Combining X-Ray Crystallography with Small Angle X-Ray Scattering to Model Unstructured Regions of Nsa1 from S. Cerevisiae

Podsumowanie

This method describes the cloning, expression, and purification of recombinant Nsa1 for structural determination by X-ray crystallography and small-angle X-ray scattering (SAXS), and is applicable for the hybrid structural analysis of other proteins containing both ordered and disordered domains.

Streszczenie

Determination of the full-length structure of ribosome assembly factor Nsa1 from Saccharomyces cerevisiae (S. cerevisiae) is challenging because of the disordered and protease labile C-terminus of the protein. This manuscript describes the methods to purify recombinant Nsa1 from S. cerevisiae for structural analysis by both X-ray crystallography and SAXS. X-ray crystallography was utilized to solve the structure of the well-ordered N-terminal WD40 domain of Nsa1, and then SAXS was used to resolve the structure of the C-terminus of Nsa1 in solution. Solution scattering data was collected from full-length Nsa1 in solution. The theoretical scattering amplitudes were calculated from the high-resolution crystal structure of the WD40 domain, and then a combination of rigid body and ab initio modeling revealed the C-terminus of Nsa1. Through this hybrid approach the quaternary structure of the entire protein was reconstructed. The methods presented here should be generally applicable for the hybrid structural determination of other proteins composed of a mix of structured and unstructured domains.

Wprowadzenie

Ribosomes are large ribonucleoprotein machines that carry out the essential role of translating mRNA into proteins in all living cells. Ribosomes are composed of two subunits which are produced in a complex process termed ribosome biogenesis^1,2,3,4. Eukaryotic ribosome assembly relies on the aid of hundreds of essential ribosomal assembly factors^2,3,5. Nsa1 (Nop7 associated 1) is a eukaryotic ribosome assembly factor that is specifically required for the production of the large ribosomal subunit⁶, and is known as WD-repeat containing 74 (WDR74) in higher organisms⁷. WDR74 has been shown to be required for blastocyst formation in mice⁸and the WDR74 promoter is frequently mutated in cancer cells⁹. However, the function and precise mechanisms of Nsa1/WDR74 in ribosome assembly are still largely unknown. To begin to uncover the role of Nsa1/WDR74 during eukaryotic ribosome maturation, multiple structural analyses were performed, including X-ray crystallography and small angle X-ray scattering (SAXS)¹⁰.

X-ray crystallography, nuclear magnetic resonance (NMR) spectroscopy, electron microscopy, and SAXS are all important techniques for studying macromolecular structure. Size, shape, availability, and stability of macromolecules influences the structural biology method for which a particular macromolecule will be best suited, however combining multiple techniques through a so-called "hybrid" approach is becoming an increasingly beneficial tool¹¹. In particular X-ray crystallography and SAXS are powerful and complementary methods for structural determination of macromolecules¹².

Crystallography provides high-resolution atomic structures ranging from small molecules to large cellular machinery such as the ribosome, and has led to numerous breakthroughs in the understanding of the biological functions of proteins and other macromolecules¹³. Furthermore, structure-based drug design harnesses the power of crystal structures for molecular docking by computational methods, adding a critical dimension to drug discovery and development¹⁴. Despite its broad applicability, flexible and disordered systems are challenging to assess by crystallography since crystal packing can be hindered or electron density maps may be incomplete or of poor quality. Conversely, SAXS is a solution-based and low-resolution structural approach capable of describing flexible systems ranging from disordered loops and termini to intrinsically disordered proteins^12,15,16. Considering it is compatible with a broad range of particle sizes¹², SAXS can work synergistically with crystallography to expand the range of biological questions that can be addressed by structural studies.

Nsa1 is suitable for a hybrid structural approach because it contains a well-structured WD40 domain followed by a functional, but flexible C-terminus which is not amenable to X-ray crystallography methods. Following is a protocol for the cloning, expression, and purification of S. cerevisiae Nsa1 for hybrid structural determination by X-ray crystallography and SAXS. This protocol can be adapted to study the structures of other proteins that are comprised of a combination of ordered and disordered regions.

