetition rate within a pulse train was 564 kHz, a reduction from the possible 4.5 MHz to avoid pristine, upstream jet volumes being affected by previous X-ray pulses (Yefanov et al., 2019 ; Pandey et al., 2020 ; Grünbein et al., 2021 ). Given a flow rate of about 80 µl min⁻¹ (Table 2) and an assumed jet diameter of 8 µm, the jet advances 26.5 m in a second. With a 564 kHz pulse rate the jet is intercepted every 47 µm, which is much larger than the gap (∼20 µm; Wiedorn, Oberthür et al., 2018 ) in the jet produced by the intense X-ray pulse. The X-ray beam size at the jet position was ∼3 µm. The design of the mixers allowed us to recapture the record (Mehrabi, Schulz, Agthe et al., 2019) for the shortest MISC time point, while maintaining the high jet speed necessary for the 564 kHz measurements (Wiedorn, Oberthür et al., 2018). Reference data were obtained by mixing with water.

Table 2
Parameters for the mix-and-inject experiments

Concentrations of ceftriaxone (CEF) and sulbactam (SUB) are shown as were flowed through the outer capillary line of the mixing injectors. Time delays are achieved after mixing in a constriction as per Calvey et al. (2019).

	Water	SUB	CEF	CEF	CEF
Δt_m (ms)	(10)	66	5	10	50
Ligand concentration (mM)	—	100	200	200	200
Ligand buffer	—	0.8 M AP pH 4.6	0.8 M AP pH 4.6	0.8 M AP pH 4.6	0.8 M AP pH 4.6
Ligand flow (µl min⁻¹)	74.5	54.5	76.7	74.5	71.8
Crystal flow (µl min⁻¹)	5.5	11.6	3.3	5.5	8.2
Mixing injector capillary internal diameter (µm)	50	75	50	50	75
Constriction length (mm)	17.8	36.1	9.3	17.8	36.1
Timing uncertainty (ms)	—	9.3	1.8	3.0	10.4
Experimental time to collect the data set (min)	50	56	138	250	32

Figure 2
Experimental setup at the European XFEL. BlaC microcrystals are mixed with substrate and injected into the X-ray interaction region (dotted circle) after a delay determined by the distance between the mixing region and the X-rays, the capillary width and the flow rate. Diffusion of substrate into the crystals occurs during this time. The mixture is probed by trains of X-ray pulses. The trains repeat ten times per second. Pulses within the trains repeat at 564 kHz, hence the pulses are spaced by 1.78 µs. 202 pulses were in each train for this experiment. The AGIPD collects the diffraction patterns and reads them out for further analysis. Inset: data collection. With a selected injector geometry and flow rate, the delay is fixed by the distance of the mixing region from the X-ray interaction region. All pulses in all trains (here pulse 3) probe the same time delay. The EuXFEL pulse structure is most efficiently used.

Diffraction patterns (DPs) were collected using the Adaptive Gain Integrating Pixel Detector (AGIPD; Allahgholi et al., 2019 ) operating at a 565 kHz frame rate. The experiment was monitored using OnDA (Mariani et al., 2016 ), which is designed to estimate hit rates and spatial resolution in real time. DPs with Bragg reflections were selected by Cheetah (Barty et al., 2014 ) and indexed, integrated, scaled and merged by CrystFEL (White et al., 2016 ) in a manner consistent with previous work (Pandey et al., 2020). In brief, diffraction images with Bragg reflections were found by Cheetah (peakfinder8, minSNR=8, minADC=200, minPix=1, minPeaks=25) using the calibration process described by Wiedorn, Awel et al. (2018 ). Careful masking of shadowed and unreliable regions of the detector was performed on a run-by-run basis (Appendix B). Independent masks were used for peak finding to avoid false hits, for example due to ice formation. Indexing was performed with CrystFEL (version 0.9.0) using the indexing package XGANDALF (Gevorkov et al., 2019 ) with the following parameters: peaks=peakfinder8, Min-SNR=5, Min-pixel-count=1, Threshold=400. The detector geometry was refined using geoptimiser (Yefanov et al., 2015 ). Merging and scaling of the Bragg peak intensities were performed using the partialator program from CrystFEL. To avoid the integration of noise for weakly scattering patterns, reflections were included up to 1.0 nm⁻¹ above a conservative resolution estimate for each crystal (--push-res=1.0). Hit rates and indexing rates were stable in the order of 1.0% and 70%, respectively, irrespective of the pulse index in the train (Appendix A). The lower hit rate is a consequence of diluting the crystalline slurry with the ligand/substrate. It has been shown that the X-ray pulse position in the train has no effect on the structure (Yefanov et al., 2019). Structure-factor amplitudes were generated from the measured intensities using programs from the CCP4 software suite (Winn et al., 2011 ). Data-collection statistics are shown in Table 1.

As a control, and to investigate the result of the complete reaction of BlaC with SUB in the platelet crystal form, macroscopic crystals were grown in sitting drops (10 µl BlaC at 45 mg ml⁻¹ mixed in a 1:1 ratio with 2.1 M AP pH 4.1). Crystals grew within three days. The crystals were soaked for 3 h in a cryobuffer consisting of 2 M AP, 20% glycerol and 100 mM SUB. The crystals were cooled in liquid nitrogen. Data were collected on beamline ID-19 of the Structural Biology Center, Advanced Photon Source, Argonne National Laboratory. Data were processed to 2.7 Å using HKL-3000 (Minor et al., 2006 ). Details will be presented elsewhere.

2.3. Difference-map calculation and structure determination

The structures of BlaC and the BlaC–CEF complexes were determined as described previously (Kupitz et al., 2017; Olmos et al., 2018). Since the unit-cell constants change substantially after mixing (Table 1), isomorphous difference maps cannot be calculated and OMIT difference maps (DED_omit) were used. An initial BlaC model, PDB (Berman et al., 2002 ) entry 6b5x (Olmos et al., 2018), was refined against the structure-factor amplitudes |F_o(t)|_CEF collected at a particular Δt_m. The content of the active sites (water and phosphate) was removed during the refinement. From the refined model amplitudes, |F_c| were determined. From the amplitudes (and the phases obtained from the refined model), weighted m|F_o(t)|_CEF − D|F_c| OMIT maps (DED_omit) were calculated. Polder difference maps (Liebschner et al., 2017 ; DED_Polder) were calculated to display weak difference electron-density features. The CEF was modeled in the polder maps. To refine the structure and to determine the fractional concentration of both P_i and CEF, grouped occupancy refinement was performed using Phenix (Liebschner et al., 2019). CEF was flagged together with P_i as a pair of molecules occupying the same space. The positions and B factors of all atoms as well as the occupancies of P_i and CEF were refined simultaneously. As a check, the sum of the occupancies of the flagged molecules should not deviate too much from unity.

Initial structures of the BlaC–SUB complexes were determined by inspecting both isomorphous and OMIT difference maps. The OMIT map was calculated in a similar way as described above except that amplitudes |F_o(t)|_SUB were used. A weighted DED_iso map was calculated from difference amplitudes w[|F_o(t)|_SUB − |F_o|_WAT], where the reference amplitudes |F_o|_WAT were obtained by mixing with water. The weighting factor was calculated as described previously for photoactive yellow protein (Ren et al., 2001 ; Pandey et al., 2020) and for the needle crystal form of BlaC (Olmos et al., 2018). The trans-EN and SUB molecules were inserted into the OMIT map. The positions and orientations were cross-examined to agree with the DED_iso map. The complexes were refined using REFMAC (Murshudov et al., 2011 ) against the |F_o(t)|_SUB amplitudes. The refinement statistics for the BlaC–CEF and BlaC–SUB complexes are shown in Table 3.

Table 3
Refinement statistics

	Water	5 ms CEF	10 ms CEF	50 ms CEF	66 ms SUB	30 ms CEF (Olmos et al., 2018, revisited)
Refinement program	Phenix	Phenix	Phenix	Phenix	REFMAC	Phenix
Resolution	2.8	2.4	2.6	2.6	2.7	2.75
Reflections used	36804	52163	43274	45264	36434	40951
R_cryst/R_free	0.21/0.27	0.24/0.25	0.22/0.26	0.22/0.27	0.21/0.29	0.22/0.26
Occupancy (CEF/phosphate) (%)	—	B, 46/60; D, 43/53	B, 61/35; D, 64/38	B, 84/11; D, 79/27	100, not refined	B, 76/20; D, 74/21
〈B〉_CEF (B/D) (Å²)	—	51/48	55/58	53/50	—	70/67
R.m.s.d., bond lengths (Å²)	0.009	0.003	0.003	0.003	0.007	0.003
R.m.s.d., bond angles (°)	1.09	1.07	1.03	1.34	1.67	1.10
H₂O	129	246	251	247	201	146

2.4. Binding kinetics of CEF

Refined occupancies are fitted by functions that account for saturation of CEF and decline of P_i,

$[C_{\rm CEF}(t) = {{C_{\rm S,CEF} \cdot t} \over {t_{1/2} + t}}, \eqno(1)]$

and

$[C_{\rm P_{i}}(t) = {{C_{\rm ini,P_{i}} \cdot t_{1/2}} \over {t_{1/2} + t}}, \eqno(2)]$

respectively. $[C_{\rm S,CEF}]$ and $[C_{\rm ini,P_{i}]$ are the occupancy of CEF after a long time (at saturation) and the initial occupancy of P_i, respectively. The constant t_1/2 is either the time taken to reach half saturation of CEF or denotes the time when P_i has declined to half its initial concentration. The initial occupancy of P_i was set as 1.0, but the final occupancy of CEF was not constrained to 1.0 to account for a more realistic scenario.

2.5. The diffusion coefficient of CEF in the BlaC platelets

The occupancy of CEF bound noncovalently to the active center of BlaC was calculated with typical sized 10 × 10 × 2 µm (platelet-like) crystals (Appendix A) by varying the diffusion coefficient D for the CEF in crystals until agreement with the experiment was achieved. The crystal was divided into 20 voxels along each direction and 20 time intervals were used. For each time interval, the concentration of the CEF substrate (C_CEF) in each of the 8000 voxels in the crystal was determined using the known solution to Fick's second law for a rectangular volume, represented by the first 20 modes (Schmidt, 2013, 2020 ; Carslaw & Jaeger, 1959 ),

$[\eqalignno{C_{\rm CEF}&(x,y,z,t) = \cr & C_{\rm 0,CEF} \biggr (1 - {{64} \over {\pi^3}} {\textstyle\sum\limits_{l=0}^{19} \sum\limits_{m=0}^{19} \sum\limits_{n=0}^{19}} {{(-1)^{l+m+n}} \over {(2l+1)(2m+1)(2n+1)}} \cr & \times \cos {{(2l+1)\pi x} \over {2a}}\cos {{(2m+1)\pi y} \over {2b}}\cos {{(2n+1)\pi z} \over {2c}} \cr & \times \exp \left \{-{{D\pi^2} \over 4}\left [{{(2l+1)^2} \over {a^2}} + {{(2m+1)^2} \over {b^2}} + {{(2n+1)^2} \over {c^2}} \right]t\right\}\biggr),\cr &&(3)}]$

where l, m, n are integer numbers that define the modes. x, y and z are coordinates within the crystal that extend from −a to +a, −b to +b and −c to c, where a, b, c are the half edge lengths of the platelet-shaped BlaC crystals. D is the diffusion coefficient, t is the time after mixing and C_0,CEF is the outside CEF concentration, which was set to 150 mM. This analytical approach to diffusion is strictly speaking only valid in the absence of substrate binding. However, here the substrate concentration (∼150 mM) is much higher than the concentration of the subunits that bind the CEF (7.8 mM). The concentration of substrate in the crystals increases rapidly to values much higher than the stoichiometric concentration. At saturation, the ES concentration is only 5.2% of that of the substrate. In addition, the speed (rate) of substrate binding is low until sufficient substrate is present. Accordingly, substrate binding is a small perturbation of the free CEF concentration on all but the very shortest timescales.

