Direct Enzymatic Digestion of Protein Complexes for MS Analysis

doi:10.1101/pdb.prot4662

Cite as: Cold Spring Harb. Protoc.; 2006; doi:10.1101/pdb.prot4662

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protocol Protocol

Direct Enzymatic Digestion of Protein Complexes for MS Analysis

Sherry Niessen, Ian Mcleod, and John R. Yates, III

This protocol was adapted from "Identification of Novel Protein Complexes and Protein-Protein Interactions by Mass Spectrometry," Chapter 18, in Protein-Protein Interactions, 2nd ed. (eds. Golemis and Adams). Cold Spring Harbor Laboratory Press, Cold Spring Harbor, NY, USA, 2005.

INTRODUCTION

The individual components of a purified protein complex canbe determined by MS. Components can be separated by SDS-PAGEand subsequently digested, or the entire protein complex canbe digested by chemical agents or by proteases. The mixtureof peptides that results from digestion without prior separationis more complex than that obtained from the digestion of a singleprotein, and can best be resolved subsequently using HPLC incombination with a biphasic column. Protein complexes can bedigested directly using several different protocols. Commonmethods include a double digest with endoproteinase Lys-C andtrypsin, or a triple digest with elastase, subtilisin, and trypsin.Endoproteinase Lys-C cleaves carboxy-terminal to lysine residues,while trypsin cleaves carboxy-terminal to lysine and arginineresidues. The triple digest uses the relatively nonspecificproteases elastase and subtilisin to create a large number ofoverlapping peptides for the analysis of post-translationalmodifications. The double and triple digest protocols beginwith the reduction and alkylation of cysteine residues to disruptdisulfide bonds and, therefore, higher-order protein structure.

RELATED INFORMATION

See Overview of Affinity Purification in Combination with Mass Spectrometry.

Materials

Reagents

Acetone, ice cold

CaCl₂, 1 M

Elastase Grade II (Roche)

Endoproteinase Lys-C (Roche)

Formic acid, 90%

Iodoacetamide (IAA), 500mM (Sigma)

Prepare fresh before each use.

Protein complex of interest, in solution

Subtilisin (Boehringer Mannheim)

Trichloroacetic acid (TCA),20%

Tris (2-carboxyethyl)-phosphinehydrochloride (TCEP), 100 mM (Pierce)

Tris-HCl, 100 mM (pH 8.0)(Sigma)

Trypsin, sequencing grade,modified (Promega)

Urea/Trissolution

Over time, urea breaks down into ammonium cyanate, which cancause carbamylation of the amino termini of peptides as wellas lysine and arginine side chains. It is therefore essentialto prepare the urea/Tris solution fresh before each use.

Equipment

Incubator, 37°C

Microcentrifuge, 4°C

METHOD

Precipitation and Preparation of Purified Protein Complexes

1. Add an equal volume of 20% TCA to the protein sample (theprotein concentration will vary depending on the experiment).Incubate for 30 minutes on ice.

2. Centrifuge the sample at12,000g in a microfuge for 15 minutesat 4°C.

3. Carefullyremove all the supernatant. Add 300 µl ofcold acetone.Centrifuge at 12,000g for 5 minutes at 4°C.

4. Removethe supernatant. Air-dry the pellet.

5. Redissolve the proteinpellet in 50-100 µl of urea/Trissolution.

6. Add 100mM TCEP to the protein solution to a final concentrationof5 mM. Incubate for 20-30 minutes at room temperature.

7. Add500 mM freshly prepared IAA to a final concentrationof 10 mM.Incubate for 20-30 minutes in the dark at room temperature.

8. Digest the protein complex using one of the following methods:

For double digestion:

i. Add endoproteinase Lys-C to a finalconcentration of 0.002µg/µl. Incubate in the darkfor 4 hours at 37°C.
For complex mixtures of proteins,incubate the samples overnight.

ii. Dilute the sample to 2M urea by adding 100 mM Tris-HCl(pH 8.0).

iii. Add 1 M CaCl₂to a final concentration of 2mM. Add trypsinto a final concentrationof 0.01 µg/µl.Incubateovernight (12-24 hr) at37°C.

iv. After incubation,quench the digestion by adding90% formicacid to a final concentrationof 5%.
Store at -20°Cuntil needed for analysis by ESIMS/MS.

For triple digestion:

i. Divide the IAA-treated sample (from Step 7) into threealiquotsof equal volume.
Each aliquot will be treated witha differentprotease and thenpooled after digestion.

ii.Dilute Fractions1 and 2 to 2 M urea with 100 mM Tris-HCl(pH8.0). Dilute Fraction3 to 4 M urea with 100 mM Tris-HCl(pH8.0).

iii. To Fraction1, add 1 M CaCl₂ to a final concentrationof2 mM. Add trypsinto a final concentration of 0.01 µg/µl.Incubateovernight (12 hr) at 37°C.

iv. To Fraction 2,add elastaseto a final concentration of0.005 µg/µl.Incubatefor 4 hours at 37°C.
Store at -20°C untilFraction1 is ready.

v. To Fraction 3, add subtilisin to afinal concentrationof0.002 µg/µl. Incubate for4 hours at 37°C.
Store at -20°C until Fraction 1 isready.

vi. Afterdigestion, pool the three fractions.

vii.Quench the reactionsby adding 90% formic acid to a finalconcentrationof 5%.
Storeat -20°C until needed for analysis by ESIMS/MS.

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