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== Protocol to isolate total, soluble and insoluble protein fractions from galactose-inducible strains of ''S. cerevisiae'' ==
= Isolating protein fractions from ''S. cerevisiae'' =


This protocol describes extraction of total, soluble and insoluble protein fractions from ''S. cerevisiae'' grown to mid-exponential phase. We lyse cells using a single 7mm stainless-steel ball, which prevents protein aggregation observed in glass-bead lysis. Aqueous-insoluble proteins are solublized using 8M urea and 2% SDS. For preparation of these samples for analysis by mass spectrometry, consider [[Drummond:ChlorMethExtraction|choroform-methanol extraction]].


* Inoculate a 3 mL pre-culture of YPD with a single yeast colony and incubate overnight at 30⁰ C with shaking or rotation.
== Buffers ==


* The next day, inoculate 70 mL of YP sucrose (2%) raffinose (1%) with 3 µL of the overnight pre-culture and incubate for 18 h at 30⁰ C with shaking in a 500 mL baffled flask.
=== Stock solutions ===
*200mM DTT in H<sub>2</sub>O (store as 50μL aliquots at -20°C and thaw just before use).
*100mM PMSF in ethanol (store at -20°C; half-life in aqueous solution is ~30 minutes).
*4M NaCl (store at RT)
*20% SDS (w/v) (store at RT)
*1M Tris-HCl, pH 8.5 (store at RT)
*50mM Tris-HCl, pH 8.5 (store at 4°C)


* The next day, measure the optical density of the 70 mL assay culture to confirm that it is at an OD<sub>600</sub> of around 0.400. Transfer 45 mL of the assay culture to a new 500 mL baffled flask and induce with 40 mM galactose (add 1622 µL of 20% galactose) for 2 h at 30⁰ C with shaking.  Continue to incubate the original flask of remaining uninduced cells alongside the flask of galactose-induced cells.
For protease inhibitors, we use:
*AEBSF, HCl, MW=239.5, targets serine proteases, 100 mM
*E-64, MW=357.4, targets cysteine proteases, 1.5 mM
*Pepstatin A, MW=685.9, targets aspartic proteases, 2 mM
*o-Phenanthroline, MW=198.2, targets metalloproteases, 500 mM


* Harvest aliquots of the assay cultures.  The aliquots will be for either the isolation of total protein, or for the sequential isolations of soluble and insoluble protein fractions.  There are three aliquots to harvest; two aliquots from the galactose-induced culture flask, and one aliquot from the remaining uninduced culture flask.  The volumes to harvest should be equivalent to 15 mL of cells that are at an OD600 of 0.850. <br>  For example, if the OD600 is 0.725, harvest 17.6 mL of cells; if the OD600 is 0.950, harvest 13.4 mL of cells (i.e., 15 mL X 0.850).
This mixture is commercially available as Calbiochem protease inhibitor cocktail set IV, or BioVision EZBlock protease inhibitor cocktail IV.
 
* Pellet each aliquot at 3,000 g for 2 min and thoroughly drain the media.  Wash the pellet in 1.8 mL of protease-free water and transfer to a 2 mL microcentrifuge tube.  Pellet again at 20,000 g for 10 sec and remove the wash with a vacuum trap, being careful to not disturb the cell pellet.  Resuspend the cells in 1.4 mL of Buffer Z and 14 µL of 1M β-mercaptoethanol.  Add 33 µL of Zymolyase (10 µg/µL), mix by inversion and incubate at 30⁰C for 30 to 35 min with gentle shaking.
 
* Pellet the resulting spheroplasts at 3,000 g for 5 min at 4⁰ C.  Aspirate the supernatant with a vacuum trap, being careful to not disturb the cell pellet, and gently wash the pellet with 750 µL of ice cold Buffer Z (do not resuspend the pellet, but rather rinse the walls of the tube and the top of the pellet by gentle inversion).  Centrifuge again at 3000 g for 3 min at 4⁰ C and remove the wash with a vacuum trap, being careful to not disturb the cell pellet.
 
Note: Perform the following two steps A and B together, side-by-side.
 
