Multi-target Parallel Processing Approach for Gene-to-structure Determination of the Influenza Polymerase PB2 Subunit

An overview of the protocol is presented in Figure 1.

Biologie moléculaire

1. Construct Design

Use Gene Composer software to design protein construct and codon engineered synthetic gene sequences. The use of Gene Composer software has been offered in detail elsewhere ³.

1. Use the Alignment Viewer Module and Construct Design Module to compare protein sequence alignments and define protein construct. Align target amino acid sequence to both the primary and 3D structural elements from homologs in the Protein Data Bank (PDB), if available (Figure 2).
2. Use alignment information to make structure-guided construct designs by choosing new termini based on conservation of the primary structure and 3D structures of homologs.
3. Design insert PCR (iPCR) and vector PCR (vPCR) amplimers (terminal primers).
4. Using Gene Composer’s protein-to-DNA algorithm, back-translate the construct amino acid sequence into codon engineered nucleic acid sequence.
5. Use the proper codon usage table (CUT) to optimize sequence for expression in E. coli.
6. Virtually clone insert into pET28 vector modified to incorporate a N-terminal 6x Histidine tag and Smt3/SUMO fusion protein that allows for easy purification.
7. Place synthetic gene order with DNA 2.0 and order primers from Integrated DNA Technologies.

2. Polymerase Incomplete Primer Extension (PIPE) Cloning

1. Prepare Primers and Genes
   1. Centrifuge the vendor-supplied plates containing primers at 1,000 rpm for 1 min.
   2. Bring primer concentration to 100 μM and add 50 μl TE buffer.
   3. Dilute primers to 10 μM with deionized (DI) water in a 96-well v-bottom plate.
   4. Centrifuge the vendor-supplied gene in a 1.5 ml tube at 1,300 rpm for 1 min.
   5. Using TE buffer, bring the DNA concentration of each tube to 50 ng/μl.
   6. In 1.5 ml tubes, make dilutions of each primer to 10 ng/μl.
   7. Store primers and genes at -20 °C when not in use.
2. Prepare Insert PCR (iPCR)
   1. Thaw a vial of Pfu Master Mix on ice; keep genes and primers at room temperature.
   2. Create a plate map assigning wells to a set of primers and construct.
   3. Add 13 μl of DI water into each well of a 96-well PCR plate.
   4. Add 5 μl of forward and 5 μl of reverse primer to each reaction in the 96-well plate according to the plate map, ensuring to change tips between each well.
   5. Add 2 μl of each full length gene to its appropriate well according to the plate map.
   6. Add 25 μl of Pfu master mix to each well, ensuring to change tips between each well.
   7. Cycle the reactions using the following PCR conditions:
      1. 95 °C 2 min
      2. 95 °C 30 sec
      3. 50 °C 45 sec
      4. 68 °C 3 min
      5. 4 °C ∞
   8. Repeat steps b-d for 25 cycles.
   9. Transfer 10 μl of each iPCR reaction to a new 96-well PCR plate.
   10. Add 3 μl of 6X load dye to each sample.
   11. Separate each sample on a 1% TAE EtBr agarose gel at 110 V next to a 100-500 bps DNA ladder to confirm fragment amplification.
   12. Store iPCR product at -20 °C when not in use (avoid freeze thaw as much as possible).

3. Prepare Vector PCR (vPCR)

1. Start overnight culture of transformed E. coli with pET28 vector plasmid.
   1. Inoculate two 5 ml tubes of 2-YT broth with 50 μg/ml kanamycin.
   2. Grow cultures overnight at 37 °C in shaker at 220 rpm.
2. Spin down cultures after overnight growth by centrifuging at 3,000 rpm for 15 min.
3. Use a Qiagen QIAprep Spin Miniprep Kit to extract pET28 vector from bacterial pellets according to the manufacturer’s instructions.
4. Setup restriction enzyme digestions of extracted pET28 plasmid.
   1. Add 2.2 μl of 10X BamHI buffer and 1 μl of BamHI and HindIII to 20 μl of pET28 vector.
   2. Incubate reaction for 1 hr at 37 °C.
5. Separate digestion product on a gel.
   1. Refer to step 2.2.10.
   2. Cut vector band from gel and purify it using the QIAquick Gel Extraction Kit according to the manufacturer’s instructions.
6. Using a NanoDrop, quantify DNA concentration.
7. Dilute cut vector to 10 ng/μl. Store at -20 °C when not in use.
8. Prepare vPCR primers.
   1. Centrifuge IDT supplied oligonucliotides for 1 min at 1,300 rpm.
   2. Bring concentration to 100 μM with DI water.
   3. Prepare 10 μM dilution of both forward and reverse primers in a 1.5 ml tube.
   4. Store primers and primer dilutions at -20 °C.
9. Thaw Pfu Master Mix on ice and thaw template and primers at room temperature.
10. Setup vPCR reactions in a 96-well PCR plate:
    1. In the first row of a 96-well plate combine 60 μl of both forward and reverse vPCR primers and 24 μl of digested pET28 template (10 ng/μl).
    2. Using a 12-tip multichannel pipette, transfer 12 μl of the primer and template master mix to each remaining well of the plate. This should result in 12 μl of primer and template master mix in each well of the plate.
    3. Add 13 μl of DI water to each well.
    4. Add 25 μl of Pfu Master Mix to each well.
11. Cycle the reactions through the PCR conditions used in step 2.2.7.
12. Pool all of the vPCR reactions into a 15 ml Falcon tube.
13. Verify fragment amplification by separating 10 μl of pooled PCR product on a gel (expected length of digested pET28 vector is approximately 6 kb).
    1. Refer to step 2.2.10.
14. Prepare merge plates.
    1. Aliquot 3 μl of vPCR product into each well of a 96-well v-bottom plate.
    2. Store plates at -20 °C until merge with iPCR product.