On the timescales employed here, the formation of later intermediates and the catalytic turnover of BlaC with CEF do not play a role (Boyd & Lunn, 1979 ; Hugonnet & Blanchard, 2007 ; Tremblay et al., 2010 ; Olmos et al., 2018). Both processes unfold over much longer timescales (Fig. 3) than the time delays examined here.

Figure 3
Simplified enzymatic cycle of, and the timescales associated with, the reaction of BlaC with CEF. CEF is delivered to the crystals by diffusion. It noncovalently binds to the free BlaC enzyme (E) to form the enzyme–substrate complex (ES). The acyl intermediate EP, which is covalently bound to Ser70, is formed within ∼200 ms. The leaving group R₂ is cleaved off the CEF. The modified CEF (EP) is hydrolyzed and released as product (P) and the free enzyme is recovered within about 2 s. In this paper, only the formation of the ES complex up to 50 ms (gray, blurred vertical line) was explored.

CEF binding to the active sites of BlaC is dependent on the free BlaC concentration in the crystal and the rate coefficients that describe the binding kinetics (Fig. 3). Here, the rate coefficient k_on of 3.2 M⁻¹ s⁻¹ as estimated by Olmos and coworkers was used. The k_off rate coefficient (dashed arrow in Fig. 3) was assumed to be negligible relative to the on-rate coefficient. There is only one free parameter, the diffusion coefficient D, which can be inferred by matching calculated occupancies to the refined occupancies observed at Δt_m. (3) provides substrate (CEF) concentrations in each individual voxel (at each position in the crystal) at any particular time t. CEF binding to BlaC was calculated for each voxel by numerically integrating the rate equation with time intervals dt,

$[\eqalignno{ {\rm d}[{\rm ES}] &= [{\rm E}(t_i)]_{\rm free} \cdot [C_{\rm CEF}(t_i)] \cdot k_{\rm on} \,{\rm d}t, \cr [{\rm ES}(t_{i+1})] & = [{\rm ES}(t_i)] + {\rm d}[{\rm ES}], \cr [{\rm E}(t_{i+1})]_{\rm free} & = [{\rm E}(t_i)]_{\rm free} - {\rm d}[{\rm ES}], \cr t_{i+1} & = t_i + {\rm d}t.&(4)}]$

In (4), d[ES] is the change in concentration of the BlaC–CEF complex ([ES]) given the free enzyme ([E]) and free CEF ([C_CEF]) concentrations at time t_i and the k_on rate. The free-enzyme concentration [E] decreases and that of the BlaC–CEF complex increases with each time step. (4) is repeated by increasing t_i by dt until t_i is larger than a given delay time, for example 10 ms. The substrate [C_CEF] is provided everywhere by diffusion (3) and its concentration is also dependent on t_i. The goal was to reproduce the approximate 50% BlaC–CEF occupancy in the B and D subunits (occ_obs) which was observed in the experiment at around 5 ms. The calculated BlaC–CEF occupancy (occ_calc) is the average of the calculated occupancies found in all voxels of the crystal. Occ_calc can then be compared with occ_obs and adjusted by varying the diffusion coefficient of CEF.

3. Results and discussion

3.1. Formation of the enzyme–substrate complex

The EuXFEL 564 kHz pulse structure was used to measure the binding of the large CEF substrate to BlaC at a Δt_m of 5, 10 and 50 ms. The Δt_m of 5 ms is about an order of magnitude faster than the earliest (30 ms) time point collected previously (Olmos et al., 2018). The ∼2 µm thin, platelet-shaped BlaC microcrystals allow fast diffusion times across the thin dimension. Furthermore, diffusion is facilitated by large channels in the crystals (Olmos et al., 2018). Therefore, these crystals are ideally suited for mix-and-inject investigations on fast timescales.

As observed in the previous studies at longer Δt_m, CEF only binds to BlaC subunits B and D. In Figs. 4(b)–4(d) polder difference electron-density maps (Liebschner et al., 2017; DED_Polder) are shown in the active site of subunit B. On early timescales (5 and 10 ms after mixing) we simultaneously observe electron densities for CEF and the close-by phosphate (P_i) molecule. Since CEF and P_i occupy the same space, their presence is mutually exclusive and the electron density reflects an average over sites occupied by P_i and others occupied by CEF. P_i is also found near the CEF binding site in the unliganded (unmixed) form [Fig. 4(a)]. At Δt_m = 5 ms, the P_i and CEF occupancies are both approximately 50%. The available catalytic sites in subunits B and D are equally occupied either by a CEF or by a P_i. At Δt_m = 50 ms, the P_i density vanishes. Nevertheless, the P_i occupancy refines to 19% and that of CEF to 82% (Table 3). Here, an electron-rich compound (P_i) is refined in conjunction with CEF, occupying equivalent spaces in different unit cells. This may result in an overestimate of the occupancy of P_i. As there is no indication of phosphate-shaped electron density at 50 ms [Fig. 4(d)], we consider this to be the error margin of our occupancy refinement.

Figure 4
Polder difference electron density, contour level 3σ, in the active center of BlaC subunit B. (a) The CEF ligand has not yet diffused in; the phosphate (P_i) from the crystallization buffer is dominant in the active site. (b) 5 ms after mixing: the phosphate is beginning to be displaced by CEF. (c) 10 ms after mixing: the phosphate is no longer dominant. (d) 50 ms after mixing: little evidence of the phosphate remains and the density only has features of the antibiotic compound. Nearby amino acids are marked in (a).

In agreement with previous work (Olmos et al., 2018), an additional CEF molecule is identified close to each active site that weakly interacts (stacks) with the CEF already bound there (Fig. 5). The stacking sites seem to be only transiently visited by CEF molecules until the active sites are fully occupied. The unit-cell parameter changes roughly follow CEF binding and P_i release [Fig. 6(a), inset; Table 1]. When sulbactam, which is about 2.5 times smaller, binds the P_i is not replaced and the unit-cell parameters do not change (see below and Table 1). We postulate that the displacement of the strongly negatively charged P_i, as well as the occupancy of the stacking site, may contribute to the unit-cell changes observed when CEF is mixed in. The needle crystal form described earlier (Olmos et al., 2018) does not show unit-cell changes. There, neither the P_i nor the stacking site is present. In our BlaC platelets the CEF occupancy can be very heterogenous, in particular at 5 ms, which should result in different unit-cell parameters near the surface and in the center, respectively. However, the Bragg reflections are not split, which is in accordance with observations by others (Ramakrishnan et al., 2021 ; Stagno et al., 2017; Kupitz et al., 2014 ). This may be a consequence of the fully coherent illumination of the entire microcrystal volume by the XFEL radiation or may be due to the plasticity of microcrystals that even supports phase transitions and space-group changes (Ramakrishnan et al., 2021).

Figure 5
Additional ligands. (a) CEF in the active site and the stacking site (dotted oval) located between subunits D and C. A DF_o − mF_c OMIT difference electron-density map in the active site is shown in green and that in the stacking site in gray–green (at a 2.5σ contour level). Substantial CEF density in the active site is shown in green. There is also electron density for P_i present due to averaging over all unit cells in the crystal. The stacking site is not occupied (gray CEF_s molecule). (b) At 50 ms the maximum occupancy of CEF in the active center is reached. The stacking site is substantially occupied (blue CEF molecule). Important residues and distances are marked in Å. (c) The covalently bound trans-EN is present in subunit A of the static cryostructure of BlaC when soaked with SUB (blue; 2F_o − F_c map at a 1.5σ contour level).

Figure 6
BlaC–CEF complex formation as a function of time. (a) Occupancies of CEF in the active site of BlaC at 5, 10, 30 and 50 ms in subunits B (spheres) and D (squares) as well as those of P_i (green triangles and blue diamonds) are plotted as a function of delay (the 30 ms data are from Olmos et al., 2018

). The data are fitted with saturation curves [equations (1

) and (2

), black and blue dashed lines]. The two curves intersect at around 6 ms. Inset: the corresponding change in the unit-cell axis c. (b) Concentrations (in %) as calculated from diffusion and binding [equations (1)–(5)]; green dashed line and green triangles, increase of the calculated BlaC–CEF complex concentration averaged over all voxels in the crystal; red dashed line and squares, decrease of the free enzyme (BlaC); blue dashed line and diamonds, increase of the BlaC–CEF complex in the center of the platelet-shaped crystals. For comparison, the observed (refined) occupancies of the BlaC–CEF complex (normalized to 100% at 50 ms) are also shown (black spheres).

As more CEF binds, Ser70 moves towards the P_i position (by about 1 Å) and the P_i is replaced at the same time (Table 4c). Other amino acids such as Asn172 and Asp241 move closer to the CEF. We can now develop a mini-movie for the formation of an enzyme–substrate (ES) complex (Supplementary Movie S1). This movie visualizes how CEF interacts with BlaC. The initial binding phase is complete when the CEF occupancy approaches saturation. Since the aminothiazole ring and, in particular, the dioxotriazine ring of CEF stick out from the center [the β-lactam ring fused to the six-membered thiazine ring; Fig. 1(b)], they are more disordered and their electron densities are weaker. However, clear density features guide a structural refinement that shows that CEF binds through a succession of conformations which may be associated with distinct BlaC intermediates. The separation of these intermediates from the X-ray data is difficult since we have not collected a sufficiently large number of time delays to apply meaningful deconvolution algorithms (Schmidt et al., 2003 ; Kostov & Moffat, 2011 ). The high X-ray pulse-repetition rate of the EuXFEL may make this possible since it allows the fast collection of data sets at tightly spaced delays. Given the resolution of our X-ray data (Table 1), it is challenging to make a distinction between ligand binding being supported by conformational disorder (Tzeng & Kalodimos, 2012 ) or by adaptation of the structure to a changing energy landscape, which would resemble an `induced fit' (Changeux & Edelstein, 2011 ). Both scenarios (Vogt & Di Cera, 2012 ) would most likely result in the same (or a very similar) crystallographic signal. We hypothesize that both mechanisms are involved to some degree, which might be unraveled by single-particle experiments, as recently demonstrated for an unrelated biological system (Dashti et al., 2020 ). However, the structures of BlaC as well as of CEF change [Table 4(c), Supplementary Movie S1], which might be interpreted as the signature of an induced fit after the initial binding event.

Table 4
Important distances in the active centers of BlaC

(a) Distances in (Å) in subunits A and C to the sulbactam (0RN).

	Subunit A	Subunit C
Ser70 OG to P_i O	3.2 (h)	2.6 (h)
Ser70 OG to 0RN OAF	3.1 (h)	3.2 (h)
Gln112 OE1 to 0RN OX	Gln from B, 2.8 (h)	Gln from D, 3.3 (w)
Asn172 ND2 to 0RN OAF	3.2 (h)	3.1 (h)
Glu168 O2 to 0RN OAF	3.0 (h)	2.8 (h)
Arg173 NH1 to 0RN O	2.5 (s)	3.9 (w)
Thr239 O to 0RN OAO	3.9 (w)	2.9 (h)

(b) Distances in (Å) in subunits B and D to the Ser70 trans-enamine (TSS).

	Subunit B	Subunit D
Lys73 NZ to TSS O13	2.8 (h)	3.0 (h)
Gln109 OE1 to TSS O12	Gln from A, 2.7 (h)	Gln from C, 2.9 (h)
Thr239 O to TSS 08	2.9 (h)	2.9 (h)
Asp241 OD2 to TSS O11	6.4	4.1

	Subunit B				Subunit D
	0 ms	5 ms	10 ms	50 ms	0 ms	5 ms	10 ms	50 ms
Ser70 OG to H₂O	3.1 (h)	2.8 (h)	3.3 (w)	2.8 (h)	3.5 (w)	2.4† (s)	3.1 (h)	3.2 (h)
Ser70 OG to P_i O4	3.6 (w)	3.5 (w)	3.4 (w)	2.6 (s)	2.7 (h)	3.7 (w)	3.9 (w)	2.7 (h)
Ser70 OG to CEF O	na‡	3.1 (h)	2.9 (h)	2.9 (h)	na	2.9 (h)	3.0 (h)	2.8 (h)
Ser128 OG to CEF OAD	na	2.4 (s)	2.4 (s)	2.5 (s)	na	2.3 (s)	2.4 (s)	2.6 (h)
Asn172 ND2 to CEF OAR	na	2.7 (h)	3.1 (h)	3.2 (h)	na	2.8 (h)	3.0 (h)	3.1 (h)
Thr237 OG1 to CEF OA1	na	2.7 (h)	3.1 (h)	3.0 (h)	na	2.7 (h)	2.6 (h)	3.1 (h)
Thr239 OG2 to CEF OA1	na	3.3 (w)	3.0 (h)	3.0 (h)	na	3.4 (w)	3.4 (w)	3.1 (h)
Asp241 OD1 to CEF NAC	na	4.7	4.3	3.2 (h)	na	4.4	4.2	3.6 (w)

†Weak OMIT difference electron density.
‡Not applicable.