* A: Total protein isolation
**Lyse a sample of galactose-induced, spheroplasted cells, and another sample of uninduced spheroplasted-cells in 400 µL of room temperature IPB by vigorously vortexing for 3 min on the benchtop.  Centrifuge the samples at 20,000 g for 5 min at 4⁰ C.  Thoroughly decant the supernatant to a 1.5 mL microcentrifuge tube, add 67 µL of room temperature IPLB, vortex and heat-denature at 60⁰ C for 5 min.  Chill on ice and store at -20⁰ C.  This is the '''total protein fraction'''.
 
* B: Soluble and insoluble protein isolation
**Lyse a sample of galactose-induced, spheroplasted cells in 400 µL of ice-cold SPB by vigorously vortexing for 5 min in a cold room.  Centrifuge the sample at 20,000 g for 5 min at 4⁰ C.  Thoroughly decant the supernatant to a 1.5 mL microcentrifuge tube, add 67 µL of room temperature SPLB, vortex and heat denature at 60⁰ C for 5 min.  Chill on ice, and later store at -20⁰ C.  This is the '''soluble protein fraction'''.
**Wash the pellet in 400 µL of ice cold SPB by vigorously vortexing for 5 min in a cold room.  Centrifuge the sample at 20,000 g for 5 min at 4⁰ C.  Thoroughly decant the supernatant to a 1.5 mL microcentrifuge tube, add 67 µL of room temperature SPLB, vortex and heat denature at 60⁰C for 5 min.  Chill on ice, and later store at -20⁰ C.  Repeat this step twice on the remaining pellet for a total of 3 washes. Vigorously vortex the washed pellet in 400 µL of room temperature IPB for 3 min on the bench top.  Centrifuge the sample at 20,000 g for 5 min at 4⁰ C.  Thoroughly decant the supernatant to a 1.5 mL microcentrifuge tube, add 67 µL of room-temperature IPLB, vortex and heat denature at 60⁰ C for 5 min.  Chill on ice and store at -20⁰ C.  This is the '''insoluble protein fraction'''.
* Store all samples at -20⁰ C to -80⁰ C.
 
== Buffer recipes ==
 
=== Stock solutions ===
*200mM DTT
*100mM PMSF
*4M NaCl
*1M Tris-HCl, pH 8.5
*20% SDS (w/v)


=== Soluble Protein Buffer, pH 8.5 (SPB) ===
=== Soluble Protein Buffer, pH 8.5 (SPB) ===
Line 44: Line 31:
* 2.5 mL    1M Tris-HCl, pH 8.5
* 2.5 mL    1M Tris-HCl, pH 8.5
*      6.25 mL    4M NaCl
*      6.25 mL    4M NaCl
* 45.4 mL    protease-free H<sub>2</sub>O
*     41.25 mL    protease-free H<sub>2</sub>O


Then mix 9.8 mL of SPB stock solution with 100 µL 100mM PMSF and 100uL protease inhibitors to make 10mL SPB.
Then mix 9.8 mL of SPB stock solution with 100 µL 100mM PMSF and 100uL protease inhibitors to make 10mL SPB.


For protease inhibitors, we use:
=== Wash Buffer (WB) ===
*AEBSF, HCl, MW=239.5, targets serine proteases, 100 mM
(50mM Tris-HCl, 150mM NaCl, 1:100 protease inhibitors) Same as SPB, but with reduced salt to limit pellet loss.
*E-64, MW=357.4, targets cysteine proteases, 1.5 mM
 
*Pepstatin A, MW=685.9, targets aspartic proteases, 2 mM
Start by making 50 mL WB stock solution:
*o-Phenanthroline, MW=198.2, targets metalloproteases, 500 mM
* 2.5 mL    1M Tris-HCl, pH 8.5
*     1.875 mL    4M NaCl
*     45.625 mL    protease-free H<sub>2</sub>O


This mixture is commercially available as Calbiochem protease inhibitor cocktail set IV, or BioVision EZBlock protease inhibitor cocktail IV.
Then mix 9.8 mL of WB stock solution with 100 µL 100mM PMSF and 100µL protease inhibitors to make 10mL WB.


