Peptide-Based Drug Design

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Solid-Phase Synthesis of O-Phosphopeptides 213 a) Eluent A: Water (see Notes 7 and 8) containing 0.1% TFA as ion pair reagent. b) Eluent B: 60% aqueous acetonitrile containing 0.1% TFA (see Note 9). 5. Analytical separation: Inject 20- to 50-�g sample and keep the starting conditions of 5% eluent B for 2 min. Elute the peptides with a linear increase of 3% eluent B per min to 95% eluent B using a flow rate of 1 mL/min. Hold these conditions for 5 min before equilibrating the column again with 5% eluent B for at least 15 min. 6. Preparative separation: Purify up to 40 mg crude peptide in a single separation using 5% eluent B as starting conditions. After 2 min increase the content of eluent B to 95% using a linear gradient of 1–3% acetonitrile per minute and a flow rate of 10 mL/min (see Note 10). The slope of the gradient depends on the number of by-products eluting close to the target peptide. Hold the final conditions of 95% eluent B for 5 min before equilibrating the column with the starting conditions of 5% eluent B. 7. Detection: Absorption at 220 nm (see Note 11). 2.5. Mass Spectrometry 1. MALDI-TOF/TOF-MS (4700 Proteomics Analyzer, Applied Biosystems GmbH, Darmstadt, Germany). 2. �-Cyano 4-hydroxy-cinnamic acid (CHCA) matrix: a) Weigh 2 mg α-cyano 4-hydroxy-cinnamic acid (Bruker Daltonics GmbH, Bremen, Germany, store at 4 ◦ C) in a microcentrifuge tube and dissolve in 250 �L water containing 0.1% TFA. b) Vortex the solution for 10 s. c) Add 250 �L acetonitrile (HPLC grade). d) Vortex well until the matrix is completely dissolved. e) Store at −20 ◦ C. This solution can be used for one month. 3. �-Cyano 4-hydroxy-cinnamic acid with phosphate (pCHCA) matrix: a) Prepare a fresh matrix solution as described above. b) Add ammoniumphosphate (ultra ≥99.5%, Fluka) to the matrix solution to a final concentration of 10 mM. c) Store at −20◦C. This solution can be used for one month. 4. 2,5-Dihydroxybenzoic acid (DHB) matrix: a) Weigh approximately 5 mg 2,5-dihydroxybenzoic acid (Bruker Daltonics, store at 4 ◦ C) exactly in a 1.5-mL Eppendorf tube. b) Add 450 �L water and 450 �L methanol (calculated for 5 mg matrix, adjust according the weighed amount). c) Vortex well until the matrix is completely dissolved. d) Store at −20 ◦ C. This solution can be used for up to one month.
214 Singer and Hoffmann 3. Methods There are two general strategies to synthesize phosphopeptides by Fmoc chemistry. First, the postsynthetic global phosphorylation approach (7,9) incorporates an Fmoc-protected Ser, Thr, or Tyr without side-chain protection. An obvious advantage of this approach is that both the unmodified and phosphorylated peptides can be obtained from a single synthesis by splitting the resin after the peptide synthesis prior to phosphorylation. The second approach incorporates phosphorylated Fmoc amino acid derivatives carrying TFA-labile protecting groups in the side chain, referred to as the building block strategy. Both methods have inherent advantages and disadvantages, but usually work well for singly phosphorylated peptides up to 20 residues in length. For longer or multiply phosphorylated peptides, the appropriate strategy has to be selected depending on the peptide sequence and the number of residues to be phosphorylated. Moreover, it might be necessary in some cases to optimize the heredescribed standard protocols for “difficult” sequences by using longer reaction times or a higher reagent excess. Alternatively, the purification strategy has to be optimized to separate the desired phosphopeptide from by-products. For the synthesis of monophosphorylated peptides with “easy-to-synthesize” sequences containing no bulky side chains or protecting groups proximal to the phosphorylation site, the direct incorporation of monobenzyl protected phosphoserine (10), phosphothreonine (6), and phosphotyrosine (4) is usually preferred, as standard peptide synthesis reagents are used and no additional postsynthetic handling steps are required (see Note 12). For multiply phosphorylated peptides and especially for proximal phosphorylation sites, we prefer the global phosphorylation approach. This strategy is also more efficient and cost saving if several phosphopeptides or the corresponding unmodified peptides are synthesized, for example, in a parallel peptide synthesis. 3.1. Multiple Solid Phase <strong>Peptide</strong> Synthesis 1. Swell the resin in DMF for 30 min (e.g., 40 mg Rink-amide MBHA resin, 25 �mol amino groups). 2. Add 1 mL piperidine (40% by vol. in DMF) and discard after 3 min. 3. Add 1 mL piperidine (20% by vol. in DMF) for 10 min and remove. 4. Wash the resin six times with 1 mL DMF for 1 min each. 5. Prepare a solution of 0.5 M HOBt in DMF or in a mixture of NMP and DMF (1:1 by vol.). 6. Dissolve the desired amount of the Fmoc amino acids in the HOBt-solution to a final concentration of 0.5 M (see Note 13). 7. Add the amino acid solution from step 6 at a 4- to 10-fold molar excess over the amino groups of the resin (e.g., 200 �mol [8 eq] amino acid derivative corresponding to 400 �L Fmoc amino acid solution).
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Peptide-Based Drug Design
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METHODS IN MOLECULAR BIOLOGY TM Pep
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Preface Natural products chemistry
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Contents Preface...................