Formation of the ES complex is most important since it triggers the enzymatic cycle. Hence, it determines the time resolution of the MISC method. The ES complex consists of CEF noncovalently bound in the active site of BlaC (Fig. 4). CEF is delivered by diffusion into the crystals. The crystals must be small enough to enable short enough diffusion times so that the binding kinetics can be observed. However, MISC does not measure the free substrate concentration in the crystals, and therefore diffusion is rather observed indirectly through the increase in the occupancies of well ordered substrate molecules in the active centers of BlaC. When the diffusion times are very short, occupancies may accumulate on a timescale longer than the diffusion time, as they are governed by the binding kinetics. The formation of the ES complex, and therefore the time resolution of the MISC method, is therefore not only dependent on the ligand concentration delivered by diffusion but also on the magnitude of the rate coefficients that characterize the kinetic mechanism.

3.2. Inhibitor binding

The structure of the BlaC–SUB complex was probed at Δt_m = 66 ms. Strong positive DED_iso shows SUB binding to all four subunits of BlaC, which is in stark contrast to CEF, which only binds to subunits B and D. The absence of negative DED_iso at the P_i position [Figs. 7(a) and 7(b)] shows that the P_i does not move and stays in the active site. At the time delay of 66 ms sulbactam binding to BlaC is heterogeneous. In subunits B and D the DED_iso is elongated and stretches outwards from Ser70 [Fig. 7(b)]. In subunits A and C the DED_iso is pillow-like and is more distant from Ser70 [Fig. 7(a)]. The elongated DED_iso in subunits B and D [Fig. 7(b)] can be explained by a covalently bound trans-EN as a result of the reaction of the sulbactam with the catalytic Ser70. The diffusion time is fast enough that 66 ms after mixing all B and D subunits contain trans-EN, the position of which is stabilized by a network of BlaC residues [Fig. 7 and Table 4(b)]. This is quite unexpected, as it was suggested that it would take minutes for the enamine to form after binding of SUB to BlaC (Totir et al., 2007; Cheng et al., 2020; Tassoni et al., 2019). In subunits B and D Arg173 displays a stretched, open conformation, allowing the SUB to orient correctly towards Ser70 and to react swiftly to the trans-EN, which then irreversibly inhibits BlaC (Tassoni et al., 2019). The nearby P_i, which is displaced when the much larger ligand CEF is present, stays in place in all subunits and is likely to add to the stability of both complexes.

Figure 7
BlaC–SUB complexes at Δt_m = 66 ms. (a) Active site in subunit C with noncovalently bound intact sulbactam; left side, DED_iso map (contour: 3σ); right side, 2mF_o − DF_c map (contour: 1.7σ) after refinement. Close-by amino acids and the phosphate (P_i) are marked. (b) Active site in subunit B with trans-enamine bound to Ser70; left side, DED_iso map (contour: 3σ); right side, 2mF_o − DF_c map (contour: 1.7σ) after refinement. Red and blue dots show important differences between the subunits. Gln112 from the adjacent subunit is not located close by and Arg173 is extended in subunit B, leaving subunit B more accessible to ligands and substrate.

The pillow-like DED_iso in a region more distant from Ser70 in subunits A and C [Fig. 7(a)] can be explained by an intact sulbactam molecule that is noncovalently bound to the active site. The SUB is oriented so that the ring sulfur dioxide points towards Ser70, with the β-lactam ring pointing away from Ser70. We hypothesize that this `upside-down' orientation is enforced by Arg173 and Gln112 [Fig. 7(a) and Table 4(a)], where Gln112 protrudes deep into the active sites from the adjacent, noncrystallographically related subunits [Fig. 7(a)]. As the noncovalently bound SUB is oriented incorrectly, Ser70 cannot attack and open the β-lactam ring within the Δt_m of 66 ms. However, the static (cryo) X-ray structure of this complex [Fig. 5(c)] shows that SUB indeed also reacts to the trans-EN in subunits A and C. Accordingly, the BlaC–SUB structure is an interesting intermediate on the catalytic pathway from SUB to trans-EN. The detection of this intermediate would be difficult if not impossible without the MISC experiment.

3.3. Diffusion of substrate in BlaC microcrystals

With D = 2.3 × 10⁻⁶ cm² s⁻¹ for CEF in water [Table 5(b)], the diffusion time into the center of a 10 × 10 × 2 µm crystal volume consisting of water is 1.6 ms. This means that at 5 ms the concentration of CEF molecules would be 96% of the outside concentration (about 144 mM), which is about 20 times higher than the stoichiometric concentration [Table 5(a)]. After integration of the rate equation, the average occupancy would be 99%, which is essentially saturation. This result does not reflect the crystallographically observed occupancy at 5 ms. When decreasing the diffusion coefficient to 2.0 × 10⁻⁷ cm² s⁻¹, the diffusion time into the crystal center increases to 19 ms [see Fig. 6(b) and Table 5(b)]. From this, the decrease of the free BlaC enzyme concentration, the increase of the free CEF concentration and the increase of the BlaC–CEF complex concentration were calculated as explained in Section 2.5. The results are shown in Fig. 6(b). The BlaC–CEF concentration in the center of the crystal lags behind [blue diamonds in Fig. 6(b)] since CEF requires additional time to reach the center and to bind to BlaC. The resulting sigmoidal-shaped response was fitted by a logistic function,

$[{[{\rm ES}]_{\rm center}} = {{100} \over {1 + \exp[-k(t - t_0)]}}, \eqno(5)]$

where t₀ = 13.1 ms denotes the characteristic time when the binding reaction accelerates in the crystal center. With k = 0.3 ms⁻¹ a reasonable steepness of (5) was achieved [Fig. 6(b), blue dashed line]. The t₀ roughly coincides with the diffusion time. Averaged over the entire crystal volume, ∼50% BlaC–CEF occupancy is reached at 5 ms, which is equal to the occupancy determined experimentally at Δt_m = 5 ms [compare the green dashed line in Fig. 6(b) with Fig. 6(a)]. Fig. 8 shows a heatmap that plots BlaC–CEF occupancies through the center of half a BlaC crystal (see also Fig. 9 for a 3D representation). The concentrations of the BlaC–CEF complex are depicted with various colors (see the scale bar on the right). At the edge of the crystal, almost all active BlaC subunits (B and D) are already bound to CEF at 5 ms. In the center the BlaC–CEF complex concentration is 0.21 mM (2.7% of the total concentration of B and D subunits in the crystal), although the CEF concentration delivered by diffusion is already 35 mM (which is the mentioned 23% of the outside CEF concentration but is 5.5 times the stoichiometric concentration). The situation changes completely at 30 ms, where almost 100% occupancy is reached everywhere in the crystal, which is in accordance with earlier results (Olmos et al., 2018) and with the occupancy at Δt_m = 50 ms reported here (see also Supplementary Movie S2). As also discussed earlier, the variation of occupancy across microcrystals at faster mix-and-inject delays does not affect the enzyme kinetics, as the nucleophilic attack of Ser70 of BlaC on the β-lactam ring happens long after the crystals establish full CEF occupancy. It needs to be pointed out here that the simple model of CEF diffusion into BlaC microcrystals and the binding of CEF to BlaC molecules can be augmented by taking into account, for example, the exclusion volume occupied by reacting and nonreacting BlaC subunits (Geremia et al., 2006 ), by the mentioned pointwise depletion of the free CEF concentration in each voxel by binding to BlaC active centers, or the diffusion of substrate directly through protein molecules facilitated by protein dynamics. Since the exact mechanism of diffusion through protein crystals (Geremia et al., 2006) is difficult to determine, the unknown parameters are tied up in the effective diffusion coefficient (D_eff) determined here.

Table 5
Characterization of BlaC–CEF complex formation in crystals

(a) Parameters for the binding of CEF to BlaC [see also Fig. 3 and equation (4)]. The concentration E₀ of all subunits in the BlaC platelet crystal form is 15.5 mM. Only subunits B and D bind substrate. C_0,CEF is the mixed-in substrate concentration [see equation (3)].

E₀ (mM)	C_0,CEF (mM)	k_on (M⁻¹ s⁻¹)
7.8	150	3.2

(b) Parameters in equations (1)–(5) that were fitted to the respective refined occupancy values of CEF and P_i. The comparison of observed and calculated occupancies allows the determination of a diffusion coefficient D_eff.

BlaC–CEF increase, (1)		P_i decrease, (2)	BlaC–CEF in the crystal center, (5)
Observed†		Observed†	Sigmoidal increase‡		D (cm² s⁻¹) for CEF, (3) and (4)
C_S,CEF	τ_1/2 (ms)	τ_1/2 (ms)	k (ms⁻¹)	t₀ (ms)	Water	D_eff§
88%	4.6	6.7	0.3	13.1	2.3 × 10⁻⁶	2 × 10⁻⁷

(c) Calculated occupancies which could be determined with the help of D_eff. The free CEF, free BlaC ([E_free]) and BlaC–CEF complex ([ES]) concentrations were averaged (angle brackets) over all voxels in the crystal. [ES_center] is the BlaC–CEF complex concentration in the center of the microcrystal platelets. Values in parentheses either denote the inside CEF concentration in terms of the percentage of the outside CEF concentration or represent the occupancy values of the relevant species.

Δt_m (ms)	〈[CEF]〉 (mM)	〈[E_free]〉 (mM)	〈[ES]〉 (mM)	[ES_center] (mM)
5	79.4 (53%)	3.9 (50%)	3.9 (50%)	0.2 (2.7%)
10	98.4 (66%)	1.7 (21%)	6.1 (79%)	2.4 (30%)
30	133.3 (89%)	0.0 (0.1%)	7.8 (99.9%)	7.7 (99%)
50	144.4 (96%)	0.0 (0%)	7.8 (100%)	7.8 (100%)

†From fitting saturation curves to refined occupancy values. C_S,CEF is the saturation concentration of CEF; τ_1/2 are characteristic times where 50% of the final concentrations of CEF and phosphate are reached, respectively.
‡Parameters of the logistics function (5

) fitted to occupancies determined in the centers of the BlaC platelets.
§D_eff was obtained by matching the calculated and observed CEF binding kinetics.

Figure 8
Concentrations of the BlaC–CEF complex in 10 × 10 × 2 µm platelet-shaped crystals (a) 5 ms, (b) 10 ms and (c) 30 ms after mixing with 200 mM ceftriaxone (150 mM final concentration assumed). The concentrations are shown in different colors (see the scale bar on the right) in central cross sections through half the width of the crystals. The drawings are not to scale, since the sections displayed are 5 µm horizontally (width) and 2 µm vertically (thickness). The enlargement along the short 2 µm axis allows the display of the nuanced occupancy differences.

Figure 9
3D representation of CEF occupancy values in the BlaC catalytic cleft 5 ms (a) and 10 ms (b) after mixing in a typical BlaC microcrystal platelet. Dark blue colors denote low occupancies and lighter hues denote high occupancies.

