2.1. Preparing microcrystals

Equine hemoglobin (Sigma, CAS 9047-09-0) stock solution at 20–25 mg ml⁻¹ was prepared in 10 mM HEPES pH 7.5 and crystallized using the stirred batch method (Sato-Tomita & Shibayama, 2017) by mixing in precipitant solution [26%(v/v) PEG 3350, 10 mM HEPES pH 7.5]. At 20°C, 500 µl precipitant was added to 250 µl protein solution. The mixture was stirred in small HPLC vials with rice-grain-sized stir bars on a magnetic stirrer for about 20 h, after which crystals of 5 × 5 × 5 µm in size were obtained.

2.2. 3D-printed holder and accessories

Since handling this type of chip is challenging due to its small size and thinness, we have designed an assembling tool, a chip tray and a MX sample holder for easier manipulation. The MX sample holder was printed with Tough 1500 Resin (Formlabs, USA), while for the rest of the 3D-printed components Tough Resin V5 (Formlabs, USA) was used. The assembling tool went through a few iterations, as can be seen in Supplementary Fig. S1. The final iteration accounts for imperfections in chip size (some sides being longer or with `horns' in the edges), avoids too high pressure with the lever that would destroy the chips and leaves one corner easily accessible for handling upon assembly (Fig. 1a). Using the chip tray (Fig. 1b), several chips can be prepared for quicker assembly. To ease sample mounting to the goniometer head at MX beamlines, the MX sample holder was designed to be easily attached to SPINE bases (Cipriani et al., 2006; Fig. 1c). The tightening screws allow extra pressure to be applied to the sides of the sandwiched chips during data collection, further ensuring airtightness.

Figure 1 3D-printed accessories for SiN chip handling. (a) Assembling tool; (b) SiN chip tray; (c) MX sample holder.

2.3. Anaerobic chip assembly for X-ray crystallography

Before data collection, DeoxyHb crystals were freshly prepared inside a nitrogen-filled glovebox (Coy Laboratory Products). The average oxygen concentration in the glovebox was 2 p.p.m. during sample preparation and never went above 10 p.p.m.. The aerobically grown hemoglobin microcrystals were transferred into the glovebox and chemically reduced by mixing sodium dithionite solution [50 mM sodium dithionate, 26%(w/v) PEG 3350, 10 mM HEPES pH 7.5] (Vojtěchovský et al., 1999) with hemoglobin microcrystals (5 and 20 µl, respectively) and incubated within the glovebox at room temperature for 2 h (during which the crystal slurry undergoes a colour change from brown to pink). Inside the glovebox, SiN chips (membrane size 2.5 × 2.5 mm, membrane thickness 1000 nm, frame size 5.0 × 5.0 mm, frame thickness 200 µm; Silson, United Kingdom) were loaded onto the assembling tool (Figs. 2a and 2b), followed by the addition of 2 µl microcrystal slurry (Fig. 2c). To seal the chip, a small amount of superglue (Loctite Super Glue Brush On) was applied onto all four corners of the chip frame in an L-shape with a single hair from a small paintbrush (Fig. 2d). A second chip was then placed on the top (Fig. 2e) and pressed gently with the lever (Fig. 2f) to secure it and to create a seal, as confirmed by a tiny amount of glue overflowing along all edges. The assembled chip was then placed in the MX sample holder (Fig. 1c) for data collection.

Figure 2 Procedure for anaerobic chip assembly. (a) Assembling tool with chip tray. (b) The first chip is loaded into the assembling tool. (c) 2 µl of sample slurry is gently loaded onto the chip. (d) Small drops of superglue are added to all four corners of the chip. (e) A second chip is placed on top to create a sealed chip sandwich. (f) Chips are gently pressed with the lever of the assembling tool to secure the seal between them.