4. Merge iPCR and vPCR Products

1. Thaw iPCR products and pre-aliquoted vPCR 96-well merge plate at room temperature.
2. Add 3 μl of each iPCR product to its respective well of the merge plate.
3. Transform merge plate into Top Ten chemically competent cells.
4. Add 2 μl of each merge reaction into a single 50 μl tube of vendor-supplied chemically competent cells and proceed with manufacturer’s supplied protocol.
5. Prepare overnight cultures for each construct from transformation plate.
6. Aliquot 5 ml TB broth (with 50 μg/ml kanamycin) from a 25 ml sterile reservoir into each well of a deep well block.
7. Using sterile technique, pick an isolated colony from each transformation plate and inoculate the appropriate well of the deep well block.
8. Cover the block with an Airpore cover.
9. Shake block at 220 rpm at 37 °C overnight.
10. Pellet cells by centrifuging the block for 30 min at 4,000 rpm.
11. Pour off the supernatant and pat the top of the block dry with a paper towel.
12. Mini-prep using a Qiagen 96-well vacuum apparatus according to the manufacturer’s instructions.

5. Preparing Glycerol Stocks of Successfully Cloned Constructs

1. Transform successfully cloned sequence validated DNA into BL21(DE3) chemically competent cells according to the manufacturer’s instructions.
2. For each construct, pick a single isolated colony from the BL21(DE3) transformation and inoculate into 1 ml of 2-YT broth (with 50 μg/ml kanamycin).
3. Shake cultures at 220 rpm for 3-4 hr at 37 °C.
4. Label a 1.5 ml screw cap tube with the unique construct identification number, cell strain, and date. Add 500 μl of 50% glycerol and 500 μl of cell culture and invert several times. Immediately store glycerol stock on dry ice or in a -80 °C freezer.

6. Expression Testing

* Add Benzonase, lysozyme, and protease inhibitor immediately before lysis.

1. Streak a sample from glycerol stock onto kanamycin selective agar and incubate overnight at 37 °C.
2. Start a non-inducing pre-culture in a 96-well round bottom block; inoculate 1.2 ml TB broth (with 50 mg/ml kanamycin) supplemented with 0.5% glucose with a freshly grown E. coli isolate. Grow overnight shaking at 220 rpm at 37 °C.
3. After overnight growth, start induction cultures by inoculating 1.2 ml of TB broth (with 50 mg/ml kanamycin) supplemented with Novagen Overnight Express System 1 (according to the manufacturer’s protocol) with 40 μl of the pre-culture.
4. Grow the small-scale induction cultures at 20 °C for 48 hr, shaking at 220 rpm.
5. Harvest cells by centrifuging at 4,000 rpm for 15 min, pour off supernatant and store at -20 °C for at least 1 hr prior to processing.
6. In the 96-well block, resuspend the cell pellets in 300 μl lysis buffer.
7. Incubate cells in lysis buffer at room temperature for 30 min followed by mechanical lysis by vigorously shaking for 30 min at room temperature.
8. Clarify the crude lysate by centrifugation for 30 min at 4,000 rpm at 4 °C.
9. Use a multi-channel pipette to transfer 200 μl of the clarified lysate (soluble fraction) to a 96-well flat bottom tray (Qiagen). For each well containing a sample, add 40 μl Ni-NTA magnetic beads (Qiagen).
10. Gently agitate the plate on a rocker for 1 hr at 16 °C.
11. Place the plate on a magnetic post plate (Qiagen) and remove the unbound soluble fraction. Take care to not pipette out any of the Ni-NTA beads.
12. Remove the plate from the post plate and gently resuspended the beads in 200 μl wash buffer. Pipette up and down for 30 sec and then place the plate back on the post plate.
13. Remove the wash buffer and repeat step 6.12.
14. Remove plate from post plate and elute the Ni-NTA bound target protein by washing with 50 μl elution buffer for 5 min.
15. Return flat bottom plate to magnetic post plate and transfer the elution to a fresh 96-well v-bottom plate.
16. Transfer 20 μl of the elution to a fresh 96-well v-bottom plate and react with 1 μl ULP1 protease.
17. According to the manufacturer’s protocol, analyze the eluted and eluted+Ulp1 fraction by capillary electrophoresis using a LabChip 90.
18. Alternatively, all fractions from the expression testing can be analyzed via SDS-PAGE.