3.4. Reaction initiation by diffusion

CEF diffusion is about a factor of 12 slower in the BlaC crystals than in water, with a D_eff of about ∼2 × 10⁻⁷ cm² s⁻¹ [Table 5(b)]. This slowdown is in agreement with findings that were previously obtained from simulations on substrate diffusion in enzyme crystals (Geremia et al., 2006). Estimates of enzyme–ligand occupancies can now be directly deduced from time-resolved X-ray crystallography everywhere in a crystal after mixing. Not surprisingly, at 5 ms the occupancy is high (>90%) only near the crystal surface [Fig. 8(a)], where sufficient substrate is present to promote ES formation at a high rate. In the center of the crystals the ES complex concentration is initially small [Table 5(c), Figs. 8(a) and 9(a)]. The binding rate is not sufficiently high to generate significant occupancy. After Δt_m = 10 ms the binding rate increases, until at 30 ms full occupancy of the BlaC–CEF complex is reached everywhere (Olmos et al., 2018) [Fig. 6(b), green dashed line, Table 5(c)]. With the rapid diffusion of CEF into small BlaC crystals, we are now able to quantify variations of substrate, enzyme and ES concentrations across the enzyme crystal volume at any time [Table 5(c), Figs. 8 and 9]. The remarkable speed of ES accumulation shows that the mix-and-inject technique can be used to characterize enzymes with turnover times much faster than that of BlaC. The direct observation of the important initial ligand- and substrate-binding phase in biomedically relevant enzymes is possible at the EuXFEL.

Since the ES complex (here the BlaC–CEF complex) triggers the enzymatic cycle, accurate kinetics can be extracted to the point where the time required to accumulate sufficient ES complex approaches the lifetime of the next intermediate in the catalytic cycle (Schmidt, 2013). This finding holds for any other technique (Šrajer & Schmidt, 2017) which aims to trigger enzymatic reactions, even in noncrystalline samples. Not only is it required to bring sufficient substrate into the vicinity of the enzyme, but the binding kinetics also need to be taken into account. With microcrystals below a certain crystal size, the binding of substrate, and not the diffusion of substrate into the crystal volume, may become rate-limiting. As a consequence, for BlaC crystals of a size of about 1 µm the speed of ES complex formation is not substantially different from that in solution. The D_eff determined here suggests that accurate measurements of the substrate-binding kinetics would not be possible with significantly larger crystals. Enzymes with turnover times faster than that of BlaC will usually also display faster substrate-binding kinetics with larger k_on rate coefficients. In such cases, the crystal sizes (and their size distributions) or perhaps the temperature must be adjusted appropriately to ensure that the diffusion times can catch up with the substrate-binding rates.

Diffusion is an effective way to initiate reactions. Given a sufficient substrate concentration, and appropriately small crystals, all of the crystal volume is already infused with a multiple of the stoichiometric substrate concentration after a few milliseconds [Table 5(c)]. This is very important for fast reaction initiation since the rate (speed) of enzyme–substrate complex formation, and therefore the time resolution of the method, depends decisively, and primarily, on the concentration of the substrate, and of course also on the free enzyme concentration and the kinetic rate coefficients. Others (Mehrabi, Schulz, Dsouza et al., 2019) have reported significant substrate occupancy in the active site only 30 ms after the activation of a caged substrate that is even located close by. This slow occupancy increase may be a result of (sub-)stoichiometric substrate concentrations in the unit cell, which strengthens our point of view. BlaC is not a fast enzyme. Apart from the possibility of investigating the initial substrate-binding phase(s) potentially on submillisecond timescales, the benefits of XFEL-based mix-and-inject approaches may come to light once faster enzymes with turnover times of <50 ms are investigated. These experiments require small crystals. Exploration of how to investigate these small crystals using either XFELs or synchrotrons, perhaps after upgrade to an advanced accelerator lattice (Eriksson, 2016 ; Wanzenberg et al., 2019 ), remains to be performed.

4. Outlook

In order to further investigate CEF and SUB binding and their reactions with Ser70, a time series should be collected that consists of data sets at multiple Δt_m values that span from a few milliseconds to seconds. To achieve this, the EuXFEL pulse structure must be exploited most efficiently. Every X-ray pulse in all pulse trains provides observations of the same time delay, and our experiments took maximum advantage of the high pulse rate (Fig. 2, inset). This is in contrast to optical pump–X-ray probe experiments, which require appropriate waiting times between laser excitations to guarantee that the laser-excited volume exits the X-ray interaction region, so that multiple laser activations can be avoided (Pandey et al., 2020). We showed that diffraction data sufficient for good-quality structure determination can be collected in about half an hour, as demonstrated for the 50 ms CEF time point. This time can be reduced substantially by limiting the number of diffraction patterns per data set (around 25 000 is appropriate for this space group; Olmos et al., 2018) and by optimizing the crystal density that flows through the mixing device. High crystal density will lead to higher hit rates, but might also cause frequent interruptions caused by injector clogging. In our experiments, a fine balance between crystal size and crystal density was found so that the mix-and-inject experiments with CEF and SUB could be completed successfully with acceptable hit rates (Table 1) given the high X-ray pulse-repetition rate at the EuXFEL. Previous experiments have shown that the collection of sufficient patterns for structure determination should be possible in less than 20 min at the detector-limited repetition rate of the EuXFEL (Yefanov et al., 2019; Pandey et al., 2020). This provides the tantalizing possibility of directly characterizing kinetic processes in biomolecules from single-digit millisecond to longer timescales within relatively short experimental times. The kinetics can rapidly change when environmental conditions are varied. It may be possible, for example, to control the temperature in the mixing injector delay line to determine barriers of activation from the resulting X-ray data (Schmidt et al., 2013 ). The full analysis of such a multidimensional data set requires the development and deployment of user-friendly classification algorithms to separate mixtures into their pure components (Schmidt et al., 2003) and to derive kinetics and energetics (Schmidt et al., 2013) consistent with the electron-density maps and the structures of intermediate states along the reaction pathway.

5. Summary

Our experiments permitted a real-time view into the active sites of an enzyme during substrate binding. They facilitate more mix-and-inject experiments at the EuXFEL with unprecedented data-collection rates, allowing more structures to be determined per allocated experimental time. This capability will become an important tool for biomedically relevant research in years to come.

APPENDIX A

Microcrystals and data collection

Fig. 10(a) shows a microscopic image of the BlaC platelets used for the experiments. They appear to be uniform in size and shape. In Fig. 10(b) the hit and indexing rates achieved with these crystals in our MISC experiments are displayed across all of the pulses in the pulse train of the EuXFEL. A decay in the hit rate following pulse 1 is not observed. This is an indication that the jet is fast enough that a fresh jet volume is intercepted by the following X-ray pulses (Wiedorn, Oberthür et al., 2018; Yefanov et al., 2019; Pandey et al., 2020).

Figure 10
Crystals, hit and indexing rates. (a) Microscopic image of the platelet crystal form of BlaC and (b) exemplary hit (red squares) and indexing (black spheres) rates from BlaC/CEF mixing as a function of the pulse ID in the train. Both rates are stable across the entire pulse train.

APPENDIX B

Diffraction patterns and masks

The ability to mask out detector pixels and other parts of the diffraction pattern (Fig. 11) is important for the successful identification of DP-containing Bragg reflections (hits) from the stream of detector images (Wiedorn, Oberthür et al., 2018; Carrillo et al., 2021). Only peaks [blue squares in Figs. 11(a) and 11(b)] outside the mask are found. In the hit-finder Cheetah (Barty et al., 2014) a convenient masking tool is available that facilitates the exclusion of any part of the detector image. The central `hole' and the gaps (except for the tile edges) do not need to be masked since the detector geometry is known.

Figure 11
(a) Example of a diffraction pattern collected by the AGIPD. In (b) a mask (in red) is superposed that covers the strong rings at low resolution and inactive detector areas.

Supporting information

3D view

PDB references: BlaC, unmixed, 7k8l; mixed with ceftriaxone, 5 ms, 7k8e; 10 ms, 7k8f; 50 ms, 7k8h; mixed with sulbactam, 66 ms, 7k8k

Acknowledgements

We are very grateful to those who supported this experiment by being present in person at the European XFEL during the onset of the COVID-19 pandemic in March 2020. We acknowledge the European XFEL in Schenefeld, Germany for the provision of X-ray free-electron laser beamtime on the SPB/SFX scientific instrument and would like to thank the staff for their assistance. We acknowledge the use of the XBI facility at the European XFEL. The SFX stream files were deposited in the CXIDB with code 170. Individual contributions were as follows. SP, TM, JM-G, JH-Y, FK, IP, MM, RJ, MS, WX and JO expressed, purified and crystallized the protein. RB, KD, HK, MK, JK, GM, TS and MV operated the SPB/SFX instrument. LP, AMK, GC and KAZ designed and provided injector nozzles. MV, FK and MK assembled and operated the nozzles. FK, JM-G, J-HY, LG and PS collected the data. SP, IP, OY, VM, PS, AT and AB processed the data. SP, IP, TM, GP and MS analyzed the data. IP, MF, AS, FK, PS and MS logged the experiment. RB, APM, MS and GP designed the experiment. SP, PF, APM, RB, GP and MS wrote the manuscript with input from all other authors.

Funding information

This work was supported by the National Science Foundation Science and Technology Center `BioXFEL' through award STC-1231306, and in part by the US Department of Energy, Office of Science, Basic Energy Sciences under contract DE-SC0002164 (AO, algorithm design and development) and by the National Science Foundation under contract Nos. 1551489 (AO, underlying analytical models) and DBI-2029533 (AO, functional conformations). This material is based upon work supported by the National Science Foundation Graduate Research Fellowship Program under Grant No. 1450681 to JLO. The work was also supported by funds from the National Institutes of Health grant R01 GM117342-0404. Funding and support are also acknowledged from the National Institutes of Health grant R01 GM095583, from the Biodesign Center for Applied Structural Discovery at ASU, from National Science Foundation award No. 1565180 and the US Department of Energy through Lawrence Livermore National Laboratory under contract DE-AC52-07NA27344. KAZ was supported by the Cornell Molecular Biophysics Training Program (NIH T32-GM008267). This work was also supported by the Cluster of Excellence `CUI: Advanced Imaging of Matter' of the Deutsche Forschungsgemeinschaft (DFG), EXC 2056, project ID 390715994. CFEL is supported by the Gottfried Wilhelm Leibniz Program of the DFG, the `X-probe' project funded by the European Union 2020 Research and Innovation Program under Marie Sklodowska-Curie grant agreement 637295, the European Research Council, `Frontiers in Attosecond X-ray Science: Imaging and Spectroscopy (AXSIS)', ERC-2013-SyG 609920, and the Human Frontiers Science Program grant RGP0010 2017. This work is also supported by the AXSIS project funded by the European Research Council under the European Union Seventh Framework Program (FP/2007-2013)/ERC Grant Agreement No. 609920.