=== Insoluble Protein Buffer, pH 8.5 (IPB) ===
=== Insoluble Protein Buffer, pH 8.5 (IPB) ===
(50mM Tris-HCl, 150mM NaCl, 8M urea, 2% SDS, 1mM PMSF, 200mM DTT, 1:1000 protease inhibitors)
(50mM Tris-HCl, 150mM NaCl, 8M urea, 2% SDS, 1mM PMSF, 2mM DTT, 1:1000 protease inhibitors)
Make fresh before each use. Note that at 8M, urea occupies ~72% of the solution volume, so that 4.8g urea occupies 7.2mL of a 10mL solution. Do not use 500mM NaCl in this solution, as it loosens pellets and causes sample loss.
Make fresh just before each use. Note that at 8M, urea occupies ~72% of the solution volume, so that 4.8g urea occupies 7.2mL of a 10mL solution. Do not use 500mM NaCl in this solution, as it loosens pellets and causes sample loss.


*8M urea
*8M urea
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=== 6x Soluble Protein Loading Buffer, pH 6.8 (SPLB) ===
=== 6x Soluble Protein Loading Buffer, pH 6.8 (SPLB) ===
(50 mM Tris-HCl pH 8.5, 10% SDS, 0.05% bromophenol blue, 30% glycerol, 5% β-mercaptoethanol [βME])
(50 mM Tris-HCl pH 6.8, 10% SDS, 0.05% bromophenol blue, 30% glycerol, 5% β-mercaptoethanol [βME])


Start by making 9 mL 6x SPLB Stock Solution:
Start by making 9 mL 6x SPLB Stock Solution:
* 0.5 mL  1M Tris-HCl, pH 8.5
* 0.5 mL  1M Tris-HCl, pH 6.8
*   1 g    SDS
*   1 g    SDS
*   5 mg  bromophenol blue
*   5 mg  bromophenol blue
Line 113: Line 101:


Then mix 712.5 µL of 6x SPLB stock solution with 37.5 µL of 14.3M βME immediately before use.
Then mix 712.5 µL of 6x SPLB stock solution with 37.5 µL of 14.3M βME immediately before use.
=== 6x Soluble Protein Storage Buffer, pH 8.5 (SPSB) ===
(50 mM Tris-HCl pH 8.5, 12% SDS, 5% β-mercaptoethanol [βME])
Start by making 10 mL 6x SPSB Stock Solution:
* 0.5 mL  1M Tris-HCl, pH 8.5
*   6 mL  20% SDS
* 3.5 mL  protease-free water
Then mix 712.5 µL of 6x SPSB stock solution with 37.5 µL of 14.3M βME immediately before use.


=== 6x Insoluble Protein Loading Buffer, pH 6.8 (IPLB) ===
=== 6x Insoluble Protein Loading Buffer, pH 6.8 (IPLB) ===
(50 mM Tris-HCl, 0.05% bromophenol blue, 30% glycerol, 5% βME)
(50 mM Tris-HCl, 0.05% bromophenol blue, 30% glycerol, 5% βME)


Start by making 9 mL 6x SPLB Stock Solution:
Start by making 9 mL 6x IPLB Stock Solution (nearly the same as SPLB stock, but
* 0.5 mL  1M Tris-HCl, pH 6.8
* 0.5 mL  1M Tris-HCl, pH 6.8
*   5 mg  bromophenol blue
*   5 mg  bromophenol blue
Line 123: Line 121:
* 5.5 mL  protease-free water
* 5.5 mL  protease-free water


Then mix 475 µL of 6x SPLB stock solution with 25 µL 14.3M βME immediately before use.
Then mix 475 µL of 6x IPLB stock solution with 25 µL 14.3M βME immediately before use.
 
==Protocol==
 
===Day -2===
* For each strain, inoculate a 3 mL YPD pre-culture of YPD with a single yeast colony and incubate overnight at 30⁰C with shaking or rotation.
 
===Day -1===
* Inoculate 50 mL of synthetic complete medium (SC) with labeled amino acids with 3 µL of the overnight pre-culture and incubate for 18 h at 30⁰ C with shaking in a 500 mL baffled flask.
 
===Day 0===
''Cell preparation''
* Grow 50mL culture of cells to a density of 4×10<sup>6</sup> cells/mL  (OD<sub>600</sub> ≈ 0.4).
 