Protokół

1. Recombinant Protein Production and Purification of Nsa 1

1. Nsa1 Expression Plasmid Design and Cloning
   1. Obtain or purchase S. cerevisiae genomic DNA.
   2. PCR amplify the target sequences of Nsa1 (Nsa1_FL, residues 1-463) and C-terminal truncated Nsa1 (Nsa1_ΔC, residues 1-434) with appropriate primers using genomic DNA isolated from S. cerevisiae and a melting temperature of approximately 60 °C with an extension time of 1-2 min. The following primers were used to amplify Nsa1:
      SC_Nsa1_FLFw:CGCCAAAGGCCTATGAGGTTACTAGTCAGCTGTGTGGATAG
      SC_Nsa1_FLRv:AATGCAGCGGCCGCTCAAATTTTGCTTTTCTTACTGGCTTTAGAAGCGC
      SC_Nsa1_ΔcFw:GGGCGCCATGGGATCCATGAGGTTACTAGTCAGCTGTGTGG
      SC_Nsa1_ΔcRv: GATTCGAAAGCGGCCGCTTAAACCTTCCTTTTTTGCTTCCC
   3. Subclone Nsa1 into the Escherichia coli (E. coli) expression vector pHMBP containing an N-terminal 6X-Histidine tag followed by the Maltose Binding Protein (MBP) and a Tobacco Etch Virus (TEV) protease site using standard cloning techniques¹⁷.
   4. Use DNA sequencing to verify that Nsa1 was cloned in frame with the N-terminal His-MBP tag.
2. Nsa1 Protein Expression
   1. Transform the expression plasmid(s) into a suitable E. coli expression strain with a T7 promoter-based system. Plate the transformants on LB agar plates containing 100 µg/mL ampicillin and incubate the plate inverted overnight at 37 °C.
   2. Inoculate a 50 mL culture of LB with 100 µg/mL ampicillin from the transformation plate, and grow it overnight with shaking at 200 rpm at 37 °C.
   3. Inoculate 3 x 1000 mL of LB in Fernbach flasks with 100 µg/mL ampicillin with 15 mL of the overnight culture and grow it with shaking at 200 rpm at 37 °C.
      NOTE: For protein structure solution, selenomethionyl (SeMet) incorporation can be achieved by growing cells in M9 minimal medium that is supplemented with SeMet and an amino acid mixture to inhibit methionine production prior to induction, as opposed to LB media¹⁸.
   4. Induce expression of Nsa1 when the OD₆₀₀ reaches ~0.8 by addition of isopropyl β-D-1 thiogalactopyranoside (IPTG) at a final concentration of 1 mM followed by incubation at 25 °C overnight with shaking at 200 rpm.
   5. Harvest cells by centrifugation at 4 °C for 15 min at 5,050 x g.
      NOTE: Cells can be stored long-term at -80 °C or used immediately for protein purification.
3. Nsa1 Protein Purification
   1. Resuspend the cells in 25 mL of Lysis buffer (50 mM Tris-HCl, pH 7.5, 500 mM NaCl, 10% glycerol, 10 mM MgCl₂) pre-chilled at 4 °C containing one EDTA-free protease inhibitor tablet.
   2. Lyse cells by sonication at 4 °C (time 7 min, 2 s on cycle, 2 s off cycle; amplitude: 70%).
   3. Clarify lysate by centrifugation at 26,900 x g for 45 min at 4 °C.
   4. Apply clarified lysate to a gravity flow column loaded with 10 mL of immobilized cobalt affinity resin, pre-equilibrated with Lysis buffer.
   5. Allow the supernatant to pass over the resin by gravity flow at 4 °C and wash the resin twice with 100 mL of Lysis buffer.
   6. Elute Nsa1 with 20 mL of Elution buffer (50 mM Tris-HCl pH 7.5, 500 mM NaCl, 5 mM MgCl₂, 5% glycerol and 200 mM imidazole).
   7. Take 15 μL of the eluate and run it on a 4-15% SDS-PAGE gel to verify that the protein is eluted from the affinity resin (Figure 1A).
   8. Remove the MBP tag by TEV protease digestion. Add 1 mL of TEV protease¹⁹ (1 mg/mL stock) to the Nsa1 affinity resin elution and incubate it at 4 °C overnight.
   9. Concentrate MBP cleaved Nsa1 to ~ 5 mL using a centrifugal filter with a molecular weight cut off of 10 kDa.
   10. Apply MBP-cleaved Nsa1 to a gel-filtration column, pre-equilibrated in buffer A (20 mM Tris-HCl pH 7.5, 100 mM NaCl, 1 mM MgCl₂, 5% glycerol and 1 mM β-mercaptoethanol) (Figure 1B).
   11. Analyze column fractions from gel filtration to verify that MBP is cleaved and separated from Nsa1 by running 15 μL samples on a 4-15% SDS-PAGE gel (Figure 1B).
   12. Combine fractions containing Nsa1 and concentrate to 8 mg/mL using a centrifugal filter with a molecular weight cut off of 10 kDa.
   13. Determine the protein concentration by measuring the absorbance at 280 nm on a spectrophotometer using the extinction coefficient 42530 M^-1cm^-1. Use protein immediately for proteolytic screening and crystallization trials.