2.4. Anaerobic chip assembly for UV–Vis and X-ray absorption near-edge structure (XANES)

The purpose of the XANES experiment was to establish a time stamp to determine how long the chips can retain the deoxy­hemoglobin form. A special holder was designed to fit six chip sandwiches into the beamline sample environment setup (Supplementary Figs. S2b and S2c). The chips were assembled in the same way as described in Section 2.3.

UV–Vis spectroscopy using the MX sample holder, with the chip prepared in the exact same way as for X-ray crystallo­graphic data collection, was carried out with an Agilent Cary 60 UV–Vis spectrophotometer in the wavelength range 300–800 nm and followed over 2 h. The UV–Vis spectrophoto­meter was modified with an external optical cable with a probe leading to a black box with a holder for the MX sample holder.

2.5. Data collection

2.6. Data processing, model building and refinement

Diffraction data were indexed, integrated, merged and converted to MTZ format using CrystFEL 0.10.1 (White, 2019; White et al., 2012). The indexing rates were 43.3% and 53.6% for MetHb and DeoxyHb, respectively. Data truncation, phasing and structure refinement were performed in CCP4 Cloud (Krissinel et al., 2022; Agirre et al., 2023). High-resolution structures of DeoxyHb (PDB entry 1ibe; Wilson et al., 1996) and MetHb (PDB entry 6sva; Mikolajek et al., 2023) were used as models for molecular replacement with Phaser (McCoy et al., 2007). The structures were refined by one round of rigid-body refinement using REFMAC5 (Nicholls et al., 2018; Murshudov et al., 1997, 2011) followed by several rounds of restrained refinement. Model building was performed in Coot (Emsley et al., 2010; Krissinel & Henrick, 2004) and all structural representations were generated in PyMOL (Schrödinger). Room-temperature SSX structures of MetHb and DeoxyHb were obtained at 1.95 and 1.85 Å resolution, respectively. Data-collection and refinement statistics are presented in Table 1. The DeoxyHb chips were also processed and refined separately to investigate them individually (data-collection and refinement statistics are presented in Supplementary Table S1).

Table 1 Data-collection and refinement statistics Values in parentheses are for the highest resolution shell.   MetHb DeoxyHb PDB code 8puq 8pur Data collection  Diffraction source BioMAX, MAX IVLaboratory BioMAX, MAX IVLaboratory  Wavelength (Å) 0.9763 0.9763  Temperature (K) 294 294  Space group C121 C121  a, b, c (Å) 108.29, 63.06, 54.75 108.29, 63.06, 54.75  α, β, γ (°) 90, 111, 90 90, 111, 90  Resolution (Å) 53.55–1.95 (2.02–1.95) 53.50–1.85 (1.91–1.85)  Rsplit† (%) 7.50 (41.94) 6.71 (22.28)  〈I/σ(I)〉 10.60 (1.37) 12.48 (2.90)  CC1/2 0.9903 (0.7593) 0.9914 (0.9049)  Completeness (%) 100 (100) 100 (100)  Multiplicity 176 (114) 205 (115)  Collected images 97424 149207  Indexed patterns 42148 80035  Indexing rate (%) 43.3 53.6  No. of reflections 4447049 6070870  No. of unique reflections 25258 29515 Refinement      Resolution range (Å) 53.49–1.95 53.50–1.85  Rwork/Rfree (%) 12.52/17.41 12.99/16.22  No. of atoms 4644 4609  Average B factor (Å2) 66 74  R.m.s.d., bond lengths (Å) 0.016 0.015  R.m.s.d., angles (°) 1.97 1.99 †Rsplit =

