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Peptide-Based Drug Design

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Sequence Analysis of Antimicrobial <strong>Peptide</strong>s 39<br />

O<br />

peptide<br />

H<br />

N peptide<br />

peptide<br />

N<br />

H<br />

O<br />

S<br />

S<br />

peptide<br />

DTT<br />

O<br />

2 peptide<br />

H<br />

N peptide<br />

SH<br />

I<br />

O<br />

O<br />

NH 2<br />

NH 2<br />

O<br />

peptide<br />

H<br />

N peptide<br />

S<br />

O<br />

NH 2<br />

O<br />

peptide<br />

H<br />

N peptide<br />

Scheme 1. Reduction of homodimer peptide linked via a disulfide bridge with dithiothreitol<br />

(DTT) and alkylation of the resulting thiol groups of both cysteines with either<br />

acrylamide (upper reaction) or iodoacetamide (lower reaction).<br />

3.5. Counting Cysteine Residues<br />

1. Determine the molecular masses of the alkylated peptide samples by nanoESI-MS<br />

in static mode using 2-�L sample or by MALDI-MS using either CHCA matrix<br />

or DHB matrix (see Subheadings 3.2.1. and 3.2.2.).<br />

2. Calculate the differences of the original peptide mass and the recorded masses after<br />

alkylation with iodoacetamide and acrylamide (e.g., the peptide mass was shifted<br />

from 4540.35 to 4972.84 g/mol and 4888.42 after reduction and alkylation with<br />

acrylamide and iodoacetamide, respectively, corresponding to mass differences of<br />

432.49 and 348.07 g/mol.).<br />

3. Determine the number of cysteine residues by dividing the mass difference calculated<br />

for the acrylamide sample by 72.08 and 58.05 g/mol for the iodoacetamide<br />

sample (e.g., the mass shift of 432.49 g/mol for acylamide and 348.07 g/mol<br />

for iodoacetamide correspond to six cysteine residues in both cases, i.e., three<br />

disulfide bonds in the original sample).<br />

3.6. Tryptic Digest<br />

1. If the peptide to be digested contains cysteine residues, reduce and alkylate them<br />

prior to any enzymatic digest (see Subheading 3.4.) using only 1 �L of either of<br />

the two alkylation reagents for 40 pmol peptide.<br />

2. Dry the peptide solution (40 pmol) in the SpeedVac and add 8 �L 3mMABC<br />

buffer.<br />

3. Add 2 �L trypsin solution and mix carefully by aspirating and dispensing 2 �Lof<br />

the solution several times with the tip.<br />

4. Split the sample in two parts of equal volume to 0.6-mL polypropylene vials (see<br />

Note 6).<br />

+<br />

+<br />

– HI<br />

S<br />

O<br />

NH 2

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