References

Allahgholi, A., Becker, J., Delfs, A., Dinapoli, R., Goettlicher, P., Greiffenberg, D., Henrich, B., Hirsemann, H., Kuhn, M., Klanner, R., Klyuev, A., Krueger, H., Lange, S., Laurus, T., Marras, A., Mezza, D., Mozzanica, A., Niemann, M., Poehlsen, J., Schwandt, J., Sheviakov, I., Shi, X., Smoljanin, S., Steffen, L., Sztuk-Dambietz, J., Trunk, U., Xia, Q., Zeribi, M., Zhang, J., Zimmer, M., Schmitt, B. & Graafsma, H. (2019). J. Synchrotron Rad. 26, 74–82. Web of Science CrossRef CAS IUCr Journals Google Scholar
Barends, T. R. M., Foucar, L., Ardevol, A., Nass, K., Aquila, A., Botha, S., Doak, R. B., Falahati, K., Hartmann, E., Hilpert, M., Heinz, M., Hoffmann, M. C., Kofinger, J., Koglin, J. E., Kovacsova, G., Liang, M., Milathianaki, D., Lemke, H. T., Reinstein, J., Roome, C. M., Shoeman, R. L., Williams, G. J., Burghardt, I., Hummer, G., Boutet, S. & Schlichting, I. (2015). Science, 350, 445–450. Web of Science CrossRef CAS PubMed Google Scholar
Barty, A., Kirian, R. A., Maia, F. R. N. C., Hantke, M., Yoon, C. H., White, T. A. & Chapman, H. (2014). J. Appl. Cryst. 47, 1118–1131. Web of Science CrossRef CAS IUCr Journals Google Scholar
Berman, H. M., Battistuz, T., Bhat, T. N., Bluhm, W. F., Bourne, P. E., Burkhardt, K., Feng, Z., Gilliland, G. L., Iype, L., Jain, S., Fagan, P., Marvin, J., Padilla, D., Ravichandran, V., Schneider, B., Thanki, N., Weissig, H., Westbrook, J. D. & Zardecki, C. (2002). Acta Cryst. D58, 899–907. Web of Science CrossRef CAS IUCr Journals Google Scholar
Boutet, S., Lomb, L., Williams, G. J., Barends, T. R., Aquila, A., Doak, R. B., Weierstall, U., DePonte, D. P., Steinbrener, J., Shoeman, R. L., Messerschmidt, M., Barty, A., White, T. A., Kassemeyer, S., Kirian, R. A., Seibert, M. M., Montanez, P. A., Kenney, C., Herbst, R., Hart, P., Pines, J., Haller, G., Gruner, S. M., Philipp, H. T., Tate, M. W., Hromalik, M., Koerner, L. J., van Bakel, N., Morse, J., Ghonsalves, W., Arnlund, D., Bogan, M. J., Caleman, C., Fromme, R., Hampton, C. Y., Hunter, M. S., Johansson, L. C., Katona, G., Kupitz, C., Liang, M., Martin, A. V., Nass, K., Redecke, L., Stellato, F., Timneanu, N., Wang, D., Zatsepin, N. A., Schafer, D., Defever, J., Neutze, R., Fromme, P., Spence, J. C. H., Chapman, H. N. & Schlichting, I. (2012). Science, 337, 362–364. Web of Science CrossRef CAS PubMed Google Scholar
Boyd, D. B. & Lunn, W. H. (1979). J. Med. Chem. 22, 778–784. CrossRef CAS PubMed Web of Science Google Scholar
Calvey, G. D., Katz, A. M. & Pollack, L. (2019). Anal. Chem. 91, 7139–7144. Web of Science CrossRef CAS PubMed Google Scholar
Carrillo, M., Pandey, S., Sanchez, J., Noda, M., Poudyal, I., Aldama, L., Malla, T. N., Claesson, E., Wahlgren, W. Y., Feliz, D., Šrajer, V., Maj, M., Castillon, L., Iwata, S., Nango, E., Tanaka, R., Tanaka, T., Fangjia, L., Tono, K., Owada, S., Westenhoff, S., Stojković, E. A. & Schmidt, M. (2021). Structure, 29, 743–754. Web of Science CrossRef CAS PubMed Google Scholar
Carslaw, H. S. & Jaeger, J. C. (1959). Conduction Heat in Solids, 2nd ed. Oxford: Clarendon Press. Google Scholar
Cassini, A., Högberg, L. D., Plachouras, D., Quattrocchi, A., Hoxha, A., Simonsen, G. S., Colomb-Cotinat, M., Kretzschmar, M. E., Devleesschauwer, B., Cecchini, M., Ouakrim, D. A., Oliveira, T. C., Struelens, M. J., Suetens, C., Monnet, D. L., Strauss, R., Mertens, K., Struyf, T., Catry, B., Latour, K., Ivanov, I. N., Dobreva, E. G., Tambic-Andraševic, A., Soprek, S., Budimir, A., Paphitou, N., Žemlicková, H., Schytte Olsen, S., Wolff Sönksen, U., Märtin, P., Ivanova, M., Lyytikäinen, O., Jalava, J., Coignard, B., Eckmanns, T., Abu Sin, M., Haller, S., Daikos, G. L., Gikas, A., Tsiodras, S., Kontopidou, F., Tóth, Á., Hajdu, Á., Guólaugsson, Ó., Kristinsson, K. G., Murchan, S., Burns, K., Pezzotti, P., Gagliotti, C., Dumpis, U., Liuimiene, A., Perrin, M., Borg, M. A., de Greeff, S. C., Monen, J. C., Koek, M. B., Elstrøm, P., Zabicka, D., Deptula, A., Hryniewicz, W., Caniça, M., Nogueira, P. J., Fernandes, P. A., Manageiro, V., Popescu, G. A., Serban, R. I., Schréterová, E., Litvová, S., Štefkovicová, M., Kolman, J., Klavs, I., Korošec, A., Aracil, B., Asensio, A., Pérez-Vázquez, M., Billström, H., Larsson, S., Reilly, J. S., Johnson, A. & Hopkins, S. (2019). Lancet Infect. Dis. 19, 56–66. Web of Science CrossRef PubMed Google Scholar
Changeux, J.-P. & Edelstein, S. (2011). F1000 Biol. Rep. 3, 19. Google Scholar
Chapman, H. N., Fromme, P., Barty, A., White, T. A., Kirian, R. A., Aquila, A., Hunter, M. S., Schulz, J., DePonte, D. P., Weierstall, U., Doak, R. B., Maia, F. R. N. C., Martin, A. V., Schlichting, I., Lomb, L., Coppola, N., Shoeman, R. L., Epp, S. W., Hartmann, R., Rolles, D., Rudenko, A., Foucar, L., Kimmel, N., Weidenspointner, G., Holl, P., Liang, M., Barthelmess, M., Caleman, C., Boutet, S., Bogan, M. J., Krzywinski, J., Bostedt, C., Bajt, S., Gumprecht, L., Rudek, B., Erk, B., Schmidt, C., Hömke, A., Reich, C., Pietschner, D., Strüder, L., Hauser, G., Gorke, H., Ullrich, J., Herrmann, S., Schaller, G., Schopper, F., Soltau, H., Kühnel, K.-U., Messerschmidt, M., Bozek, J. D., Hau-Riege, S. P., Frank, M., Hampton, C. Y., Sierra, R. G., Starodub, D., Williams, G. J., Hajdu, J., Timneanu, N., Seibert, M. M., Andreasson, J., Rocker, A., Jönsson, O., Svenda, M., Stern, S., Nass, K., Andritschke, R., Schröter, C.-D., Krasniqi, F., Bott, M., Schmidt, K. E., Wang, X., Grotjohann, I., Holton, J. M., Barends, T. R. M., Neutze, R., Marchesini, S., Fromme, R., Schorb, S., Rupp, D., Adolph, M., Gorkhover, T., Andersson, I., Hirsemann, H., Potdevin, G., Graafsma, H., Nilsson, B. & Spence, J. C. H. (2011). Nature, 470, 73–77. Web of Science CrossRef CAS PubMed Google Scholar
Cheng, Q., Xu, C., Chai, J., Zhang, R., Wai Chi Chan, E. & Chen, S. (2020). ACS Infect. Dis. 6, 577–587. Web of Science CrossRef CAS PubMed Google Scholar
Coquelle, N., Sliwa, M., Woodhouse, J., Schirò, G., Adam, V., Aquila, A., Barends, T. R. M., Boutet, S., Byrdin, M., Carbajo, S., De la Mora, E., Doak, R. B., Feliks, M., Fieschi, F., Foucar, L., Guillon, V., Hilpert, M., Hunter, M. S., Jakobs, S., Koglin, J. E., Kovacsova, G., Lane, T. J., Lévy, B., Liang, M. N., Nass, K., Ridard, J., Robinson, J. S., Roome, C. M., Ruckebusch, C., Seaberg, M., Thepaut, M., Cammarata, M., Demachy, I., Field, M., Shoeman, R. L., Bourgeois, D., Colletier, J.-P., Schlichting, I. & Weik, M. (2018). Nat. Chem. 10, 31–37. Web of Science CrossRef CAS PubMed Google Scholar
Dashti, A., Mashayekhi, G., Shekhar, M., Ben Hail, D., Salah, S., Schwander, P., des Georges, A., Singharoy, A., Frank, J. & Ourmazd, A. (2020). Nat. Commun. 11, 4734. Web of Science CrossRef PubMed Google Scholar
Decking, W., Abeghyan, S., Abramian, P., Abramsky, A., Aguirre, A., Albrecht, C., Alou, P., Altarelli, M., Altmann, P., Amyan, K., Anashin, V., Apostolov, E., Appel, K., Auguste, D., Ayvazyan, V., Baark, S., Babies, F., Baboi, N., Bak, P., Balandin, V., Baldinger, R., Baranasic, B., Barbanotti, S., Belikov, O., Belokurov, V., Belova, L., Belyakov, V., Berry, S., Bertucci, M., Beutner, B., Block, A., Blocher, M., Bockmann, T., Bohm, C., Bohnert, M., Bondar, V., Bondarchuk, E., Bonezzi, M., Borowiec, P., Bosch, C., Bosenberg, U., Bosotti, A., Bospflug, R., Bousonville, M., Boyd, E., Bozhko, Y., Brand, A., Branlard, J., Briechle, S., Brinker, F., Brinker, S., Brinkmann, R., Brockhauser, S., Brovko, O., Bruck, H., Brudgam, A., Butkowski, L., Buttner, T., Calero, J., Castro-Carballo, E., Cattalanotto, G., Charrier, J., Chen, J., Cherepenko, A., Cheskidov, V., Chiodini, M., Chong, A., Choroba, S., Chorowski, M., Churanov, D., Cichalewski, W., Clausen, M., Clement, W., Cloue, C., Cobos, J. A., Coppola, N., Cunis, S., Czuba, K., Czwalinna, M., D'Almagne, B., Dammann, J., Danared, H., Wagner, A. D., Delfs, A., Delfs, T., Dietrich, F., Dietrich, T., Dohlus, M., Dommach, M., Donat, A., Dong, X., Doynikov, N., Dressel, M., Duda, M., Duda, P., Eckoldt, H., Ehsan, W., Eidam, J., Eints, F., Engling, C., Englisch, U., Ermakov, A., Escherich, K., Eschke, J., Saldin, E., Faesing, M., Fallou, A., Felber, M., Fenner, M., Fernandes, B., Fernandez, J. M., Feuker, S., Filippakopoulos, K., Floettmann, K., Fogel, V., Fontaine, M., Frances, A., Martin, I. F., Freund, W., Freyermuth, T., Friedland, M., Frohlich, L., Fusetti, M., Fydrych, J., Gallas, A., Garcia, O., Garcia-Tabares, L., Geloni, G., Gerasimova, N., Gerth, C., Gessler, P., Gharibyan, V., Gloor, M., Glowinkowski, J., Goessel, A., Golebiewski, Z., Golubeva, N., Grabowski, W., Graeff, W., Grebentsov, A., Grecki, M., Grevsmuehl, T., Gross, M., Grosse-Wortmann, U., Grunert, J., Grunewald, S., Grzegory, P., Feng, G., Guler, H., Gusev, G., Gutierrez, J. L., Hagge, L., Hamberg, M., Hanneken, R., Harms, E., Hartl, I., Hauberg, A., Hauf, S., Hauschildt, J., Hauser, J., Havlicek, J., Hedqvist, A., Heidbrook, N., Hellberg, F., Henning, D., Hensler, O., Hermann, T., Hidvegi, A., Hierholzer, M., Hintz, H., Hoffmann, F., Hoffmann, M., Hoffmann, M., Holler, Y., Huning, M., Ignatenko, A., Ilchen, M., Iluk, A., Iversen, J., Iversen, J., Izquierdo, M., Jachmann, L., Jardon, N., Jastrow, U., Jensch, K., Jensen, J., Dotabek, M. J. O., Jidda, M., Jin, H., Johansson, N., Jonas, R., Kaabi, W., Kaefer, D., Kammering, R., Kapitza, H., Karabekyan, S., Karstensen, S., Kasprzak, K., Katalev, V., Keese, D., Keil, B., Kholopov, M., Killenberger, M., Kitaev, B., Klimchenko, Y., Klos, R., Knebel, L., Koch, A., Koepke, M., Kohler, S., Kohler, W., Kohlstrunk, N., Konopkova, Z., Konstantinov, A., Kook, W., Koprek, W., Korfer, M., Korth, O., Kosarev, A., Kosinski, K., Kostin, D., Kot, Y., Kotarba, A., Kozak, T., Kozak, V., Kramert, R., Krasilnikov, M., Krasnov, A., Krause, B., Kravchuk, L., Krebs, O., Kretschmer, R., Kreutzkamp, J., Kroplin, O., Krzysik, K., Kube, G., Kuehn, H., Kujala, N., Kulikov, V., Kuzminych, V., La