2. Crystallization and Proteolytic Screening of Nsa 1

1. Sparse Matrix Crystal Screening of Nsa1
   1. Centrifuge 500 μL of the 8 mg/mL stock of Nsa1 at 16,000 x g at 4 °C for 10 min.
   2. Setup crystallization trials using a crystallization robot and sparse matrix crystal screens. Fill the reservoir of 96 well trays with 30 μl of the individual crystal screen reagents from sparse matrix crystallization screens. Setup sitting drops with the robot by mixing 250 nL of the well solution with 250 nL of the protein solution.
   3. Seal the crystallization plates with tape and incubate them at 25 °C.
   4. Inspect the plates every two days for the first 2-3 weeks with a stereomicroscope.
   5. Verify that potential crystals hits contain protein with a UV microscope.
      NOTE: For Nsa1 two different crystal forms (cubic and orthorhombic, Figure 2A) were obtained within 1 week from the following screens: JCSG+ condition B11 (1.6 M sodium citrate tribasic dehydrate, pH 6.5) and Wizard Precipitant Synergy Screen Block 2 condition C11 (20.1%(v/v) PEG 1500, 13.4%(v/v) PEG 400, 0.1 M Tris HEPES/sodium hydroxide, pH 7.5).
2. Proteolytic Screening
   NOTE: During crystallization optimization, it was discovered that the orthorhombic crystals of Nsa1 arose as a result of proteolytic cleavage and the crystals could not be duplicated using the full-length protein. Using a combination of limited proteolysis coupled with mass spectrometry, it was determined that the C-terminus of Nsa1 was sensitive to proteolysis and removal of the C-terminal tail was required for subsequent reproduction of the orthorhombic crystal form (Nsa1_ΔC).
   1. Prepare 1 mg/mL protease stock solutions of the following proteases α-chymotrypsin, trypsin, elastase, papain, subtilisin, and endoproteinase Glu-C.
   2. Create 1:10, 1:100, and 1:1000 dilutions of each 1 mg/mL protease stock with Dilution Buffer (10 mM HEPES, pH 7.5, 500 mM sodium chloride).
   3. Pipette 1 μL of protease stock (1:10, 1:100 and 1:1000) into 9 μL aliquots of protein (1 mg/mL) for each protease to be screened.
   4. Incubate the solution at 37 °C for 1 h.
   5. Stop the reaction by adding 10 μL of 2x SDS-PAGE sample buffer and heat the reaction at 95 °C for 5 min.
   6. Analyze the digests by running them on a 4-15% SDS-PAGE gel (Figure 2B).
   7. Identify protease resistant domains of the target protein by in-gel mass spectrometry analysis.
   8. Remove the protease-labile regions from the target protein by creating truncated expression constructs and following the cloning, expression, and purification protocol described above.
3. Crystallization Optimization