7. Large Scale Fermentation

1. Use a sterile pipette tip to obtain a scrape from a glycerol stock, inoculate 100 ml TB broth (with 50 mg/ml kanamycin) and grow overnight. Shake at 220 rpm and 37 °C.
2. After overnight growth, expand pre-culture by inoculating 1 L of TB broth with EMD autoinduction solutions (see manufacturer’s protocol) (with 50 mg/ml kanamycin) in a 2 L baffled flask with 10 ml of the pre-culture (1:100 dilution).
3. Shake the expanded 1 L cultures at 37 °C; change the temperature of the shaking incubator to 20 °C when an optical density of 0.6 (OD₆₀₀) is reached.
4. After overnight growth, take a representative 10 ml aliquot from each construct for expression testing.
5. Harvest cell paste by centrifugation at 5,000 rpm for 15 min and discard supernatant.
6. Freeze cell paste at -80 °C.

PROTEIN PURIFICATION

Buffers:

* Add Benzonase, lysozyme, and protease inhibitor tablets to each 150 ml sample immediately before lysis.

8. Cell Lysis

1. Make 2 L of lysis buffer; do not add lysozyme, protease inhibitor tablets or benzonase (each sample will be lysed separately in 150 ml of lysis buffer).
2. Thaw and resuspend cell paste in lysis buffer at a 1:5 mass:volume ratio by vigorously stirring for 30 min at 4 °C. Break chunks loose from sides of beaker using a clean spatula. During this time period prepare Ni and Dialysis Buffers
3. On ice, lyse the cells using a Misonix sonicator (70% power, 2 sec on/1 sec off pulses for 3 min) and gently swirl container to prevent overheating. Save a small (200 μl) aliquot of crude lysate for future analysis.
4. Clarify the crude lysate by centrifugation at 18,000 x g for 35 min at 4 °C, collect the supernatant and save a small (200 μl) aliquot for future analysis. Store pellet at 4 °C until it is confirmed the protein has been lysed into the soluble fraction.

9. Pre-run Protein Maker Setup

1. With the protein maker turned on and the software open, initialize the instrument.
2. Once initialized, attach one 5.0 ml GE Healthcare HisTrap FF Nickel-chelate column (Ni column) on a separate line of the gantry for each of the samples.
3. Run 3-4 column volumes (CV) of equilibration buffer through each column.
4. Prime the equilibration and elution buffer lines.
5. Equilibrate the columns by aspirating buffer A through the column once.

10. Nickel 1 (Ni1) Column

1. Wash each column with 20 ml Milli-Q water to remove storage buffer. Run 5 ml buffer B and 25 ml buffer A for equilibration.
2. Load the clarified lysate containing solubilized protein into the columns at a rate of 2 ml/min then follow by a 15 ml wash with buffer A.
3. Elute the bound protein in a step gradient with buffers A and B by the following ratios respectfully: 5 ml 95:5, 5 ml 60:40, 10 ml 0:100. Collect each elution fraction separately.
4. Analyze: eluted fractions, crude lysate, clarified lysate, and flow-through by SDS-PAGE. Pool fractions containing the protein and use a Nanodrop to measure A₂₈₀ to roughly determine the amount of protein present.

11. ULP1 Cleavage

1. Keep a small aliquot (250 μl) of the Ni1 column pool for subsequent gel analysis. Bring the rest of the Ni1 pool to 10 ml and add ubiquitin-like protease 1 (ULP1) at 1 μl/5 mg of total protein to remove the His-Smt affinity tag.
2. Dialyze the Ni1 pool + ULP1 against 2 L of buffer A for 4 hr at 4 °C in a 10 kDa molecular-weight cutoff (MWCO) on a stir plate at 4 °C.
3. After dialysis, run SDS-PAGE of Ni1 pool and Ni1 pool+ULP1 to determine if ULP1 cleavage was successful.