Civita, D., Lacroix, M., Lamb, T., Lancetov, A., Larsson, M., Le Pinvidic, D., Lederer, S., Lensch, T., Lenz, D., Leuschner, A., Levenhagen, F., Li, Y., Liebing, J., Lilje, L., Limberg, T., Lipka, D., List, B., Liu, J., Liu, S., Lorbeer, B., Lorkiewicz, J., Lu, H. H., Ludwig, F., Machau, K., Maciocha, W., Madec, C., Magueur, C., Maiano, C., Maksimova, I., Malcher, K., Maltezopoulos, T., Mamoshkina, E., Manschwetus, B., Marcellini, F., Marinkovic, G., Martinez, T., Martirosyan, H., Maschmann, W., Maslov, M., Matheisen, A., Mavric, U., Meissner, J., Meissner, K., Messerschmidt, M., Meyners, N., Michalski, G., Michelato, P., Mildner, N., Moe, M., Moglia, F., Mohr, C., Mohr, S., Moller, W., Mommerz, M., Monaco, L., Montiel, C., Moretti, M., Morozov, I., Morozov, P., Mross, D., Mueller, J., Muller, C., Muller, J., Muller, K., Munilla, J., Munnich, A., Muratov, V., Napoly, O., Naser, B., Nefedov, N., Neumann, R., Neumann, R., Ngada, N., Noelle, D., Obier, F., Okunev, I., Oliver, J. A., Omet, M., Oppelt, A., Ottmar, A., Oublaid, M., Pagani, C., Paparella, R., Paramonov, V., Peitzmann, C., Penning, J., Perus, A., Peters, F., Petersen, B., Petrov, A., Petrov, I., Pfeiffer, S., Pfluger, J., Philipp, S., Pienaud, Y., Pierini, P., Pivovarov, S., Planas, M., Plawski, E., Pohl, M., Polinski, J., Popov, V., Prat, S., Prenting, J., Priebe, G., Pryschelski, H., Przygoda, K., Pyata, E., Racky, B., Rathjen, A., Ratuschni, W., Regnaud-Campderros, S., Rehlich, K., Reschke, D., Robson, C., Roever, J., Roggli, M., Rothenburg, J., Rusinski, E., Rybaniec, R., Sahling, H., Salmani, M., Samoylova, L., Sanzone, D., Saretzki, F., Sawlanski, O., Schaffran, J., Schlarb, H., Schlosser, M., Schlott, V., Schmidt, C., Schmidt-Foehre, F., Schmitz, M., Schmokel, M., Schnautz, T., Schneidmiller, E., Scholz, M., Schoneburg, B., Schultze, J., Schulz, C., Schwarz, A., Sekutowicz, J., Sellmann, D., Semenov, E., Serkez, S., Sertore, D., Shehzad, N., Shemarykin, P., Shi, L., Sienkiewicz, M., Sikora, D., Sikorski, M., Silenzi, A., Simon, C., Singer, W., Singer, X., Sinn, H., Sinram, K., Skvorodnev, N., Smirnow, P., Sommer, T., Sorokin, A., Stadler, M., Steckel, M., Steffen, B., Steinhau-Kuhl, N., Stephan, F., Stodulski, M., Stolper, M., Sulimov, A., Susen, R., Swierblewski, J., Sydlo, C., Syresin, E., Sytchev, V., Szuba, J., Tesch, N., Thie, J., Thiebault, A., Tiedtke, K., Tischhauser, D., Tolkiehn, J., Tomin, S., Tonisch, F., Toral, F., Torbin, I., Trapp, A., Treyer, D., Trowitzsch, G., Trublet, T., Tschentscher, T., Ullrich, F., Vannoni, M., Varela, P., Varghese, G., Vashchenko, G., Vasic, M., Vazquez-Velez, C., Verguet, A., Vilcins-Czvitkovits, S., Villanueva, R., Visentin, B., Viti, M., Vogel, E., Volobuev, E., Wagner, R., Walker, N., Wamsat, T., Weddig, H., Weichert, G., Weise, H., Wenndorf, R., Werner, M., Wichmann, R., Wiebers, C., Wiencek, M., Wilksen, T., Will, I., Winkelmann, L., Winkowski, M., Wittenburg, K., Witzig, A., Wlk, P., Wohlenberg, T., Wojciechowski, M., Wolff-Fabris, F., Wrochna, G., Wrona, K., Yakopov, M., Yang, B., Yang, F., Yurkov, M., Zagorodnov, I., Zalden, P., Zavadtsev, A., Zavadtsev, D., Zhirnov, A., Zhukov, A., Ziemann, V., Zolotov, A., Zolotukhina, N., Zummack, F. & Zybin, D. (2020). Nat. Photonics, 14, 391–397. Web of Science CrossRef CAS Google Scholar
Dods, R., Båth, P., Morozov, D., Gagnér, V. A., Arnlund, D., Luk, H. L., Kübel, J., Maj, M., Vallejos, A., Wickstrand, C., Bosman, R., Beyerlein, K. R., Nelson, G., Liang, M. N., Milathianaki, D., Robinson, J., Harimoorthy, R., Berntsen, P., Malmerberg, E., Johansson, L., Andersson, R., Carbajo, S., Claesson, E., Conrad, C. E., Dahl, P., Hammarin, G., Hunter, M. S., Li, C. F., Lisova, S., Royant, A., Safari, C., Sharma, A., Williams, G. J., Yefanov, O., Westenhoff, S., Davidsson, J., DePonte, D. P., Boutet, S., Barty, A., Katona, G., Groenhof, G., Brändén, G. & Neutze, R. (2021). Nature, 589, 310–314. Web of Science CrossRef CAS PubMed Google Scholar
Eriksson, M. (2016). AIP Conf. Proc. 1741, 020001. Google Scholar
Fair, R. J. & Tor, Y. (2014). Perspect. Medicin. Chem. 6, PMC.S14459. CrossRef Google Scholar
Geremia, S., Campagnolo, M., Demitri, N. & Johnson, L. N. (2006). Structure, 14, 393–400. Web of Science CrossRef PubMed CAS Google Scholar
Gevorkov, Y., Yefanov, O., Barty, A., White, T. A., Mariani, V., Brehm, W., Tolstikova, A., Grigat, R.-R. & Chapman, H. N. (2019). Acta Cryst. A75, 694–704. Web of Science CrossRef IUCr Journals Google Scholar
Gourinchas, G., Etzl, S., Göbl, C., Vide, U., Madl, T. & Winkler, A. (2017). Sci. Adv. 3, e1602498. Web of Science CrossRef PubMed Google Scholar
Grünbein, M. L., Gorel, A., Foucar, L., Carbajo, S., Colocho, W., Gilevich, S., Hartmann, E., Hilpert, M., Hunter, M., Kloos, M., Koglin, J. E., Lane, T. J., Lewandowski, J., Lutman, A., Nass, K., Nass Kovacs, G., Roome, C. M., Sheppard, J., Shoeman, R. L., Stricker, M., van Driel, T., Vetter, S., Doak, R. B., Boutet, S., Aquila, A., Decker, F. J., Barends, T. R. M., Stan, C. A. & Schlichting, I. (2021). Nat. Commun. 12, 1672. Web of Science PubMed Google Scholar
Han, H., Round, E., Schubert, R., Gül, Y., Makroczyová, J., Meza, D., Heuser, P., Aepfelbacher, M., Barák, I., Betzel, C., Fromme, P., Kursula, I., Nissen, P., Tereschenko, E., Schulz, J., Uetrecht, C., Ulicný, J., Wilmanns, M., Hajdu, J., Lamzin, V. S. & Lorenzen, K. (2021). J. Appl. Cryst. 54, 7–21. Web of Science CrossRef CAS IUCr Journals Google Scholar
Hartmann, N., Helml, W., Galler, A., Bionta, M. R., Grünert, J. L., Molodtsov, S., Ferguson, K. R., Schorb, S., Swiggers, M. L., Carron, S., Bostedt, C., Castagna, J., Bozek, J., Glownia, J. M., Kane, D. J., Fry, A. R., White, W. E., Hauri, C. P., Feurer, T. & Coffee, R. N. (2014). Nat. Photonics, 8, 706–709. Web of Science CrossRef CAS Google Scholar
Holtorf, H., Reinbothe, S., Reinbothe, C., Bereza, B. & Apel, K. (1995). Proc. Natl Acad. Sci. USA, 92, 3254–3258. CrossRef CAS PubMed Web of Science Google Scholar
Hugonnet, J. E. & Blanchard, J. S. (2007). Biochemistry, 46, 11998–12004. Web of Science CrossRef PubMed CAS Google Scholar
Imming, P., Sinning, C. & Meyer, A. (2006). Nat. Rev. Drug Discov. 5, 821–834. Web of Science CrossRef PubMed CAS Google Scholar
Ishigami, I., Lewis-Ballester, A., Echelmeier, A., Brehm, G., Zatsepin, N. A., Grant, T. D., Coe, J. D., Lisova, S., Nelson, G., Zhang, S., Dobson, Z. F., Boutet, S., Sierra, R. G., Batyuk, A., Fromme, P., Fromme, R., Spence, J. C. H., Ros, A., Yeh, S. R. & Rousseau, D. L. (2019). Proc. Natl Acad. Sci. USA, 116, 3572–3577. Web of Science CrossRef CAS PubMed Google Scholar
Jeffrey, G. A. (1997). An Introduction to Hydrogen Bonding. Oxford University Press. Google Scholar
Kern, J., Chatterjee, R., Young, I. D., Fuller, F. D., Lassalle, L., Ibrahim, M., Gul, S., Fransson, T., Brewster, A. S., Alonso-Mori, R., Hussein, R., Zhang, M., Douthit, L., de Lichtenberg, C., Cheah, M. H., Shevela, D., Wersig, J., Seuffert, I., Sokaras, D., Pastor, E., Weninger, C., Kroll, T., Sierra, R. G., Aller, P., Butryn, A., Orville, A. M., Liang, M., Batyuk, A., Koglin, J. E., Carbajo, S., Boutet, S., Moriarty, N. W., Holton, J. M., Dobbek, H., Adams, P. D., Bergmann, U., Sauter, N. K., Zouni, A., Messinger, J., Yano, J. & Yachandra, V. K. (2018). Nature, 563, 421–425. Web of Science CrossRef CAS PubMed Google Scholar
Kostov, K. S. & Moffat, K. (2011). Biophys. J. 100, 440–449. Web of Science CrossRef CAS PubMed Google Scholar
Kupitz, C., Basu, S., Grotjohann, I., Fromme, R., Zatsepin, N. A., Rendek, K. N., Hunter, M. S., Shoeman, R. L., White, T. A., Wang, D., James, D., Yang, J.-H., Cobb, D. E., Reeder, B., Sierra, R. G., Liu, H., Barty, A., Aquila, A. L., Deponte, D., Kirian, R. A., Bari, S., Bergkamp, J. J., Beyerlein, K. R., Bogan, M. J., Caleman, C., Chao, T.-C., Conrad, C. E., Davis, K. M., Fleckenstein, H., Galli, L., Hau-Riege, S. P., Kassemeyer, S., Laksmono, H., Liang, M., Lomb, L., Marchesini, S., Martin, A. V., Messerschmidt, M., Milathianaki, D., Nass, K., Ros, A., Roy-Chowdhury, S., Schmidt, K., Seibert, M., Steinbrener, J., Stellato, F., Yan, L., Yoon, C., Moore, T. A., Moore, A. L., Pushkar, Y., Williams, G. J., Boutet, S., Doak, R. B., Weierstall, U., Frank, M., Chapman, H. N., Spence, J. C. H. & Fromme, P. (2014). Nature, 513, 261–265. Web of Science CrossRef CAS PubMed Google Scholar