   1. Prepare or obtain stock solutions of the following initial crystallization reagents: 1.6 M sodium citrate tribasic dehydrate pH 6.5, 100%(v/v) PEG 400, 50%(v/v) PEG 1500, 1 M HEPES/sodium hydroxide, pH 7.5.
   2. Prepare a stock solution of Nsa1_FL and Nsa1_ΔC at 8 mg/mL as described above.
   3. Optimize the Nsa1 cubic crystals (Nsa1_FL).
      1. Prepare a 24-well grid screen with wells containing 500 µL with a gradient of 1-1.6 M of sodium citrate with pH 6.5 from a stock solution of 1.6 M sodium citrate tribasic with pH 6.5.
      2. Mix 1 µL of protein with 1 µL of well solution and place the mixture onto a siliconized cover slide. Carefully invert the cover slide on top of the pre-greased well and ensure it is well sealed but take care to not disturb the drop or break the cover slide. Repeat this process until the tray is filled and then store at 25 °C.
         NOTE: Small cubic crystals should appear in 2-7 days.
      3. Prepare a microseed stock of the cubic crystals. Use a mounted nylon loop to transfer ~10 small cubic crystals to a 1.5 mL micro-centrifuge tube containing a small bead and 50 µL of 1.6 M sodium citrate tribasic wit pH 6.5.
      4. Vortex the 1.5 mL micro-centrifuge tube at high speed (~ 3000 rpm) for 1 min.
      5. Make a series of 10-fold serial dilutions of the seed stock with 1.6 M sodium citrate tribasic and vortex the mixture thoroughly for 5 s.
      6. Fill each well of a 24-well grid, screen with 500 µL of 1.6 M sodium citrate tribasic pH 6.5.
      7. Optimize the microseeding conditions by setting up drops with varying ratios of protein with the seed stock solutions (Figure 3A). Larger cubic crystals of high diffraction quality should appear in 2-5 days (Figure 3C).
   4. Optimize the orthorhombic crystals (Nsa1_ΔC)
      1. Prepare a grid screen with 500 µL in each well with 24 different conditions (Figure 3B) from stock solutions of 50%(v/v) PEG 1500, and 100%(v/v) PEG 400. In addition to gradients of PEG 1500 and PEG 400, each well should also contain 0.1 M HEPES/sodium hydroxide pH 7.5.
      2. Mix 1 µL of protein solution with 1 µL of well solution on a siliconized cover slide. Carefully invert the cover slide on top of the pre-greased well and ensure it is well sealed. Repeat this process until the entire tray has been filled. Store the trays at 25 °C.
         NOTE: Nsa1 orthorhombic crystals should appear in 2-7 days.
      3. Further optimize the orthorhombic crystals by microseeding as described for the cubic crystals (steps 2.3.3.3 to 2.3.3.7) using 500 µL of 20.1%(v/v) PEG 1500, 13.4%(v/v) PEG 400, and 0.1 M HEPES/sodium hydroxide pH 7.5 as the well solution.
         NOTE: Nsa1 SeMet crystals should be optimized analogous to the native crystals.