3.1. Structural differences between deoxy and met forms

The α-subunits of DeoxyHb have a water molecule in the heme pocket about 3 Å (3.1 Å in this case) from the iron and hydrogen-bonded to the distal histidine (Fig. 3). In MetHb the α- and β-heme groups have a water molecule as the sixth ligand, approximately 2 Å (2.2 Å in this case) from the iron (Fig. 4). When hemoglobin changes from the deoxy form to the oxy or met form there is no significant change in the inner region of the α1β1/α2β2 dimer. Visible changes are present in the outer region of the dimer and in the dimer-interface area. The interaction between α1β2 and α2β1 moves towards the centre of the molecule. Residues in contact in the αβ interfaces are between αB (Glu30/A–Phe36/A) and βH (Phe122/B–Lys132/B), αG (Ser102/A–Leu113/A) and βG (Gly107/B–Phe118/B), and αH (Phe117/A–Lys127/A) and βB (Arg30/B–Pro36/B). The most noticeable movement is at the β-heme, where a water molecule is bound in MetHb compared with the empty β-heme in DeoxyHb. The β-heme of MetHb moves downwards to the proximal side of the heme pocket (Supplementary Fig. S3). Both structures are in agreement with published structures (Baldwin & Chothia, 1979; Liddington et al., 1992; Wilson et al., 1996).

Figure 3 View of the final 2mFo − DFc electron-density map for the heme pockets of DeoxyHb: (a) the α subunit and (b) the β subunit. Density is contoured at 1.1σ. The distance between His58/63 and the heme iron is 4.2 Å, while the distance between the water molecule and the heme iron is 3.1 Å

Figure 4 View of the final 2mFo − DFc electron-density map for the heme pockets of MetHb: (a) the α subunit and (b) the β subunit. Density is contoured at 1.1σ. The distance between His58/63 and the heme iron is 4.1 Å, while the distance between the water molecule and the heme iron is 2.1 Å

All five chips with DeoxyHb that were also independently processed exhibited the presence of the deoxy state (Supplementary Table S1 and Supplementary Figs. S12–S15), with the exception of chip 3 that contained a bubble following the preparation, resulting in too few indexed images for a separate analysis.

3.2. XANES data

From the preliminary test of the chip sandwiches with an X-ray beam at the Balder beamline, we learned that the Fe K edge shifts after long exposure (60 s). The position of the Fe K edge shifted to higher energy after the first scan (30 s), and by the second XANES scan the edge had already approached the position for fully oxygenated hemoglobin. This fact was used in a strategy to find out how long the chip seal lasts under ambient conditions in air by waiting 20 min between starting to scan each of the consecutive chip sandwiches, i.e. only the first scan of each chip was compared (10 s to reach the edge, 23 s full scan). XANES data for the six individual chip sandwiches mounted in the chip holder made for the Balder beamline showed that two of the chip sandwiches (chips 3 and 4) had intact seals when the measurement started (i.e. were still in the deoxy state; Supplementary Fig. S4), as their absorption edges were not shifted to higher energy as observed on O₂ binding. This gave us a time stamp for the seal of at least 40 min (the time between the start of scan 1 of chip 2 and of chip 4). Fig. 5 shows a comparison of the edge position of chip 4 upon the first scan and the second scan with the deoxy and oxy states, respectively. The conclusion from this comparison is that only the first scan of chip 4 (black dashed line) had an edge position corresponding to the hemoglobin deoxy state (blue line), while the second scan (grey dashed line) had already shifted to the position of the oxygenated state (red line).

Figure 5 The Fe K-edge XANES of hemoglobin crystals in the deoxy state (blue, single scan) and in the fully oxygenated state (red) compared with crystals in SiN chip 4: first scan (black dashed line) and second scan (grey dashed line). Inset, a close-up view of the edge position from the area marked with a grey rectangle in the main figure.

3.3. UV–Vis data

Chips were prepared as described in Section 2.3. The samples in both chips measured stayed pink, and neither chip changed from the deoxy to the met form in the first 30 min according to the spectra (Fig. 6 and Supplementary Fig. S11). The second chip was also measured 1 h 30 min and 2 h 10 min after the start of the experiment (Supplementary Fig. S11). These later time points show a change from the deoxy form, which could also be seen by eye as the sample colour changed from pink to brown.

Figure 6 UV–Vis spectra of a chip sandwich (chip 1) with DeoxyHb in the MX sample holder (the spectra have been normalized in Origin 2018b).