2.1. Crystallization

To create complexes of RoAb13 with each peptide, RoAb13 at 5, 8 and 10 mg ml⁻¹ in 20 mM HEPES pH 7.0, 0.1 M NaCl was incubated with 8 mM peptide in 0.1 M NaOH to give a final peptide concentration of ∼660 µM. Each peptide was incubated with RoAb13 for varying periods between 24 h and seven days before setting up crystallization trials.

RoAb13 complexed with each peptide was screened with Crystal Screen HT and Index (Hampton Research) in sitting-drop vapor-diffusion format using a Mosquito robot (TTP Labtech, UK). All screening trials used 400 nl drops comprised of a 1:1 ratio of protein solution and screen solution. The crystallization trials were incubated at 293 K.

Optimization trials with the 31-peptide complex at 5, 8 and 10 mg ml⁻¹ RoAb13 were set up at ammonium sulfate concentrations ranging between 1.5 and 3.0 M in increments of 0.5 M using both the hanging-drop vapor-diffusion and microbatch methods (Chayen et al., 1992; Chayen, 1997b) at 293 K. The hanging-drop vapor-diffusion trials were carried out using 15-well EasyXtal plates and EasyXtal X-seal screw lids (Qiagen, UK) inverted over 300 µl reservoir solution. Trials with the microbatch method were carried out by mixing equal volumes of the RoAb13–peptide complex and precipitant solutions in 72-well HLA plates from Douglas Instruments (UK) incubated under a layer of paraffin oil (VWR International).

Further fine-tuning of the conditions was performed for the 31-peptide complex with 8 and 10 mg ml^–1 RoAb13 and 1.5–2.0 M ammonium sulfate in increments of 0.1 M using the hanging-drop method. 10 µM nickel chloride was used as an additive in further optimization experiments using 1.8–2.0 M ammonium sulfate in steps of 0.05 M. In addition, a 200 µl oil barrier consisting of a 1:1 ratio of paraffin and silicone oils was introduced over the reservoir solution in the abovementioned conditions (Chayen, 1997a). A range of heterogeneous nucleants such as Naomi's nucleant (Khurshid et al., 2014), Chayen Reddy MIP (Saridakis & Chayen, 2013) and PEGylated Carbon Black (Govada et al., 2016) were also introduced in trials with the 31-peptide complex at 8 and 10 mg ml⁻¹ and 1.8 M ammonium sulfate. A single grain was introduced in the case of a solid nucleant and a tenth of the total drop volume was used in the case of a liquid nucleant (i.e. 0.2 µl of the nucleant in a 2 µl drop).

Trials with the 31-peptide complex were also optimized with 5 mg ml⁻¹ RoAb13 and 1.8–2.0 M ammonium sulfate in increments of 0.05 M by inducing nucleation in a controlled manner and arresting it before excess nucleation occurred (Govada & Chayen, 2009). 24 h after setting up the experiments, the screw caps of the 15-well EasyXtal plates were loosened for two hours by rotating them by 90° and were then resealed.

In the case of the short peptide (PIYDIN), 10 mg ml⁻¹ RoAb13 was incubated for 24 h with peptide stock and the optimization trials for this complex were set up with 1.8–2.0 M ammonium sulfate in increments of 0.05 M with and without 10 µM nickel chloride.

All optimization trials were performed manually and were observed over a four-week period.

Several soaking experiments were also performed with crystals obtained using 8–10 mg ml^–1 RoAb13 and 1.8–2.0 M ammonium sulfate. These crystals failed to diffract satisfactorily.

2.2. Data availability

RoAb13 co-crystallized with the 31 peptide (with the PIYDIN residues of the 31 peptide included in the model) was deposited in the Protein Data Bank (PDB) as entry 7njz. RoAb13 co-crystallized with PIYDIN was also deposited in the PDB as entry 7nw3. The diffraction images are available at Zenodo as run DLS i04 MX12579-11 Sample 4 (https://doi.org/10.5281/zenodo.4912886) and run DLS i04 MX17221-38 Sample 7 (https://doi.org/10.5281/zenodo.4916326).

3.1. Crystallization

Initial crystallization hits were produced with 2.0 M ammonium sulfate (Hampton Research Crystal Screen HT condition C8). Both RoAb13–peptide complexes, at an antibody concentration of 10 mg ml⁻¹, produced crystals one week after setting up the trials.

Conventional optimization produced crystals of RoAb13 complexed with the 31 peptide that diffracted to 7 Å resolution at 10 mg ml⁻¹ antibody, 2.0 M ammonium sulfate, 10 µM nickel chloride [Fig. 1(a)]. Crystals were obtained using both the hanging-drop and microbatch methods.

Figure 1 Crystals of RoAb13 complexed with (a) the 31 peptide and (b) the PIYDIN peptide.

A portfolio of crystallization methods of optimization, such as slowing down vapor diffusion with an oil barrier (Chayen, 1997a) and the use of Naomi's nucleant (Khurshid et al., 2014), Chayen Reddy MIP (Saridakis & Chayen, 2013) and PEGylated Carbon Black (Govada et al., 2016), showed considerable improvement in crystal diffraction from 7 to 4 Å for RoAb13 complexed with the 31 peptide. The best diffracting crystals (to ∼3.2 Å resolution) of the above complex at an initial concentration of 5 mg ml⁻¹ were obtained with 1.85 M ammonium sulfate after one week. This was achieved by the induction of nucleation and its subsequent arrest (Govada & Chayen, 2009).