3. X-ray Diffraction Data Collection and Nsa 1 Structure Solution

1. Cryo-protection of Crystals and X-ray Diffraction Data Collection
   1. For the orthorhombic crystals (Nsa1_ΔC), prepare a 1 mL cryoprotectant solution containing 22.5%(v/v) PEG 1500, 15%(v/v) PEG 400 and 0.1 M HEPES/sodium hydroxide pH 7.5.
   2. Fill a foam Dewar with liquid nitrogen, and pre-cool a crystal puck. Use caution when working with liquid nitrogen and wear protective gloves and goggles.
   3. Carefully invert the cover slide of the crystallization well containing crystals onto the stage of a stereomicroscope.
   4. Pipette 2 µL of the cryoprotectant solution onto a new cover slide.
   5. Attach a mounted nylon loop of the appropriate size for the crystal to a magnetic cryo wand.
   6. Using the aid of the stereomicroscope, quickly transfer a crystal to the cryoprotectant solution with the mounted cryo loop.
   7. Let the crystal equilibrate for 5 min in the cryoprotectant solution.
   8. Using the aid of the stereomicroscope, quickly loop the crystal from the cryoprotectant solution and plunge-freeze into liquid nitrogen.
   9. Wait for the liquid nitrogen around the loop to stop boiling and then release the loop from the wand into a specific location within the crystal puck.
   10. Cubic Nsa1_FL crystals do not need to be cryoprotected and can be directly flash frozen (following steps 3.1.8-3.1.9 above).
   11. Seal the crystal puck using cryo tools and transfer to a shipping cane in a pre-chilled dewar. Store crystals in the pucks/dewars until data collection.
   12. If collecting data at a synchrotron, ship crystals to the synchrotron using a dry shipper.
   13. Collect X-ray diffraction data following standard techniques²⁰.
       NOTE: For Nsa1 native and SAD (single-wavelength anomalous dispersion) datasets were collected at 100 K on the SER-CAT beam lines 22-ID and 22-BM of the Advanced Photon Source at Argonne National Laboratory (Chicago, IL). The SAD Nsa1 dataset was collected at λ= 0.97911 Å. Data was recorded using a 1 s exposure time and 0.5° oscillations. The mosaicity of these crystals was typically around 0.3°.
   14. Process and scale the X-ray diffraction images to generate reflection files for each data set in the appropriate space group.
       NOTE: Nsa1 diffraction datasets were processed with HKL2000²¹. The Nsa1 cubic crystals were processed in the space group P2₁3 and the orthorhombic crystals were processed in the space group P2₁2₁2₁.
2. Nsa1 Structure Solution.
   NOTE: There are several crystallography software packages that can be used to solve and refine crystal structures including Phenix and CCP4^22,23. Following is the protocol for Nsa1 structure solution using the Phenix software suite²².
   1. Analyze the Native and SAD scaled datasets with phenix.xtriage²².
   2. Solve the structure of Nsa1 with Phenix.autosol using the SAD peak reflection file^22,24. To run the program of AutoSol, input the number of selenomethionine sites (sites= 9), the fasta sequence file of Nsa1_ΔC, and the wavelength used for SAD data collection (λ= 0.97911 Å).
      NOTE: From the Nsa1 SAD dataset, phenix.autosol should be able to determine the experimental phases and build most of the model.
   3. Make manual adjustments to the model with Coot²⁵, followed by refinement in phenix.refine^22,26.
   4. Solve the structure of the high-resolution native orthorhombic crystal and the cubic crystal by molecular replacement using Phaser^27,28.
   5. After successful structure solution, inspect the model and the electron density map in Coot²⁵.
   6. Build and refine the structures by running iterative rounds of refinement in phenix.refine^22,26 and model building in Coot²⁵.

