Peptide-Based Drug Design

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18 Bulet 3. Centrifuge between 8000 and 12,000g (30 min, 4 ◦ C) to remove lipids (upper phase), denaturized proteins, and debris. If necessary, the supernatant can be clarified by an additional step with filter units (0.8-�m membranes, Millipore). 3.2.3. Extraction from Hemocytes, Epithelia, and Salivary Glands 1. Thaw the sample (hemocytes, epithelia) on ice if not freshly prepared. 2. The salivary glands are snap-frozen in liquid nitrogen. 3. Homogenize (see Note 7) using sonication (3 × 30 s) at medium power in the presence of 2 M acetic acid (in an ice-cold water bath, a solution of 0.2 M acetic acid is also an option to decrease the protein content of the extracted material). Extract overnight at 4 ◦ C under gentle stirring in 2 M acetic acid supplemented with a protease inhibitor (e.g., aprotinin). 4. Centrifuge between 8000 and 12,000g (30 min, 4 ◦ C) to separate the supernatant (cytosolic fraction) from the organelle-rich fraction or tissue debris (pellet). If necessary, the supernatant can be clarified by additional step with filter units (0.8-�m membranes, Millipore). 3.3. Purification of the Natural Bioactive <strong>Peptide</strong>s Because of their well-recognized physicochemical properties (relatively high hydrophobicity, cationic character, and short length) reversed-phase, sizeexclusion, and cation exchange chromatographies are particularly appropriate to purify bioactive peptides from the immune system of invertebrates. The sensitivity of HPLC, MS, Edman degradation, and liquid growth inhibition assays allow one to use from narrow (e.g., 2.1-mm internal diameter) down to microor nano-columns. 3.3.1. Prepurification To limit the co-precipitation of the peptides of interest with remaining proteins, the first purification step is performed either by SPE on open-columns or cartridges that supports large volumes of diluted extracts or using disposable Ultrafree-CL (Millipore) ultrafiltration (UF) cartridge units (both strategies can be combined, UF prior SPE or SPE prior UF; see ref. 28). Open columns can be bought manufactured (e.g., Sep-Pak cartridges, WatersTM ) or handmade (bulk phase available, e.g., from WatersTM ). 3.3.1.1. SOLID-PHASE EXTRACTION This procedure has been already reported in ref. 22.Briefly: 1. Solvate the cartridge with methanol and equilibrate with acidified water (0.05% TFA). 2. Load the acidified extract (pH < 4).
Bioactive <strong>Peptide</strong>s in Invertebrate Immune Systems 19 3. Elute in a stepwise fashion with increasing percentages of acetonitrile prepared in acidified water: 40 and 80% (see Note 8) with 5–10 times the hold-up volume of the column (see manufacturer instructions). 4. Remove the organic solvent by lyophilization/freeze-drying or centrifugation under vacuum. 5. Reconstitute the fractions in MilliQ water (Millipore) and keep them at 4 ◦ C for immediate biological activity screening (see Note 9) or in the freezer until use. 3.3.1.2. ULTRAFILTRATION (UF PRE-SPE) 1. Dilute the extract in a large volume of 0.1% TFA. 2. Filter the diluted extract according to the manufacturer’s recommendations. 3. Load the filtrate onto the equilibrated SPE cartridge and pursue the SPE procedure. 3.3.1.3. ULTRAFILTRATION (UF POST-SPE) 1. Filter the reconstitute fractions eluted during SPE (see Subheading 3.3.1.1.). 2. Dry under vacuum and store at -20◦C until use. 3.3.2. Purification by HPLC In general, the first step of purification of the fractions eluted from SPE, SPE-UF, or UF-SPE is subjected to RP-HPLC followed either by a second RP- HPLC or by size exclusion chromatography (SEC-HPLC). The last step is often a highly sensitive RP-HPLC using highly selected elution conditions (gradient with a soft slope, low flow rate, and high sensitivity detection). However, before finalizing purification, several steps may be requested (at least three steps are needed to get a sufficient amount [1 nmol or 100 �g] of highly pure [>98%] material for structural characterization either by Edman chemistry or MS strategies (enzymatic digestion, on-line or off-line micro-RP-HPLC mass fingerprints, MSn sequencing). 3.3.2.1. STEP 1: REVERSED-PHASE HPLC (SEE NOTE 10) 1. Load the sample on an appropriate RP column (internal diameter of the column chosen according to the starting biological material available, 300 ˚A for granulometry, internal diameter from 3.8 to 7 mm, a C18 or C8 column is recommended for step 1). It is recommended to equilibrate the column with 2% acetonitrile in acidified water (0.05 % TFA) to remove the hydrophilic molecules and to properly stack the interesting material. 2. Elute the peptides with a linear gradient of acetonitrile in acidified water at a flow rate between 0.8 and 1.3 mL/min depending of the internal diameter of the column. Flow rate can be 0.8–1 mL/min if the column has 4.6 mm of internal diameter and increased to 1.3 mL/min for a semi-preparative column (7 mm of
Page 2 and 3: Peptide-Based Drug Design
Page 4 and 5: METHODS IN MOLECULAR BIOLOGY TM Pep
Page 6 and 7: Preface Natural products chemistry
Page 8 and 9: Contents Preface...................