12. Nickel 2 (Ni2) Column

1. Load cleaved protein over the same Ni column and repeat step 9.3 at a reduced flow rate of 1 ml/min. The cleaved off tag will bind to the column and the tagless target protein will now flow-through. Collect the flow-through in a fresh container.
2. Wash Ni column with 3 ml buffer A followed by 5 ml of buffer B to elute all His-tagged and nonspecifically bound protein. Collect each fraction separately.
3. Run SDS-PAGE of Ni2 flow-through, wash and Ni2 elution fractions to verify ULP1 cleavage and that protein is present in the flow-through. Use a Nanodrop to measure A₂₈₀ to roughly determine the presence of protein.

13. Concentrating

1. Concentrate the Ni2 flow-through (and Ni2 elution if protein is present) to 5 ml with an Amicon Ultra 10 kDa MWCO centrifuge tube. Spin in 10 min intervals at 4,000 rpm at 4 °C. Mix with a pipette between each spin to prevent protein from over-concentrating along membrane.

14. Size-exclusion Chromatography (SEC)

1. Set up a Sephacryl S-100 10/30 GL column (GE healthcare) by equilibrating with 200 ml SEC buffer at a flow rate of 0.5 ml/min on an AKTApurifier system (GE Healthcare).
2. Prepare 10 ml superloops for use on the SEC column according to the manufacturer’s instructions.
3. Using a 5 ml syringe, load samples onto superloops and begin the SEC run.
4. Monitor the UV-absorbance trace at 280 nm while collecting small volume fractions.
5. Run SEC fractions via SDS-PAGE.
6. Pool the SEC fractions showing the highest intensity bands.
7. Concentrate pooled SEC fractions. Refer to step 13.1.
8. Aliquot protein into 100 μl samples, flash freeze in liquid nitrogen and store at -80 °C.

CRYSTALLIZATION

15. Protein Crystallization

1. Pre-fill each reservoir of a 96-well Compact Jr crystallization plate (Emerald Bio) with 80 μl of crystallization screen (Emerald Bio) of choice.
2. Dilute protein with sizing buffer to 2-20 mg/ml and store on ice.
3. Dispense 0.4 μl of protein and 0.4 μl of the crystallization screen into each of the 96-wells and cover with crystal clear sealing tape (Manco).
4. Store the plate at 16 °C while checking for protein crystallization periodically over the next few weeks under a dissecting microscope.

16. Crystal Harvesting

1. Create a cryoprotectant from the mother liquor and ethylene glycol. Cut the clear tape covering the well with the target protein crystal. To an empty well, add 1.6 μl of the corresponding crystallizing condition and combine with 0.4 μl of ethylene glycol yielding a final concentration of 20% ethylene glycol and 80% crystallizing condition. Note: to optimize crystal diffraction try different cryoprotectants such as: glycerol, oils, low MW polyethylene glycols, and/or at varying percentages of the cryoprotectant.
2. Before harvesting cool down an ALS-style puck in a dewar filled with liquid nitrogen and cover with lid.
3. Harvest the crystal by placing a CryoLoop with the inner diameter matching the size of the crystal on a Magnetic Crystal Wand (Hampton Research) and scoop it directly from the well solution.
4. Immediately dip the CryoLoop with the harvested crystal into the cryoprotectant then submerge in the ALS-style puck to flash freeze the crystal. Repeat for a desired number of crystals.

17. Crystal Screening/Data Collection

1. Once harvesting is complete use a puck wand to place the magnetic cryo puck lid on the ALS puck. With bent tongs, flip the puck upside down.
2. Transfer the puck to a Rigaku ACTOR dewar, screw a Puck Pusher onto the puck, and punch off the lid leaving it in the dewar with pins face up.
3. Using JDirector software, screen each crystal under the following parameters: beam slit set to 0.5 degrees, detector distance set to 50 mm, image step to 70 degrees, and exposure length set to 30 sec.
4. Run Mosflm on the test images you shot with JDirector to determine what the best crystal and strategy is for data collection.
5. Collect a complete dataset based on your results from Mosflm.

18. Data Processing/Structure Determination

1. Run XDS/XSCALE ⁴ to process the dataset.
2. Open the CCP4 suite software.
   1. Run Phaser ⁵ to calculate a molecular replacement solution using a high homology search model, when available. In this case we used the PDBID 3CW4 as a search model ⁶.
   2. Run Refmac ⁷ to refine your molecular model against the observed reflection collected in the dataset. Final resolution should be based off of the highest shell and determined by the following parameters: R factor > 50%, I/sigma > 2, and completeness > 90%.
3. Build a 3-Dimensional electron density model with the molecular graphics software COOT ⁸.
4. Before depositing the structure in the PDB validate it with MolProbity ⁹ software to verify that quality of structure is suitable for deposition.