Parasite material

Onchocerca ochengi adult female gravid worms were collected from nodules in hides of infected Gudali cattle from the Ngaoundéré abattoir in the Adamawa region of Cameroon. Worm masses were dissected from collagenous tissue within nodules and male worms were removed. The females were washed in PBS and separated into 2 mL cryovial tubes before freezing and storage at −80 °C. Isolated female worms were transported to the UK on dry ice.

Glutathione transferase purification

Cytosolic extracts from O. ochengi were obtained by homogenization of frozen worms in an ice-cooled glass grinder in buffer containing 20 mm potassium phosphate, pH 7.0, 0.2% Triton X-100, 5 mm DTT and a cocktail of protease inhibitors (Roche, Mini-Complete, EDTA-free). Following homogenization, samples were centrifuged at 100 000 × g for 1 h at 4 °C and the supernatant, termed the cytosolic fraction, was retained for purification of GSTs.

GSTs were partially purified and further resolved to isolate glycosylated forms from the cytosolic fraction in two steps; ‘Step 1’ employed S-hexylglutathione-affinity (S-hexylGSH-affinity) chromatography according to the adapted method of (Simons and Vander Jagt, Reference Simons and Vander Jagt1977). In brief, the O. ochengi cytosolic fraction was passed at 0.5 mL min⁻¹ through Econo-columns (1.0 × 5 cm, 4 mL Bio-Rad, U.K.), containing 1 mL of S-hexylGSH–agarose (Sigma Aldrich), re-hydrated according to manufacturer's instructions and equilibrated with 20 mL of 20 mm potassium-phosphate buffer pH 7.0, 50 mm NaCl (equilibration buffer). Non-S-hexylGSH-affinity proteins were washed from the column with 20 mL equilibration buffer at 0.5 mL min⁻¹. Affinity-bound proteins were eluted in 3 mL 50 mm Tris-HCl pH 8.0 buffer, containing 2 mm S-hexylGSH, and concentrated via centrifugal filtration in 10 kDa molecular weight cut off filters (Amicon Ultra-4, Millipore). GST samples were reduced to a final volume of 100 µL through three successive cycles of ten-fold dilutions/centrifugal reductions in 50 mm Tris-HCl pH 8.0 to remove proteins, free glutathione and low molecular mass substances of a native weight below 10 kDa.

The partially purified pool of GSTs obtained in ‘Step 1’ was incubated with a range of different lectins to determine optimum lectin selection for ‘Step 2’ isolation of glycosylated GST from the GST pool. Glycosylated GSTs were isolated from the partially purified pool of GSTs obtained in ‘Step 1’ via lectin-affinity chromatography using concanavalin A-agarose (Sigma Aldrich) according to the manufacturer's instructions.

Glutathione transferase enzyme activity

Establishment of GST presence within O. ochengi cytosolic extracts and S-hexylglutathione-binding protein samples was assayed via enzyme activity at 25 °C over 3 min at 340 nm using 1 mm 1-chloro-2, 4-dinitrobenzene (CDNB) as standard second substrate in 100 mm potassium phosphate pH 6.5, containing 1 mm reduced glutathione in accordance with the adapted method of Habig et al. (Reference Habig, Pabst and Jakoby1974). Assays were undertaken in triplicate in a Cary Varian spectrophotometer with specific activity expressed as nmol GSH/CDNB conjugated min^-1 mg^-1 protein (± standard deviation), and calculated as described by (Barrett, Reference Barrett and Rogan1997) (see equation (1) below):

(1)$$\eqalign{& \displaystyle{{\Delta {\rm OD}} \over {\varepsilon \times t}} \times V{\rm \times} L\displaystyle{1 \over {\Pr}} \times \displaystyle{1 \over S} \times 10^n \cr & = {\rm Specific}\,{\rm Activity}\,{\rm (nmol}{\rm. mi}{\rm n}^{-1}.\,{\rm mg}\,{\rm protei}{\rm n}^{-1})}$$