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Contributors Nikolinka Antcheva •
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Contributors xi Alessandro Tossi
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2 Otvos advance of computer power a
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4 Otvos see derivatives active in b
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6 Otvos was designed based on ligan
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8 Otvos 27. Borghouts, C., Kunz, C.
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10 Bulet Key Words: Invertebrate im
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12 Bulet 6. 5 �L or higher volume
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14 Bulet 2.5.2.1. MALDI-TOF-MS 1. M
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16 Bulet 7. Small-volume low-protei
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18 Bulet 3. Centrifuge between 8000
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20 Bulet internal diameter). Increa
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22 Bulet interest. As no instrument
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24 Bulet 3. Incubate the plates in
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26 Bulet bioactive peptides from th
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28 Bulet 21. Chernysh, S., Kim, S.I
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3 Sequence Analysis of Antimicrobia
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Sequence Analysis of Antimicrobial
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4 The Spot Technique: Synthesis and
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The Spot Technique 49 3. For amine
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The Spot Technique 51 2. Biotinylat
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The Spot Technique 53 the solutions
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The Spot Technique 55 solution. Ens
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The Spot Technique 57 (see Fig. 3)
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The Spot Technique 59 Fig. 5. Princ
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The Spot Technique 61 library, the
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The Spot Technique 63 7. Regenerati
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The Spot Technique 65 following rul
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The Spot Technique 67 20. Atherton,
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The Spot Technique 69 50. Bolger, G
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5 Analysis of A� Interactions Usi
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Analysis of Aβ Interactions 73 are
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Analysis of Aβ Interactions 75 Ana
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Analysis of Aβ Interactions 77 3.
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6 NMR in Peptide Drug Development J
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NMR of Peptides 89 usually require
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NMR of Peptides 91 limiting the siz
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NMR of Peptides 93 and STD NMR expe
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NMR of Peptides 95 The basis of the
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NMR of Peptides 97 Fig. 5. Overlay
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NMR of Peptides 99 Fig. 7. Schemati
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NMR of Peptides 101 4.4.2. Saturati
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NMR of Peptides 103 4.6. Diffusion
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NMR of Peptides 105 Fig. 13. Propos
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NMR of Peptides 107 protein prevent
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NMR of Peptides 109 6. Wuthrich, K.
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NMR of Peptides 111 45. Morris, K.
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NMR of Peptides 113 78. Aumailley,
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116 Copps et al. Fig. 1. Potential
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118 Copps et al. Fig. 2. Flowchart
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120 Copps et al. 10. In accordance
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122 Copps et al. Fig. 3. DSSP for g
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124 Copps et al. ingly with the sam
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126 Copps et al. 19. Essman, U., Pe
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128 Hilpert et al. Key Words: Scree
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130 Hilpert et al. Table 1 (Continu
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132 Hilpert et al. different natura
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134 Hilpert et al. wt A C D E F …
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136 Hilpert et al. methods primaril
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144 Hilpert et al. Table 3 Summary
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148 Hilpert et al. of substituting
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150 Hilpert et al. in models that c
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152 Hilpert et al. than control. Gi
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154 Hilpert et al. Table 4 Accuracy
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156 Hilpert et al. 25. Pini, A., Gi
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158 Hilpert et al. 55. Giacometti,
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9 Investigating the Mode of Action
Page 172 and 173: Proline-Rich Antimicrobial Peptides
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Page 188 and 189: Serum Stability of Peptides 179 2.
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Page 196 and 197: 11 Preparation of Glycosylated Amin
Page 198 and 199: Glycosylated Amino Acid Synthesis 1
Page 218 and 219: 12 Synthesis of O-Phosphopeptides o
Page 220 and 221: Solid-Phase Synthesis of O-Phosphop
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Page 234 and 235: Peptidomimetics 225 O O R S N H Pep
Page 236 and 237: Peptidomimetics 227 not without its
Page 238 and 239: Peptidomimetics 229 Oxidation step:
Page 240 and 241: Peptidomimetics 231 of peptidosulfo
Page 242 and 243: Peptidomimetics 233 8. Allow the re
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Page 248 and 249: Peptidomimetics 239 nitrogen (73).
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Page 252 and 253: Peptidomimetics 243 efficient synth
Page 254 and 255: Peptidomimetics 245 55. Alsina, J.,
Page 256 and 257: 14 Synthesis of Toll-Like Receptor-
Page 258 and 259: Lipopeptides 249 2. Materials 2.1.
Page 260 and 261: Lipopeptides 251 Fig. 1. Structural
Page 262 and 263: Lipopeptides 253 8. To enable lipid
Page 264 and 265: Lipopeptides 255 Representative res
Page 266 and 267: Lipopeptides 257 Fig. 2. Immunogeni
Page 268 and 269: Lipopeptides 259 8. A large plastic
Page 270 and 271: Lipopeptides 261 26. Nardin, E.H.,
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264 Otvos response, synthetic pepti
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266 Otvos Fig. 3. Schematic present
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268 Otvos 3. Methods The main goal
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270 Otvos 3.2.3. Purification and Q
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272 Otvos 6. Meyer, D., and Torres,
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16 Cysteine-Containing Fusion Tag f
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Targeted Therapeutic and Imaging Ag
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Index A A� peptides aggregation a
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Index 297 phosphopeptides influenci
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Index 299 for genetically synthetic
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Index 301 peptidosulfonamide, disad
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Index 303 solid phase, 180, 214 sul
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Peptide-Based Drug Design

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