Kupitz, C., Olmos, J. L. Jr, Holl, M., Tremblay, L., Pande, K., Pandey, S., Oberthür, D., Hunter, M., Liang, M., Aquila, A., Tenboer, J., Calvey, G., Katz, A., Chen, Y., Wiedorn, M. O., Knoska, J., Meents, A., Majriani, V., Norwood, T., Poudyal, I., Grant, T., Miller, M. D., Xu, W., Tolstikova, A., Morgan, A., Metz, M., Martin-Garcia, J. M., Zook, J. D., Roy-Chowdhury, S., Coe, J., Nagaratnam, N., Meza, D., Fromme, R., Basu, S., Frank, M., White, T., Barty, A., Bajt, S., Yefanov, O., Chapman, H. N., Zatsepin, N., Nelson, G., Weierstall, U., Spence, J., Schwander, P., Pollack, L., Fromme, P., Ourmazd, A., Phillips, G. N. Jr & Schmidt, M. (2017). Struct. Dyn. 4, 044003. Web of Science CrossRef PubMed Google Scholar
Li, J., Liu, Z., Tan, C., Guo, X., Wang, L., Sancar, A. & Zhong, D. (2010). Nature, 466, 887–890. Web of Science CrossRef CAS PubMed Google Scholar
Liebschner, D., Afonine, P. V., Baker, M. L., Bunkóczi, G., Chen, V. B., Croll, T. I., Hintze, B., Hung, L.-W., Jain, S., McCoy, A. J., Moriarty, N. W., Oeffner, R. D., Poon, B. K., Prisant, M. G., Read, R. J., Richardson, J. S., Richardson, D. C., Sammito, M. D., Sobolev, O. V., Stockwell, D. H., Terwilliger, T. C., Urzhumtsev, A. G., Videau, L. L., Williams, C. J. & Adams, P. D. (2019). Acta Cryst. D75, 861–877. Web of Science CrossRef IUCr Journals Google Scholar
Liebschner, D., Afonine, P. V., Moriarty, N. W., Poon, B. K., Sobolev, O. V., Terwilliger, T. C. & Adams, P. D. (2017). Acta Cryst. D73, 148–157. Web of Science CrossRef IUCr Journals Google Scholar
Lomb, L., Barends, T. R. M., Kassemeyer, S., Aquila, A., Epp, S. W., Erk, B., Foucar, L., Hartmann, R., Rudek, B., Rolles, D., Rudenko, A., Shoeman, R. L., Andreasson, J., Bajt, S., Barthelmess, M., Barty, A., Bogan, M. J., Bostedt, C., Bozek, J. D., Caleman, C., Coffee, R., Coppola, N., DePonte, D. P., Doak, R. B., Ekeberg, T., Fleckenstein, H., Fromme, P., Gebhardt, M., Graafsma, H., Gumprecht, L., Hampton, C. Y., Hartmann, A., Hauser, G., Hirsemann, H., Holl, P., Holton, J. M., Hunter, M. S., Kabsch, W., Kimmel, N., Kirian, R. A., Liang, M., Maia, F. R. N. C., Meinhart, A., Marchesini, S., Martin, A. V., Nass, K., Reich, C., Schulz, J., Seibert, M. M., Sierra, R., Soltau, H., Spence, J. C. H., Steinbrener, J., Stellato, F., Stern, S., Timneanu, N., Wang, X., Weidenspointner, G., Weierstall, U., White, T. A., Wunderer, C., Chapman, H. N., Ullrich, J., Strüder, L. & Schlichting, I. (2011). Phys. Rev. B, 84, 214111. Web of Science CrossRef Google Scholar
Mancuso, A. P., Aquila, A., Batchelor, L., Bean, R. J., Bielecki, J., Borchers, G., Doerner, K., Giewekemeyer, K., Graceffa, R., Kelsey, O. D., Kim, Y., Kirkwood, H. J., Legrand, A., Letrun, R., Manning, B., Lopez Morillo, L., Messerschmidt, M., Mills, G., Raabe, S., Reimers, N., Round, A., Sato, T., Schulz, J., Signe Takem, C., Sikorski, M., Stern, S., Thute, P., Vagovič, P., Weinhausen, B. & Tschentscher, T. (2019). J Synchrotron Rad, 26, 660–676. Web of Science CrossRef CAS IUCr Journals Google Scholar
Mariani, V., Morgan, A., Yoon, C. H., Lane, T. J., White, T. A., O'Grady, C., Kuhn, M., Aplin, S., Koglin, J., Barty, A. & Chapman, H. N. (2016). J. Appl. Cryst. 49, 1073–1080. Web of Science CrossRef CAS IUCr Journals Google Scholar
Mehrabi, P., Schulz, E. C., Agthe, M., Horrell, S., Bourenkov, G., von Stetten, D., Leimkohl, J. P., Schikora, H., Schneider, T. R., Pearson, A. R., Tellkamp, F. & Miller, R. J. D. (2019). Nat. Methods, 16, 979–982. Web of Science CrossRef CAS PubMed Google Scholar
Mehrabi, P., Schulz, E. C., Dsouza, R., Müller-Werkmeister, H. M., Tellkamp, F., Miller, R. J. D. & Pai, E. F. (2019). Science, 365, 1167–1170. Web of Science CrossRef CAS PubMed Google Scholar
Minor, W., Cymborowski, M., Otwinowski, Z. & Chruszcz, M. (2006). Acta Cryst. D62, 859–866. Web of Science CrossRef CAS IUCr Journals Google Scholar
Moffat, K. (2001). Chem. Rev. 101, 1569–1582. Web of Science CrossRef PubMed CAS Google Scholar
Murshudov, G. N., Skubák, P., Lebedev, A. A., Pannu, N. S., Steiner, R. A., Nicholls, R. A., Winn, M. D., Long, F. & Vagin, A. A. (2011). Acta Cryst. D67, 355–367. Web of Science CrossRef CAS IUCr Journals Google Scholar
Nass, K. (2019). Acta Cryst. D75, 211–218. Web of Science CrossRef IUCr Journals Google Scholar
Neutze, R., Wouts, R., van der Spoel, D., Weckert, E. & Hajdu, J. (2000). Nature, 406, 752–757. Web of Science CrossRef PubMed CAS Google Scholar
Nogly, P., Weinert, T., James, D., Carbajo, S., Ozerov, D., Furrer, A., Gashi, D., Borin, V., Skopintsev, P., Jaeger, K., Nass, K., Båth, P., Bosman, R., Koglin, J., Seaberg, M., Lane, T., Kekilli, D., Brünle, S., Tanaka, T., Wu, W., Milne, C., White, T., Barty, A., Weierstall, U., Panneels, V., Nango, E., Iwata, S., Hunter, M., Schapiro, I., Schertler, G., Neutze, R. & Standfuss, J. (2018). Science, 361, eaat0094. Web of Science CrossRef PubMed Google Scholar
Olmos, J. L. Jr, Pandey, S., Martin-Garcia, J. M., Calvey, G., Katz, A., Knoska, J., Kupitz, C., Hunter, M. S., Liang, M., Oberthuer, D., Yefanov, O., Wiedorn, M., Heyman, M., Holl, M., Pande, K., Barty, A., Miller, M. D., Stern, S., Roy-Chowdhury, S., Coe, J., Nagaratnam, N., Zook, J., Verburgt, J., Norwood, T., Poudyal, I., Xu, D., Koglin, J., Seaberg, M. H., Zhao, Y., Bajt, S., Grant, T., Mariani, V., Nelson, G., Subramanian, G., Bae, E., Fromme, R., Fung, R., Schwander, P., Frank, M., White, T. A., Weierstall, U., Zatsepin, N., Spence, J., Fromme, P., Chapman, H. N., Pollack, L., Tremblay, L., Ourmazd, A., Phillips, G. N. Jr & Schmidt, M. (2018). BMC Biol. 16, 59. Google Scholar
Pande, K., Hutchison, C. D. M., Groenhof, G., Aquila, A., Robinson, J. S., Tenboer, J., Basu, S., Boutet, S., DePonte, D., Liang, M., White, T., Zatsepin, N., Yefanov, O., Morozov, D., Oberthuer, D., Gati, C., Subramanian, G., James, D., Zhao, Y., Koralek, J., Brayshaw, J., Kupitz, C., Conrad, C., Roy-Chowdhury, S., Coe, J. D., Metz, M., Xavier, P. L., Grant, T. D., Koglin, J. E., Ketawala, G., Fromme, R., Šrajer, V., Henning, R., Spence, J. C. H., Ourmazd, A., Schwander, P., Weierstall, U., Frank, M., Fromme, P., Barty, A., Chapman, H. N., Moffat, K., van Thor, J. J. & Schmidt, M. (2016). Science, 352, 725–729. Web of Science CrossRef CAS PubMed Google Scholar
Pandey, S., Bean, R., Sato, T., Poudyal, I., Bielecki, J., Cruz Villarreal, J., Yefanov, O., Mariani, V., White, T. A., Kupitz, C., Hunter, M., Abdellatif, M. H., Bajt, S., Bondar, V., Echelmeier, A., Doppler, D., Emons, M., Frank, M., Fromme, R., Gevorkov, Y., Giovanetti, G., Jiang, M., Kim, D., Kim, Y., Kirkwood, H., Klimovskaia, A., Knoska, J., Koua, F. H. M., Letrun, R., Lisova, S., Maia, L., Mazalova, V., Meza, D., Michelat, T., Ourmazd, A., Palmer, G., Ramilli, M., Schubert, R., Schwander, P., Silenzi, A., Sztuk-Dambietz, J., Tolstikova, A., Chapman, H. N., Ros, A., Barty, A., Fromme, P., Mancuso, A. P. & Schmidt, M. (2020). Nat. Methods, 17, 73–78. Web of Science CrossRef PubMed Google Scholar
Ramakrishnan, S., Stagno, J. R., Conrad, C. E., Ding, J., Yu, P., Bhandari, Y. R., Lee, Y. T., Pauly, G., Yefanov, O., Wiedorn, M. O., Knoska, J., Oberthür, D., White, T. A., Barty, A., Mariani, V., Li, C., Brehm, W., Heinz, W. F., Magidson, V., Lockett, S., Hunter, M. S., Boutet, S., Zatsepin, N. A., Zuo, X., Grant, T. D., Pandey, S., Schmidt, M., Spence, J. C. H., Chapman, H. N. & Wang, Y.-X. (2021). Nat. Commun. 12, 1762. Web of Science CrossRef PubMed Google Scholar
Ren, Z., Perman, B., Šrajer, V., Teng, T.-Y., Pradervand, C., Bourgeois, D., Schotte, F., Ursby, T., Kort, R., Wulff, M. & Moffat, K. (2001). Biochemistry, 40, 13788–13801. Web of Science CrossRef PubMed CAS Google Scholar
Schmidt, M. (2008). Ultrashort Laser Pulses in Medicine and Biology, edited by M. Braun, P. Gilch & W. Zinth, pp. 201–241. Berlin, Heidelberg, New York: Springer Google Scholar
Schmidt, M. (2013). Adv. Condens. Matter Phys. 2013, 1–10. Web of Science CrossRef Google Scholar
Schmidt, M. (2020). Crystals, 10, 116. Web of Science CrossRef Google Scholar
Schmidt, M., Rajagopal, S., Ren, Z. & Moffat, K. (2003). Biophys. J. 84, 2112–2129. Web of Science CrossRef PubMed CAS Google Scholar
Schmidt, M., Srajer, V., Henning, R., Ihee, H., Purwar, N., Tenboer, J. & Tripathi, S. (2013). Acta Cryst. D69, 2534–2542. Web of Science CrossRef IUCr Journals Google Scholar
Skopintsev, P., Ehrenberg, D., Weinert, T., James, D., Kar, R. K., Johnson, P. J. M., Ozerov, D., Furrer, A., Martiel, I., Dworkowski, F., Nass, K., Knopp, G., Cirelli, C., Arrell, C., Gashi, D., Mous, S., Wranik, M., Gruhl, T., Kekilli, D., Brünle, S., Deupi, X., Schertler, G. F. X., Benoit, R. M., Panneels, V., Nogly, P., Schapiro, I., Milne, C., Heberle, J. & Standfuss, J. (2020). Nature, 583, 314–318. Web of Science CrossRef CAS PubMed Google Scholar