Key to equation (1). ΔOD = change in optical density over time (t) in min; ε = extinction coefficient; V = total volume of assay mixture in the cuvette (mL); L = path length of the cuvette in cm; Pr = protein concentration of enzyme extract (mg mL⁻¹); S = volume of enzyme extract added to a cuvette (mL); The value of n is dependent on the extinction coefficient (ε): If ε is in cm² M⁻¹, then n = 9, If ε is in M⁻¹ cm⁻¹, then n = 6, If ε is in mm⁻¹ cm⁻¹, then n = 3)

Protein concentrations were estimated via the adapted method of Bradford (Bradford, Reference Bradford1976) using the Sigma (UK) Bradford Reagent protocol according to the manufacturer's instructions.

Electrophoresis

Quadrupole time of flight (QToF) tandem mass spectrometry (MS/MS) analysis of OoGST peptides

Tryptic peptides were generated as previously described (LaCourse et al., Reference LaCourse, Hernandez-Viadel, Jefferies, Svendsen, Spurgeon, Barrett, Morgan, Kille and Brophy2009). Peptide mixtures from trypsin digested gel spots were separated using an LC Packings Ultimate nano-HPLC System. Sample injection was via an LC Packings Famos auto-sampler and the loading solvent was 0.1% formic acid. The pre-column used was an LC Packings C18 PepMap 100, 5 mm, 100A and the nano HPLC column was an LC Packings PepMap C18, 3 mm, 100A. The solvent system was: solvent A 2% ACN with 0.1% formic acid, and solvent B, 80% ACN with 0.1% formic acid. The LC flow rate was 0.2 mL min⁻¹. The gradient employed was 5% solvent A to 100% solvent B in 1 h. The HPLC eluent was sprayed into the nano-ES source of a Waters Q-TOFμ MS via a New Objective Pico-Tip emitter. The MS was operated in the positive ion ES mode and multiple charged ions were detected using a data-directed MS-MS experiment. Collision induced dissociation (CID) MS-MS mass spectra were recorded over the mass range m/z 80–1400 Da with scan time 1 s. The raw MS-MS spectral data files were processed using Waters ProteinLynx software (Waters, UK) to produce Sequest dta file lists which were then merged into a Mascot generic format (mgf) file.

Protein identification

All tandem MS data generated were searched against partially revised Onchocerca ochengi gene models based on data downloaded from WormBase ParaSite (Armstrong et al., Reference Armstrong, Xia, Bah, Krishna, Ngangyung, LaCourse, McSorley, Kengne-Ouafo, Chounna-Ndongmo, Wanji, Enyong, Taylor, Blaxter, Wastling, Tanya and Makepeace2016) and a Bos taurus reference proteome (UniProt UP000009136, March 2019) (37957 sequences, 17775113 residues in total) using the search engine MASCOT (version 2.3.02, Matrix science) Search parameters were a precursor mass tolerance of ±1.2 Da and fragment mass tolerance of ±0.6 Da. One missed cleavage was permitted, carbamidomethylation was set as a fixed modification and oxidation (M) and deamidation (N, Q) were included as variable modifications. Individual ion scores ⩾39 were considered to indicate identity or extensive homology (P < 0.05), using MudPIT scoring. Only proteins with >2 peptides were used for analysis. Data were deposited to the PRIDE repository (Vizcaino et al., Reference Vizcaino, Csordas, del-Toro, Dianes, Griss, Lavidas, Mayer, Perez-Riverol, Reisinger, Ternent, Xu, Wang and Hermjakob2016) with the data set identifier PXD013440.