While cells are growing, make solutions: SPB, WB, IPB. Put 1.1 mL × number of samples' worth of 50mM Tris-HCl pH 8.5 on ice.
 
* Transfer 1.4×10<sup>8</sup> cells to a 50mL conical tube (35 mL of a 4×10<sup>6</sup> cells/mL culture)
* Spin at 3000g for 1 minute.
* Gently decant and discard supernatant.
* Resuspend cell pellet in 1.4mL ice-cold Tris (50mM, pH 8.5) and transfer to 1.5mL microcentrifuge tube.
* Spin at 20,000g for 15 seconds.
* Discard supernatant, clear residual liquid with a hard snap.
* Freeze pellet in liquid nitrogen.
 
Now decide whether you want total protein extraction or soluble/insoluble fractionation.
 
''Lysis for soluble/insoluble fractionation''
* For each strain, rack a 2mL flat or round-bottom microcentrifuge tube in LN2 and place a 7mm stainless-steel ball (Retsch #05.368.0035) inside. Put some LN2 in tube to speed cooling of ball and to catch the incoming sample. Label the sides as well as the tops of the tubes, as lysis will often crack off the tube cap.
* Resuspend frozen pellet in 50 µL SPB.
* Drip resuspended pellet onto upper wall of tube containing ball. Goal is to get a nugget of frozen material on the wall, and to avoid dripping the material around the ball and thus freezing the ball to the bottom of the tube; having some LN2 remaining in the tube helps.
* When all LN2 has boiled out of tube (listen -- if any popping or hissing, keep waiting), snap tube closed. Keep in LN2. (Any remaining LN2 in tube will cause tube to explode open and fire the stainless steel ball into your iPad, brain, colleague, or other important equipment.)
* Rack the tube into the PTFE 2mL tube adaptor for the Retsch Mixer Mill MM400 (Retsch #22.008.0005) and submerge the entire assembly in LN2.
* Agitate for 4×90 seconds at 30 Hz in a Retsch Mixer Mill MM400, returning sample holder to LN2 between sessions. Complete lysis produces fine snowy powder in the tube.
* Remove sample tubes from LN2 and pop the caps to relieve pressure.
* Add 450 μL SPB to each tube, and extract ball with a magnet. We rinse balls in methanol and store in 50% ethanol.
* Move 500 μL sample to a fresh 1.5mL microcentrifuge tube.
 
''Soluble fraction extraction''
* Spin at 3000g for 30 seconds (clarification step).
* Decant clarified liquid into a 1.5mL polyallomer conical centrifuge tube (Beckman Coulter).
* Spin at 100,000g for 20 minutes (fixed-angle TLA-55 rotor at 40,309 rpm in a Beckman Coulter Optimax tabletop ultracentrifuge).
* Decant supernatant into a 1.5mL microcentrifuge tube: this is the '''soluble fraction'''.
 
''Insoluble fraction extraction''
* Violently snap pellet to clear remaining liquid.
* Add 500 μL wash buffer (WB) and vortex violently. (The pellet may not resuspend; that's fine.)
* Spin at 100,000g for 20 minutes.
* Discard supernatant, clear residual liquid with a hard snap.
* Add 500 μL insoluble protein buffer (IPB).
* Vortex until pellet dissolves, 10-15 minutes for clarified samples.
* Spin at 20,000g for 5 minutes.
* Decant supernatant into a 1.5mL microcentrifuge tube: this is the '''insoluble fraction'''.
 
''Lysis for total protein extraction''
* For each strain, rack a 2mL flat or round-bottom microcentrifuge tube in LN2 and place a 7mm stainless-steel ball (Retsch #05.368.0035) inside. Put some LN2 in tube to speed cooling of ball (ultimately we want all the LN2 to boil away).
* Resuspend frozen pellet in 50 µL insoluble protein buffer (IPB).
* Drip resuspended pellet onto upper wall of tube containing ball. Goal is to get a nugget of frozen material on the wall, and to avoid dripping the material around the ball and thus freezing the ball to the bottom of the tube.
* When all LN2 has boiled out of tube (listen -- if any popping or hissing, keep waiting), snap tube closed. Keep in LN2. (Any remaining LN2 in tube will cause tube to explode open and fire the stainless steel ball into your iPad, brain, colleague, or other important equipment.)
* Rack the tube into the PTFE 2mL tube adaptor for the Retsch Mixer Mill MM400 (Retsch #22.008.0005) and submerge the entire assembly in LN2.
* Agitate for 4×90 seconds at 30 Hz in a Retsch Mixer Mill MM400, returning sample holder to LN2 between sessions. Complete lysis produces fine snowy powder in the tube.
* Add 450 μL IPB to tube, and extract ball with a magnet.
* Move 500 μL sample to a fresh 1.5mL microcentrifuge tube.
* Spin at 20,000g for 5 minutes.
* Decant supernatant into a 1.5mL microcentrifuge tube: this is the '''total protein fraction'''.
 