4. SAXS Data Collection, Processing, and Modeling

1. SAXS Data Collection
   NOTE: SAXS data were recorded for full-length S. cerevisiae Nsa1 at the Advanced Light Source, on the high-throughput SIBYLS beamline 12.3.1 at Lawrence Berkeley National Laboratory, Berkeley, CA²⁹.
   1. Purify Nsa1_FL following the protocol described above. 24 h prior to shipment of Nsa1_FL to the beamline, run protein over a gel filtration column pre-equilibrated in buffer A.
   2. Pool fractions containing Nsa1 and determine the protein concentration as described earlier.
   3. Prepare 30 μl aliquots of a concentration series of Nsa1 from 1 to 6.2 mg/mL using buffer A.
   4. Transfer 20 μl of each concentration series of Nsa1 to a clear full skirt 96 well microplate along with buffer A alone controls.
      NOTE: SAXS data is collected on dilute solutions using several concentrations of purified sample to avoid aggregation, inter-particle repulsion, and radiation damage effects.
   5. Seal the microplate with a silicone sealing mat and ship overnight at 4 °C to the beamline.
   6. Store the microplate at 4 °C until data collection.
   7. Immediately before data collection, spin the plate at 3200 x g for 10 min at 4 °C to remove potential aggregates and air bubbles.
   8. Record SAXS data.
      NOTE: For Nsa1, SAXS data were recorded for the buffer before and after each protein concentration series. Thirty-three consecutive scans of 0.3 s were collected for Nsa1_FL over a concentration series (1 to 6.2 mg/mL) at 10 °C.
   9. Perform buffer subtraction for SAXS data.
      NOTE: For Nsa1 buffer subtraction was done automatically at the beamline but buffer subtraction can also be performed using data reduction software such as Scatter³⁰ and the ATSAS suite³¹. Buffer subtraction is a critical part of SAXS data analysis and care must be taken to ensure that the buffer used for subtraction is identical to the protein sample buffer.
   10. Average the 33 consecutive scans to create a *ave.dat file for each concentration.
       NOTE: Overlay the 33 consecutive frames to compare the curves. Changes to the scattering curves over time is often indicative of radiation damage. Exclude these frames from averaging. Averaging of the Nsa1 consecutive scans was performed automatically at the SIBYLS beamline.
2. SAXS Data Processing and Comparison of Concentration Series
   NOTE: There are several software packages that can be used to analyze SAXS data. For Nsa1 the radius of gyration and pair-wise distance distribution functions were determined using PRIMUS³² and Gnom³³ from the ATSAS 2.7.2 suite³¹ and compared across all protein concentrations to ensure there was no radiation damage or concentration-dependent inter-particle interactions¹⁰.
   1. Open a terminal shell and go to the directory containing the SAXS data.
   2. Launch the PRIMUS³² GUI from within the terminal shell.
   3. Within the PRIMUS GUI, load the scattering curves (*ave.dat).
   4. Use AutoR_g to determine the Radius of Gyration (R_g) and forward scattering intensity I(0), for each scattering curve (*ave.dat).
   5. Generate Kratky plots for each scattering curve (*ave.dat), to evaluate the degree of compactness.
   6. Use AutoGNOM³³ to calculate the pair-wise distribution function (also called P(r)) for each scattering curve (*ave.dat). Enter a starting D_max ≈ 3*R_g and optimize the D_max value to obtain a smooth P(r) curve. During the optimization of D_max, ensure that the calculated P(r) function is consistent with the experimental scattering curve by checking the reported χ² value and visually assessing the overall fit to the scattering curve.
   7. Calculate the molecular weight of Nsa1 from the scattering curves using the volume of correlation³⁴.
   8. Compare the structural parameters for each concentration to ensure that there are no radiation damage or concentration-dependent effects.
      NOTE: Concentration effects can manifest as an increasing R_g and D_max in relation to an increasing protein concentration. Forward scattering I(0) divided by the sample concentration should also remain constant across the protein concentration series.