In the case of RoAb13 complexed with PIYDIN at an initial concentration of 10 mg ml⁻¹, the best diffracting crystals (to 3.3 Å resolution) were produced with 1.8 M ammonium sulfate after four days in a hanging-drop vapor-diffusion setup [Fig. 1(b)].

3.2. X-ray crystallography

The crystals were cryoprotected with 20% glycerol and data were collected at 100 K on the I04 beamline at the Diamond Light Source (DLS) using a Dectris PILATUS 6M-F detector.

X-ray diffraction data sets were collected from crystals of the antibody co-crystallized with both the 31-residue (long) and the PIYDIN (short) peptides. Two crystals of the 31-peptide complex showed acceptable diffraction and the diffraction images were processed using iMosflm (Battye et al., 2011). The diffraction data were merged with POINTLESS and SCALA (Evans, 2006). An attempt was made to combine the data from the two best diffracting crystals, but an R_merge value in the strongest intensity bin of 11% was obtained, which is of course too large, even though the unit-cell parameters were quite similar (a = 76.44, b = 76.44, c = 268.64 and a = 76.53, b = 76.53, c = 269.07 Å). The R_merge values in the strongest intensity bin for each crystal individually were 4% and 6%. Keeping the two crystals separate proved an effective approach as comparisons of their omit electron-density maps showed reproducible extended electron density in the same location. (By `omit map', here and subsequently, we mean that the PIYDIN has not been included at this stage of each analysis.) Both crystals show some anisotropic diffraction, which was checked with the UCLA web server (Strong et al., 2006) and STARANISO (Tickle et al., 2018. Both analyses showed the diffraction resolution to be 3.5 × 3.5 × 2.7 Å with an 〈I/σ(I)〉 value of 1.5. Amongst many tests, an isotropic resolution cutoff of 3.2 Å proved to be optimal for model refinement. Based on the systematic absences, the space-group symmetry was determined as either P4₁2₁2 or P4₃2₁2. In the following, we describe structure solution and refinement using the data set from the slightly better diffracting crystal (Sample 4), which corresponds to the structure deposited in the PDB.

In molecular replacement using Phaser (McCoy et al., 2007), early attempts to place the heavy (H) and light (L) chains of the antibody using the RoAb13 model with PDB code 4s2s (Chain et al., 2015) did not lead to a satisfactory solution. However, when each of these chains was split into its variable (V) and constant (C) parts (leading to four chains for placement: HV, HC, LV and LC), Phaser yielded one clear solution with one copy of each chain in the asymmetric unit. REFMAC (Murshudov et al., 2011) and phenix.refine (Afonine et al., 2012) were used for restrained protein model refinement. Refinement with phenix.refine led to an R and R_free of 26.9% and 29.2%, respectively. We have deposited the refined structure in the PDB as entry 7njz (see Table 1). In the PDB validation report, several C-terminal residues have high RSRZ values, which is due to the intrinsic flexibility of this end of the polypeptide chains: 11.8 for Ile223H, 11.3 for Thr222H and 11.1 for Cys220L.

An X-ray diffraction data set for the PIYDIN co-crystallization was also collected at DLS and evaluated via its pipeline of data-processing software options. The data, collected to 3.2 Å resolution, were processed with XDS (Kabsch, 2010) and scaled with SCALA (Evans, 2006). Again, the crystal belonged to space group P4₁2₁2, with very similar unit-cell parameters a = b = 76.6, c = 270.1 Å.

Molecular replacement was attempted with both MOLREP and Phaser, again using PDB entry 4s2s as an initial model. Attempts to separately place the heavy and light chains of the antibody again did not lead to a satisfactory solution, but when each of these chains was split into its variable and constant parts Phaser yielded one clear solution with one copy of each chain in the asymmetric unit. Model refinement was undertaken with both REFMAC and phenix.refine for comparison purposes. Refinement with phenix.refine led to an R and R_free of 26.8% and 29.3%, respectively. We have deposited the refined structure in the PDB as entry 7nw3 (see Table 1).

Omit electron-density maps are shown in Fig. 2 for crystals from both the 31-peptide study and the PIYDIN study. These show the top difference peaks in the peaks list at 6σ, which are in the same location on the antibody surface (see Table 2). The binding site of PIYDIN also forms a crystal lattice contact with a neighboring protein molecule. The resolution of the data does not permit the accurate reporting of ligand–antibody interactions. However, we observe that in the case of the PIYDIN part of the 31 peptide, Pro8 of the ligand is near (approximately within 3.5 Å of) Tyr98 and Tyr100, Ile9 is near Gly218, and Ile12 is near Tyr98 of the light chain. Tyr10 of the ligand comes near Asp61 and Arg64 of the heavy chain. Asp11 is only engaged in intra-peptide interactions with Ile12 and Asn13. In the PIYDIN-only study, Ile9 additionally comes near Thr99 of the light chain (the corresponding distance is ∼5 Å for the 31-peptide structure). The ligand also approaches symmetry-related residues within the crystal lattice; however, as these belong to the flexible C-terminal tails of the heavy and light chains, which have a poor fit to the map, precision is largely lost (Table 2).

Figure 2 Omit electron-density maps are shown for (a) the PIYDIN residues of the 31-peptide study and (b) the PIYDIN-only study; orthogonal views are contoured at 2σ in (a) and 2.7σ in (b). (c) shows the overlay of both with the 31-peptide omit map at 2σ; the peptide does not have exactly the same placement but is very similar.