=== Buffer Z for Zymolyase digestion ===
''Storage''
(50mM Tris-HCl pH 7.4, 1M sorbitol)


Mix the following to obtain 50 mL Buffer Z:
For insoluble and total-protein fractions, make 100μL aliquots and store at -80°C.
*  10 mL  5M sorbitol
*  2.5 mL  1M Tris-HCl, pH 7.4
* 37.5 mL  sterile water


For soluble fractions, mix 5:1 with fresh 6x soluble protein storage buffer (SPSB), denature for 5 minutes at 95°C, make 100μL aliquots and store at -80°C.


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Isolating protein fractions from S. cerevisiae

This protocol describes extraction of total, soluble and insoluble protein fractions from S. cerevisiae grown to mid-exponential phase. We lyse cells using a single 7mm stainless-steel ball, which prevents protein aggregation observed in glass-bead lysis. Aqueous-insoluble proteins are solublized using 8M urea and 2% SDS. For preparation of these samples for analysis by mass spectrometry, consider choroform-methanol extraction.

Buffers

Stock solutions

  • 200mM DTT in H2O (store as 50μL aliquots at -20°C and thaw just before use).
  • 100mM PMSF in ethanol (store at -20°C; half-life in aqueous solution is ~30 minutes).
  • 4M NaCl (store at RT)
  • 20% SDS (w/v) (store at RT)
  • 1M Tris-HCl, pH 8.5 (store at RT)
  • 50mM Tris-HCl, pH 8.5 (store at 4°C)

For protease inhibitors, we use:

  • AEBSF, HCl, MW=239.5, targets serine proteases, 100 mM
  • E-64, MW=357.4, targets cysteine proteases, 1.5 mM
  • Pepstatin A, MW=685.9, targets aspartic proteases, 2 mM
  • o-Phenanthroline, MW=198.2, targets metalloproteases, 500 mM

This mixture is commercially available as Calbiochem protease inhibitor cocktail set IV, or BioVision EZBlock protease inhibitor cocktail IV.

Soluble Protein Buffer, pH 8.5 (SPB)

(50mM Tris-HCl, 500mM NaCl, 1:100 protease inhibitors)

Start by making 50 mL SPB stock solution:

  • 2.5 mL 1M Tris-HCl, pH 8.5
  • 6.25 mL 4M NaCl
  • 41.25 mL protease-free H2O

Then mix 9.8 mL of SPB stock solution with 100 µL 100mM PMSF and 100uL protease inhibitors to make 10mL SPB.

Wash Buffer (WB)

(50mM Tris-HCl, 150mM NaCl, 1:100 protease inhibitors) Same as SPB, but with reduced salt to limit pellet loss.

Start by making 50 mL WB stock solution:

  • 2.5 mL 1M Tris-HCl, pH 8.5
  • 1.875 mL 4M NaCl
  • 45.625 mL protease-free H2O

Then mix 9.8 mL of WB stock solution with 100 µL 100mM PMSF and 100µL protease inhibitors to make 10mL WB.

Insoluble Protein Buffer, pH 8.5 (IPB)

(50mM Tris-HCl, 150mM NaCl, 8M urea, 2% SDS, 1mM PMSF, 2mM DTT, 1:1000 protease inhibitors) Make fresh just before each use. Note that at 8M, urea occupies ~72% of the solution volume, so that 4.8g urea occupies 7.2mL of a 10mL solution. Do not use 500mM NaCl in this solution, as it loosens pellets and causes sample loss.