3. SAXS Modeling
   NOTE: To determine the position of the C-terminus of Nsa1_FL, the Nsa1 crystal structure¹⁰ (PDB 5SUM) and the SAXS scattering curves were used to carry out a combination of rigid body and ab initio modeling, using the programs BUNCH³⁵ and Ensemble Optimization Method (EOM)³⁶ from the ATSAS software suite³¹. The WD40 domain of Nsa1 was treated as a rigid body, while the C-terminus of Nsa1 along with several disordered loops from the WD40 domain were modeled to fit the experimental SAXS data.
   1. Generate the input PDB file(s). The PDB file must be split every time residues are missing from the main chain, and the PDB file cannot contain multiple conformations, ligands, or water molecules.
   2. Run the program Pre_BUNCH³⁵ to prepare the input PDB file for BUNCH (pre_bunch.pdb). Input the sequence of the target protein (*.seq), the number of domains/PDBs generated in 4.3.1, and each of the individual PDB files generated above.
   3. Calculate the scattering amplitudes for each individual PDB file using the program CRYSOL³⁷. To run CRYSOL input the individual PDB file and the experimental SAXS scattering curve (*.dat). This will generate an amplitudes file (*.alm).
   4. Run the program BUNCH³⁵ to model the WD40 domain of Nsa1 against the SAXS data using a combined rigid body and ab initio approach. Input the PDB file from Pre_BUNCH (pre_bunch.pdb), the experimental SAXS scattering curve (*.dat), and the individual amplitude (*.alm) files for each partial PDB file generated by CRYSOL.
   5. Compare the χ² value from the starting PDB (5SUM) with that from the ab initio model generated by BUNCH using the experimental SAXS data.
      NOTE: A successful BUNCH model should have a significantly lower χ² value than the starting model. The theoretical scattering of the BUNCH model should also describe well the experimental data as judged by visual inspection of the overlay between the theoretical scattering of the BUNCH model to the SAXS data and its χ² value (Figure 4, center pipeline).
   6. Manually inspect the output files from BUNCH in Pymol³⁸ to overlay the crystal structure with the model generated by BUNCH, and the SAXS envelope (Figure 4, center pipeline).
   7. Rerun BUNCH 10-20 times to generate independent models to confirm that the models are similar.
      NOTE: For Nsa1 there was a range of χ² values from ~1 to 3 from 20 independent runs.
   8. Ensemble Modeling
      NOTE: As an optional approach to BUNCH run either EOM³⁶ or Minimal Ensemble Search³⁹ (MES). EOM and MES use ensemble approaches, which are well suited for proteins with flexible domains/regions that are in multiple conformations.
      1. Run the program EOM³⁶ using the ATSAS online server. To run EOM, input the PDB files from 4.3.1, the sequence of the target protein (*.seq), and the experimental SAXS data (*.dat).
      2. Compare the χ² values from the starting PDB (5SUM) with that from the ensemble generated by EOM using the experimental SAXS data.
         NOTE: A successful EOM ensemble should have a significantly lower χ² value than the starting model. The theoretical scattering of the ensemble should also describe well the experimental data as judged by visual inspection of the overlay between the theoretical scattering of the ensemble to the SAXS data and its χ² value (Figure 4, right pipeline). One should also compare the χ² values from BUNCH and EOM to determine which model best describes the experimental SAXS data.
      3. Manually inspect the EOM conformers in Pymol³⁸ to overlay the crystal structure with the conformers generated by EOM (Figure 4). Note the total number of conformers and the fraction of occupancy for each conformer that contributes to the scattering curve. For more rigid molecules, such as Nsa1, the number of conformers should be small (1-5) (Figure 4, right pipeline)³⁶.
      4. Re-run EOM several times to ensure consistent results.
         NOTE: For Nsa1 the number of conformers was typically 3 to 4 with χ² values ranging from 0.1 to 0.3.