Glycan analysis of O. ochengi σ class GST

Glycan structural analysis

N-glycans from OoGST were released by PNGase F and purified by gel filtration chromatography as indicated in Kozak et al., Reference Kozak, Tortosa, Fernandes and Spencer2015. Hydrophilic Interaction Liquid Chromatography – Ultra high-performance liquid chromatography (HILIC-UHPLC) analysis was performed using a Dionex Ultimate 3000 UHPLC instrument. The conditions included using a BEH-Glycan 1.7 32 µm and 2.1 × 150 mm column at 40 °C, with a fluorescence detector (lamdaex = 310 nm and lamdaem = 370 nm). These conditions were controlled by Bruker HyStar 3.2 buffer A (50 mm ammonium formate pH 4.4) and Buffer B (acetonitrile). Sample volume for injection was 25 µL⁻¹, at a ratio of 24 and 76% acetonitrile. Glucose unit (GU) values of peaks were assigned by chromeleon 7.2 data software with a cubic spline fit. The system standard and the GU calibration standard was a glucose homopolymer labelled with procainamide. The mass spectra were collected in a Bruker AmaZon Speed ETD electrospray mass spectrometer, performed immediately after the UHPLC fluorescence detector without splitting. Samples were scanned in maximum resolution mode, positive ion settings, MS scan + three MS/MS scans. The MS/MS scans were done on three ions in each scan sweep with a mixing time of 40 ms at a nebulizer pressure of 14.5 psi, a nitrogen flow of 10 litres min⁻¹ and using 4500 V capillary voltage.

Prostaglandin-synthase assay

Prostaglandin synthase activity was assessed via the composite method of LaCourse et al. (Reference LaCourse, Perally, Morphew, Moxon, Prescott, Dowling, O'Neill, Kipar, Hetzel, Hoey, Zafra, Buffoni, Perez Arevalo and Brophy2012) based upon aspects adapted from the original methods of Sommer et al. (Reference Sommer, Rickert, Fischer, Steinhart, Walter and Liebau2003), Meyer and Thomas (Reference Meyer and Thomas1995) and Meyer et al. (Reference Meyer, Muimo, Thomas, Coates and Isaac1996), with extraction modifications based upon Schmidt et al. (Reference Schmidt, Coste and Geisslinger2005).

Sequence analysis of O. ochengi glycosylated glutathione transferase OoGST1

Onchocerca ochengi glycosylated σ-class GST (OoGST1) amino acid sequence (accession number nOo.2.0.1.t09064) was obtained from the University of Edinburgh's O. ochengi genome assembly v. nOo.2.0.1 hosted by WormBase ParaSite (Howe et al., Reference Howe, Bolt, Shafie, Kersey and Berriman2017; Consortium, Reference Consortium2019). Onchocerca ochengi GST Oo_GST_t09064 was aligned to highlight key residues involved in prostaglandin H₂ binding using ClustalX Version 2.1 (Thompson et al., Reference Thompson, Gibson, Plewniak, Jeanmougin and Higgins1997; Larkin et al., Reference Larkin, Blackshields, Brown, Chenna, McGettigan, McWilliam, Valentin, Wallace, Wilm, Lopez, Thompson, Gibson and Higgins2007) with homologues Ov_GST_Ia (AAG44695.1) and Ov_GST_Ib (AAG44696.1) from O. volvulus along with the two mammalian haematopoietic prostaglandin D synthases (PGDS), highlighted in Perbandt et al., Reference Perbandt, Hoppner, Burmeister, Luersen, Betzel and Liebau2008.

Structural analysis of OoGST1

Initial protein tertiary models of O. ochengi σ class GST were produced in silico using SwissModel (Arnold et al., Reference Arnold, Bordoli, Kopp and Schwede2006) and Phyre2 (Kelley et al., Reference Kelley, Mezulis, Yates, Wass and Sternberg2015) with prostaglandin D synthase of O. volvulus (Protein Data Bank (PBD) 2HNL) used as a template structure. Homology prediction was also carried out by RaptorX (Kallberg et al., Reference Kallberg, Wang, Wang, Peng, Wang, Lu and Xu2012) to predict disordered amino acid regions and I-Tasser (Yang et al., Reference Yang, Yan, Roy, Xu, Poisson and Zhang2015) for increased confidence before refinement of the predicted model via ModRefiner (Xu and Zhang, Reference Xu and Zhang2011). Final structures were modified in PyMol (DeLano, Reference DeLano2002).