Smith, T., Wolff, K. A. & Nguyen, L. (2013). Curr. Top. Microbiol. Immunol. 374, 53–80. Web of Science CAS PubMed Google Scholar
Sorigué, D., Hadjidemetriou, K., Blangy, S., Gotthard, G., Bonvalet, A., Coquelle, N., Samire, P., Aleksandrov, A., Antonucci, L., Benachir, A., Boutet, S., Byrdin, M., Cammarata, M., Carbajo, S., Cuiné, S., Doak, R. B., Foucar, L., Gorel, A., Grünbein, M., Hartmann, E., Hienerwadel, R., Hilpert, M., Kloos, M., Lane, T. J., Légeret, B., Legrand, P., Li-Beisson, Y., Moulin, S. L. Y., Nurizzo, D., Peltier, G., Schirò, G., Shoeman, R. L., Sliwa, M., Solinas, X., Zhuang, B., Barends, T. R. M., Colletier, J., Joffre, M., Royant, A., Berthomieu, C., Weik, M., Domratcheva, T., Brettel, K., Vos, M. H., Schlichting, I., Arnoux, P., Müller, P. & Beisson, F. (2021). Science, 372, eabd5687. Web of Science PubMed Google Scholar
Sorigué, D., Légeret, B., Cuiné, S., Blangy, S., Moulin, S., Billon, E., Richaud, P., Brugière, S., Couté, Y., Nurizzo, D., Müller, P., Brettel, K., Pignol, D., Arnoux, P., Li-Beisson, Y., Peltier, G. & Beisson, F. (2017). Science, 357, 903–907. Web of Science PubMed Google Scholar
Šrajer, V. & Schmidt, V. (2017). J. Phys. D Appl. Phys. 50, 373001. Web of Science PubMed Google Scholar
Stagno, J. R., Liu, Y., Bhandari, Y. R., Conrad, C. E., Panja, S., Swain, M., Fan, L., Nelson, G., Li, C., Wendel, D. R., White, T. A., Coe, J. D., Wiedorn, M. O., Knoska, J., Oberthuer, D., Tuckey, R. A., Yu, P., Dyba, M., Tarasov, S. G., Weierstall, U., Grant, T. D., Schwieters, C. D., Zhang, J., Ferré-D'Amaré, A. R., Fromme, P., Draper, D. E., Liang, M., Hunter, M. S., Boutet, S., Tan, K., Zuo, X., Ji, X., Barty, A., Zatsepin, N. A., Chapman, H. N., Spence, J. C. H., Woodson, S. A. & Wang, Y.-X. (2017). Nature, 541, 242–246. Web of Science CrossRef CAS PubMed Google Scholar
Takala, H., Björling, A., Berntsson, O., Lehtivuori, H., Niebling, S., Hoernke, M., Kosheleva, I., Henning, R., Menzel, A., Ihalainen, J. A. & Westenhoff, S. (2014). Nature, 509, 245–248. Web of Science CrossRef CAS PubMed Google Scholar
Tassoni, R., Blok, A., Pannu, N. S. & Ubbink, M. (2019). Biochemistry, 58, 997–1009. Web of Science CrossRef CAS PubMed Google Scholar
Tenboer, J., Basu, S., Zatsepin, N., Pande, K., Milathianaki, D., Frank, M., Hunter, M., Boutet, S., Williams, G. J., Koglin, J. E., Oberthuer, D., Heymann, M., Kupitz, C., Conrad, C., Coe, J., Roy-Chowdhury, S., Weierstall, U., James, D., Wang, D., Grant, T., Barty, A., Yefanov, O., Scales, J., Gati, C., Seuring, C., Srajer, V., Henning, R., Schwander, P., Fromme, R., Ourmazd, A., Moffat, K., Van Thor, J. J., Spence, J. C. H., Fromme, P., Chapman, H. N. & Schmidt, M. (2014). Science, 346, 1242–1246. Web of Science CrossRef CAS PubMed Google Scholar
Totir, M. A., Helfand, M. S., Carey, M. P., Sheri, A., Buynak, J. D., Bonomo, R. A. & Carey, P. R. (2007). Biochemistry, 46, 8980–8987. Web of Science CrossRef PubMed CAS Google Scholar
Tremblay, L. W., Xu, H. & Blanchard, J. S. (2010). Biochemistry, 49, 9685–9687. Web of Science CrossRef CAS PubMed Google Scholar
Tzeng, S. R. & Kalodimos, C. G. (2012). Nature, 488, 236–240. Web of Science CrossRef CAS PubMed Google Scholar
Vogt, A. D. & Di Cera, E. (2012). Biochemistry, 51, 5894–5902. Web of Science CrossRef CAS PubMed Google Scholar
Wanzenberg, R., Agapov, I., Brefeld, W., Brinkmann, R., Chae, Y., Chao, H., Keil, J., Gavaldà, X. N., Röhlsberger, R., Schroer, C. G., Tischer, M. & Weckert, E. (2019). AIP Conf. Proc. 2054, 030002. Google Scholar
White, T. A., Mariani, V., Brehm, W., Yefanov, O., Barty, A., Beyerlein, K. R., Chervinskii, F., Galli, L., Gati, C., Nakane, T., Tolstikova, A., Yamashita, K., Yoon, C. H., Diederichs, K. & Chapman, H. N. (2016). J. Appl. Cryst. 49, 680–689. Web of Science CrossRef CAS IUCr Journals Google Scholar
Wiedorn, M. O., Awel, S., Morgan, A. J., Ayyer, K., Gevorkov, Y., Fleckenstein, H., Roth, N., Adriano, L., Bean, R., Beyerlein, K. R., Chen, J., Coe, J., Cruz-Mazo, F., Ekeberg, T., Graceffa, R., Heymann, M., Horke, D. A., Knoška, J., Mariani, V., Nazari, R., Oberthür, D., Samanta, A. K., Sierra, R. G., Stan, C. A., Yefanov, O., Rompotis, D., Correa, J., Erk, B., Treusch, R., Schulz, J., Hogue, B. G., Gañán-Calvo, A. M., Fromme, P., Küpper, J., Rode, A. V., Bajt, S., Kirian, R. A. & Chapman, H. N. (2018). IUCrJ, 5, 574–584. Web of Science CrossRef CAS PubMed IUCr Journals Google Scholar
Wiedorn, M. O., Oberthür, D., Bean, R., Schubert, R., Werner, N., Abbey, B., Aepfelbacher, M., Adriano, L., Allahgholi, A., Al-Qudami, N., Andreasson, J., Aplin, S., Awel, S., Ayyer, K., Bajt, S., Barák, I., Bari, S., Bielecki, J., Botha, S., Boukhelef, D., Brehm, W., Brockhauser, S., Cheviakov, I., Coleman, M. A., Cruz-Mazo, F., Danilevski, C., Darmanin, C., Doak, R. B., Domaracky, M., Dörner, K., Du, Y., Fangohr, H., Fleckenstein, H., Frank, M., Fromme, P., Gañán-Calvo, A. M., Gevorkov, Y., Giewekemeyer, K., Ginn, H. M., Graafsma, H., Graceffa, R., Greiffenberg, D., Gumprecht, L., Göttlicher, P., Hajdu, J., Hauf, S., Heymann, M., Holmes, S., Horke, D. A., Hunter, M. S., Imlau, S., Kaukher, A., Kim, Y., Klyuev, A., Knoška, J., Kobe, B., Kuhn, M., Kupitz, C., Küpper, J., Lahey-Rudolph, J. M., Laurus, T., Le Cong, K., Letrun, R., Xavier, P. L., Maia, L., Maia, F., Mariani, V., Messerschmidt, M., Metz, M., Mezza, D., Michelat, T., Mills, G., Monteiro, D. C. F., Morgan, A., Mühlig, K., Munke, A., Münnich, A., Nette, J., Nugent, K. A., Nuguid, T., Orville, A. M., Pandey, S., Pena, G., Villanueva-Perez, P., Poehlsen, J., Previtali, G., Redecke, L., Riekehr, W. M., Rohde, H., Round, A., Safenreiter, T., Sarrou, I., Sato, T., Schmidt, M., Schmitt, B., Schönherr, R., Schulz, J., Sellberg, J. A., Seibert, M. M., Seuring, C., Shelby, M. L., Shoeman, R. L., Sikorski, M., Silenzi, A., Stan, C. A., Shi, X., Stern, S., Sztuk-Dambietz, J., Szuba, J., Tolstikova, A., Trebbin, M., Trunk, U., Vagovic, P., Ve, T., Weinhausen, B., White, T. A., Wrona, K., Xu, C., Yefanov, O., Zatsepin, N., Zhang, J., Perbandt, M., Mancuso, A. P., Betzel, C., Chapman, H. & Barty, A. (2018). Nat. Commun. 9, 4025. Web of Science CrossRef PubMed Google Scholar
Winn, M. D., Ballard, C. C., Cowtan, K. D., Dodson, E. J., Emsley, P., Evans, P. R., Keegan, R. M., Krissinel, E. B., Leslie, A. G. W., McCoy, A., McNicholas, S. J., Murshudov, G. N., Pannu, N. S., Potterton, E. A., Powell, H. R., Read, R. J., Vagin, A. & Wilson, K. S. (2011). Acta Cryst. D67, 235–242. Web of Science CrossRef CAS IUCr Journals Google Scholar
Yefanov, O., Mariani, V., Gati, C., White, T. A., Chapman, H. N. & Barty, A. (2015). Opt. Express, 23, 28459–28470. Web of Science CrossRef PubMed Google Scholar
Yefanov, O., Oberthür, D., Bean, R., Wiedorn, M. O., Knoska, J., Pena, G., Awel, S., Gumprecht, L., Domaracky, M., Sarrou, I., Lourdu Xavier, P., Metz, M., Bajt, S., Mariani, V., Gevorkov, Y., White, T. A., Tolstikova, A., Villanueva-Perez, P., Seuring, C., Aplin, S., Estillore, A. D., Küpper, J., Klyuev, A., Kuhn, M., Laurus, T., Graafsma, H., Monteiro, D. C. F., Trebbin, M., Maia, F. R. N. C., Cruz-Mazo, F., Gañán-Calvo, A. M., Heymann, M., Darmanin, C., Abbey, B., Schmidt, M., Fromme, P., Giewekemeyer, K., Sikorski, M., Graceffa, R., Vagovic, P., Kluyver, T., Bergemann, M., Fangohr, H., Sztuk-Dambietz, J., Hauf, S., Raab, N., Bondar, V., Mancuso, A. P., Chapman, H. & Barty, A. (2019). Struct. Dyn. 6, 064702. Web of Science CrossRef PubMed Google Scholar
Yun, J.-H., Li, X., Yue, J., Park, J.-H., Jin, Z., Li, C., Hu, H., Shi, Y., Pandey, S., Carbajo, S., Boutet, S., Hunter, M. S., Liang, M., Sierra, R. G., Lane, T. J., Zhou, L., Weierstall, U., Zatsepin, N. A., Ohki, M., Tame, J. R. H., Park, S. Y., Spence, J. C. H., Zhang, W., Schmidt, M., Lee, W. & Liu, H. (2021). Proc. Natl Acad. Sci. USA, 118, e2020486118. Web of Science CrossRef PubMed Google Scholar
Zaitsev-Doyle, J. J., Puchert, A., Pfeifer, Y., Yan, H., Yorke, B. A., Müller-Werkmeister, H. M., Uetrecht, C., Rehbein, J., Huse, N., Pearson, A. R. & Sans, M. (2019). RSC Adv. 9, 8695–8699. CAS Google Scholar

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Observation of substrate diffusion and ligand binding in enzyme crystals using high-repetition-rate mix-and-inject serial crystallography

1. Introduction

2. Methods

2.1. BlaC crystals

2.2. Data collection at the EuXFEL

2.3. Difference-map calculation and structure determination

2.4. Binding kinetics of CEF

2.5. The diffusion coefficient of CEF in the BlaC platelets

3. Results and discussion

3.1. Formation of the enzyme–substrate complex

3.2. Inhibitor binding

3.3. Diffusion of substrate in BlaC microcrystals

3.4. Reaction initiation by diffusion

4. Outlook

5. Summary

APPENDIX A

Microcrystals and data collection

APPENDIX B

Diffraction patterns and masks

Supporting information

Acknowledgements

Funding information

References

research papers