  • 8M urea
  • 2% SDS
  • 50mM Tris pH 8.5
  • 150mM NaCl
  • 1mM PMSF
  • 20 μL 200mM DTT
  • 1:1000 protease inhibitors (see above. higher concentrations may crash out.)

Use 500μL IPB per sample, and note that foaming will make ~25% of the solution unusable.

2mL IPB (~2 samples) 13mL IPB (~10 samples)
  • 0.96g urea
  • 683 μL H2O
  • 200 μL 20% SDS (w/v)
  • 100 μL 1M Tris pH 8.5
  • 75 μL 4M NaCl
  • 20 μL 100mM PMSF
  • 20 μL 200mM DTT
  • 2 μL protease inhibitors
  • 6.24g urea
  • 5.58 mL H2O
  • 1.3 mL 20% SDS (w/v)
  • 650 μL 1M Tris pH 8.5
  • 488 μL 4M NaCl
  • 130 μL 100mM PMSF
  • 130 μL 200mM DTT
  • 13 μL protease inhibitors

6x Soluble Protein Loading Buffer, pH 6.8 (SPLB)

(50 mM Tris-HCl pH 6.8, 10% SDS, 0.05% bromophenol blue, 30% glycerol, 5% β-mercaptoethanol [βME])

Start by making 9 mL 6x SPLB Stock Solution:

  • 0.5 mL 1M Tris-HCl, pH 6.8
  • 1 g SDS
  • 5 mg bromophenol blue
  • 3 mL glycerol
  • 5.5 mL protease-free water

Then mix 712.5 µL of 6x SPLB stock solution with 37.5 µL of 14.3M βME immediately before use.

6x Soluble Protein Storage Buffer, pH 8.5 (SPSB)

(50 mM Tris-HCl pH 8.5, 12% SDS, 5% β-mercaptoethanol [βME])

Start by making 10 mL 6x SPSB Stock Solution:

  • 0.5 mL 1M Tris-HCl, pH 8.5
  • 6 mL 20% SDS
  • 3.5 mL protease-free water

Then mix 712.5 µL of 6x SPSB stock solution with 37.5 µL of 14.3M βME immediately before use.

6x Insoluble Protein Loading Buffer, pH 6.8 (IPLB)

(50 mM Tris-HCl, 0.05% bromophenol blue, 30% glycerol, 5% βME)

Start by making 9 mL 6x IPLB Stock Solution (nearly the same as SPLB stock, but

  • 0.5 mL 1M Tris-HCl, pH 6.8
  • 5 mg bromophenol blue
  • 3 mL glycerol
  • 5.5 mL protease-free water

Then mix 475 µL of 6x IPLB stock solution with 25 µL 14.3M βME immediately before use.

Protocol

Day -2

  • For each strain, inoculate a 3 mL YPD pre-culture of YPD with a single yeast colony and incubate overnight at 30⁰C with shaking or rotation.

Day -1

  • Inoculate 50 mL of synthetic complete medium (SC) with labeled amino acids with 3 µL of the overnight pre-culture and incubate for 18 h at 30⁰ C with shaking in a 500 mL baffled flask.

Day 0

Cell preparation

  • Grow 50mL culture of cells to a density of 4×106 cells/mL (OD600 ≈ 0.4).

While cells are growing, make solutions: SPB, WB, IPB. Put 1.1 mL × number of samples' worth of 50mM Tris-HCl pH 8.5 on ice.

  • Transfer 1.4×108 cells to a 50mL conical tube (35 mL of a 4×106 cells/mL culture)
  • Spin at 3000g for 1 minute.
  • Gently decant and discard supernatant.
  • Resuspend cell pellet in 1.4mL ice-cold Tris (50mM, pH 8.5) and transfer to 1.5mL microcentrifuge tube.
  • Spin at 20,000g for 15 seconds.
  • Discard supernatant, clear residual liquid with a hard snap.
  • Freeze pellet in liquid nitrogen.

Now decide whether you want total protein extraction or soluble/insoluble fractionation.