Wyniki

Nsa1 was PCR amplified from S. cerevisiae genomic DNA and subcloned into a vector containing an N-terminal 6x-Histidine affinity tag followed by MBP and a TEV protease site. Nsa1 was transformed into E. coli BL21(DE3) cells and high yields of protein expression were obtained following induction with IPTG and growth at 25 °C overnight (Figure 1A). Nsa1 was affinity-purified on immobilized cobalt affinity resin, followed by MBP cleavage w...

Dyskusje

Using this protocol, recombinant Nsa1 from S. cerevisiae was generated for structural studies by both X-ray crystallography and SAXS. Nsa1 was well-behaved in solution and crystallized in multiple crystal forms. During the optimization of these crystals, it was discovered that the C-terminus of Nsa1 was sensitive to protease degradation. The high resolution, orthorhombic crystal form could only be duplicated with C-terminal truncation variants of Nsa1, likely because the flexible C-terminus of Nsa1 prevented cry...

Materiały

Name	Company	Catalog Number	Comments
Molecular Cloning of Nsa1
pMBP2 parallel vector	Sheffield et al, Protein Expression and Purification 15, 34-39 (1999)		We used a modified version of pMBP2 which included an N-terminal His-tag (pHMBP)
S. cerevisiae genomic DNA	ATCC	204508D-5
Primers for cloning Nsa1
SC_Nsa1_FLFw	IDT		CGC CAA AGG CCT ATGAGGTTACTAGTCAGCTGTGT GGATAG
SC_Nsa1_FLRv	IDT		AATGCAGCGGCCGCTCAAATTTT GCTTTTCTTACTGGCTTTAGAAGC AGC
SC_Nsa1_DeltaCFw	IDT		GGGCGCCATGGGATCCATGAGG TTACTAGTCAGCTGTGTGG
SC_Nsa1_DeltaCRv	IDT		GATTCGAAAGCGGCCGCTTAAAC CTTCCTTTTTTGCTTCCC
Recombinant Protein Production and Purification of Nsa1
Escherichia coli BL21 (DE3) Star Cells	Invitrogen	C601003
pMBP- NSA1 and various truncations	Lo et al., 2017
Selenomethionine	Molecular Dimensions	MD12-503B
IPTG, Dioxane-Free	Promega	V3953
EDTA Free Protease Inhibitor Cocktail	Sigma-Aldrich	4693159001
Sodium Chloride	Caledon Laboratory Chemicals	7560-1-80
Magnesium Chloride hexahydrate	Sigma-Aldrich	M2670
Tris Buffer, 1 M pH7.5	KD Medical	RGF-3340
Glycerol	Invitrogen	15514-029
beta-mercaptoethanol	Sigma	M6250
1M Imidazole, pH 8.0	Teknova	I6980-06
Talon Affinity Resin	Clonetech	635503
Amicon Ultra 15 mL Centrifugal Filter (MWCO 10K)	Millipore	UFC901024
HiLoad 16/600 Superdex 200 Prep Grade Gel Filtration Column	GE-Healthcare	28989335
TEV Protease	Prepared by NIEHS Protein Expression Core	Expression plasmid provided by NCI (Tropea et al. Methods Mol Biology, 2009)
4-15% Mini-PROTEAN TGX Precast Protein Gels	BioRad	456-8056
Crystallization, Proteolytic Screening
Crystal Screen	Hampton Research	HR2-110
Crystal Screen 2	Hampton Research	HR2-112
Salt Rx	Hampton Research	HR2-136
Index  Screen	Hampton Research	HR2-144
PEG/Ion Screen	Hampton Research	HR2-139
JCSG+	Molecular Dimensions	MD1-37
Wizard Precipitant Synergy	Molecular Dimensions	MD15-PS-T
Swissci 96-well 3-drop UVP sitting drop plates	TTP Labtech	4150-05823
3inch Wide Crystal Clear Sealing Tape	Hampton Research	HR4-506
Proti-Ace Kit	Hampton Research	HR2-429
PEG 1500	Molecular Dimensions	MD2-100-6
PEG 400	Molecular Dimensions	MD2-100-3
HEPES/sodium hydroxide pH 7.5	Molecular Dimensions	MD2-011-
Sodium Citrate tribasic	Molecular Dimensions	MD2-100-127
22 mm x 0.22 mm Siliconized Coverslides	Hampton Research	HR3-231
24 Well Plates with sealant (VDX Plate with Sealant)	Hampton Research	HR3-172
18 mM Mounted Nylon Loops (0.05 mm to 0.5 mM)	Hampton Research	HR4-945, HR4-947, HR4-970, HR4-971
Seed Bead Kit	Hampton Research	HR2-320
Magnetic Crystal Caps	Hampton Research	HR4-779
Magnetic Cryo Wand	Hampton Research	HR4-729
Cryogenic Foam Dewar	Hampton Research	HR4-673
Crystal Puck System	MiTeGen	M-CP-111-021
Full Skirt 96 well Clear Plate	VWR	10011-228
AxyMat Sealing Mat	VWR	10011-130
Equipment
UVEX-m	JAN Scientific, Inc.
Nanodrop Lite Spectrophotometer	Thermo-Fisher
Mosquito Robot	TTP Labtech
Software/Websites
HKL2000	Otwinoski and Minor, 1997
Phenix	Adams et al., 2010
Coot	Emsley et al., 2010
ATSAS	Petoukhov et al., 2012		https://www.embl-hamburg.de/biosaxs/atsas-online/
Scatter	Rambo and Tainer, 2013
Pymol	The PyMOL Molecular Graphics System, Version 1.8 Schrödinger, LLC.
BUNCH	Petoukhov and Svergun, 2005
CRYSOL	Svergun et al, 1995
PRIMUS	Konarev et al, 2003
EOM	Tria et al, 2015