Page 10 and 11: Contributors Nikolinka Antcheva •
Page 12 and 13: Contributors xi Alessandro Tossi
Page 14 and 15: 2 Otvos advance of computer power a
Page 16 and 17: 4 Otvos see derivatives active in b
Page 18 and 19: 6 Otvos was designed based on ligan
Page 20 and 21: 8 Otvos 27. Borghouts, C., Kunz, C.
Page 22 and 23: 10 Bulet Key Words: Invertebrate im
Page 24 and 25: 12 Bulet 6. 5 �L or higher volume
Page 26 and 27: 14 Bulet 2.5.2.1. MALDI-TOF-MS 1. M
Page 28 and 29: 16 Bulet 7. Small-volume low-protei
Page 32 and 33: 20 Bulet internal diameter). Increa
Page 34 and 35: 22 Bulet interest. As no instrument
Page 36 and 37: 24 Bulet 3. Incubate the plates in
Page 38 and 39: 26 Bulet bioactive peptides from th
Page 40 and 41: 28 Bulet 21. Chernysh, S., Kim, S.I
Page 42 and 43: 3 Sequence Analysis of Antimicrobia
Page 44 and 45: Sequence Analysis of Antimicrobial
Page 58 and 59: 4 The Spot Technique: Synthesis and
Page 60 and 61: The Spot Technique 49 3. For amine
Page 62 and 63: The Spot Technique 51 2. Biotinylat
Page 64 and 65: The Spot Technique 53 the solutions
Page 66 and 67: The Spot Technique 55 solution. Ens
Page 68 and 69: The Spot Technique 57 (see Fig. 3)
Page 70 and 71: The Spot Technique 59 Fig. 5. Princ
Page 72 and 73: The Spot Technique 61 library, the
Page 74 and 75: The Spot Technique 63 7. Regenerati
Page 76 and 77: The Spot Technique 65 following rul
Page 78 and 79: 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
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Proline-Rich Antimicrobial Peptides
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10 Serum Stability of Peptides Håv
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Serum Stability of Peptides 179 2.
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Serum Stability of Peptides 183 �
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11 Preparation of Glycosylated Amin
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Glycosylated Amino Acid Synthesis 1
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12 Synthesis of O-Phosphopeptides o
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Solid-Phase Synthesis of O-Phosphop
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13 Peptidomimetics: Fmoc Solid-Phas
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Peptidomimetics 225 O O R S N H Pep
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Peptidomimetics 227 not without its
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Peptidomimetics 229 Oxidation step:
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Peptidomimetics 231 of peptidosulfo
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Peptidomimetics 233 8. Allow the re
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Peptidomimetics 235 3.3.2. Solid-Ph
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Peptidomimetics 237 On the other ha
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Peptidomimetics 239 nitrogen (73).
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Peptidomimetics 241 3. Cover the re
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Peptidomimetics 243 efficient synth
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Peptidomimetics 245 55. Alsina, J.,
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14 Synthesis of Toll-Like Receptor-
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Lipopeptides 249 2. Materials 2.1.
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Lipopeptides 251 Fig. 1. Structural
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Lipopeptides 253 8. To enable lipid
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Lipopeptides 255 Representative res
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Lipopeptides 257 Fig. 2. Immunogeni
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Lipopeptides 259 8. A large plastic
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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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