Lysis for soluble/insoluble fractionation

  • For each strain, rack a 2mL flat or round-bottom microcentrifuge tube in LN2 and place a 7mm stainless-steel ball (Retsch #05.368.0035) inside. Put some LN2 in tube to speed cooling of ball and to catch the incoming sample. Label the sides as well as the tops of the tubes, as lysis will often crack off the tube cap.
  • Resuspend frozen pellet in 50 µL SPB.
  • Drip resuspended pellet onto upper wall of tube containing ball. Goal is to get a nugget of frozen material on the wall, and to avoid dripping the material around the ball and thus freezing the ball to the bottom of the tube; having some LN2 remaining in the tube helps.
  • When all LN2 has boiled out of tube (listen -- if any popping or hissing, keep waiting), snap tube closed. Keep in LN2. (Any remaining LN2 in tube will cause tube to explode open and fire the stainless steel ball into your iPad, brain, colleague, or other important equipment.)
  • Rack the tube into the PTFE 2mL tube adaptor for the Retsch Mixer Mill MM400 (Retsch #22.008.0005) and submerge the entire assembly in LN2.
  • Agitate for 4×90 seconds at 30 Hz in a Retsch Mixer Mill MM400, returning sample holder to LN2 between sessions. Complete lysis produces fine snowy powder in the tube.
  • Remove sample tubes from LN2 and pop the caps to relieve pressure.
  • Add 450 μL SPB to each tube, and extract ball with a magnet. We rinse balls in methanol and store in 50% ethanol.
  • Move 500 μL sample to a fresh 1.5mL microcentrifuge tube.

Soluble fraction extraction

  • Spin at 3000g for 30 seconds (clarification step).
  • Decant clarified liquid into a 1.5mL polyallomer conical centrifuge tube (Beckman Coulter).
  • Spin at 100,000g for 20 minutes (fixed-angle TLA-55 rotor at 40,309 rpm in a Beckman Coulter Optimax tabletop ultracentrifuge).
  • Decant supernatant into a 1.5mL microcentrifuge tube: this is the soluble fraction.

Insoluble fraction extraction

  • Violently snap pellet to clear remaining liquid.
  • Add 500 μL wash buffer (WB) and vortex violently. (The pellet may not resuspend; that's fine.)
  • Spin at 100,000g for 20 minutes.
  • Discard supernatant, clear residual liquid with a hard snap.
  • Add 500 μL insoluble protein buffer (IPB).
  • Vortex until pellet dissolves, 10-15 minutes for clarified samples.
  • Spin at 20,000g for 5 minutes.
  • Decant supernatant into a 1.5mL microcentrifuge tube: this is the insoluble fraction.

Lysis for total protein extraction

  • For each strain, rack a 2mL flat or round-bottom microcentrifuge tube in LN2 and place a 7mm stainless-steel ball (Retsch #05.368.0035) inside. Put some LN2 in tube to speed cooling of ball (ultimately we want all the LN2 to boil away).
  • Resuspend frozen pellet in 50 µL insoluble protein buffer (IPB).
  • Drip resuspended pellet onto upper wall of tube containing ball. Goal is to get a nugget of frozen material on the wall, and to avoid dripping the material around the ball and thus freezing the ball to the bottom of the tube.
  • When all LN2 has boiled out of tube (listen -- if any popping or hissing, keep waiting), snap tube closed. Keep in LN2. (Any remaining LN2 in tube will cause tube to explode open and fire the stainless steel ball into your iPad, brain, colleague, or other important equipment.)
  • Rack the tube into the PTFE 2mL tube adaptor for the Retsch Mixer Mill MM400 (Retsch #22.008.0005) and submerge the entire assembly in LN2.
  • Agitate for 4×90 seconds at 30 Hz in a Retsch Mixer Mill MM400, returning sample holder to LN2 between sessions. Complete lysis produces fine snowy powder in the tube.
  • Add 450 μL IPB to tube, and extract ball with a magnet.
  • Move 500 μL sample to a fresh 1.5mL microcentrifuge tube.
  • Spin at 20,000g for 5 minutes.
  • Decant supernatant into a 1.5mL microcentrifuge tube: this is the total protein fraction.


Storage

For insoluble and total-protein fractions, make 100μL aliquots and store at -80°C.

For soluble fractions, mix 5:1 with fresh 6x soluble protein storage buffer (SPSB), denature for 5 minutes at 95°C, make 100μL aliquots and store at -80°C.

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