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Protein Protocols Protein Protocols

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1140 Index<br />

Auroprobe BL plus, 397–398<br />

Autoradiography, 307–310, 605–606<br />

Avidin-biotin, 355, 415–418<br />

Avidin conjugation, 365–373<br />

B<br />

Basic proteins<br />

blotting of, 337–340<br />

electrophoresis of, 103–111, 113–122<br />

BCA Assay, 11-14, 27–30<br />

Beer-Lambert law, 4<br />

Bicinchoninic acid assay (see BCA Assay)<br />

Biotin labeling, 355–362<br />

Bispecific antibodies, 1053–1058<br />

Blocking solutions, 330–332<br />

Blots, re-use of, 439–451<br />

Blotting (see <strong>Protein</strong> blotting)<br />

Blotting buffers, 324–326<br />

Blotting membranes, 327–328<br />

BNPS Skatole, 494, 549<br />

Bolton and Hunter reagent, 969–970<br />

Bovine serum albumin<br />

Bradford assay standard, 19<br />

UV absorbance of, 5<br />

Bradford Method, 15–20<br />

N-Bromosuccinimide, 495, 549<br />

C<br />

Calconcarboxylic acid stain, 259–262<br />

Capillary blotting, 335–336<br />

Capillary electrophoresis of carbohydrates,<br />

907–908<br />

Caprylic acid, IgG purification, 985<br />

Carbamoylation, 135<br />

Carbodiimide conjugation, 955–956, 958<br />

Carbohydrate, biotin labeling, 359–360<br />

Carboxyl groups, amidation of, 477–478<br />

Carboxymethylation, 455–456<br />

Carrier ampholytes (see Ampholytes)<br />

CAT gel electrophoresis,87–100<br />

Cell lysis, 1102–1104<br />

Cetyltrimethylammonium bromide (CTAB),<br />

87<br />

Chaotropes, 133–134<br />

Chemifluorescence, 421–428<br />

Chloraminde T, 963–964<br />

Chymostatin, 1099<br />

Chymotrypsin, 513–514, 549<br />

Cisplatin, 747<br />

Cleveland peptide mapping, 553–557<br />

Clostripain, 524<br />

Coomassie Brilliant Blue, 58, 64, 67, 94, 390<br />

Coomassie Brilliant Blue G, 238–240<br />

Copper iodide staining, 381–385<br />

CTAB electrophoresis, 87–99<br />

Cyanogen bromide cleavage<br />

at Met, 485–490<br />

at Trp, 494<br />

Sepharose activation, 1000<br />

Cysteine (see also Disulfide bridges)<br />

carboxymethylation of , 455–456<br />

cleavage at, 503–505<br />

quantitation of, 597–601<br />

performic acid oxidation of, 457–458<br />

pyridylethylation of, 461-462<br />

reaction with DTNB, 483–484, 595–596<br />

D<br />

2-D PAGE (see Two-dimensional PAGE)<br />

Databases for 2-D gels, 198–199<br />

Detergents, 134–135, 1098<br />

Diagonal electrophoresis, 589-593<br />

Diazo coupling, 959<br />

Difference gel electrophoresis, 185–196<br />

DIG (anti-DIG AP labeling of<br />

carbohydrates), 765–766<br />

Digoxigenin labeling, 349–350<br />

Direct Blue 71, 387–391<br />

Disulfide bridges<br />

detection by<br />

diagonal electrophoresis, 589–593<br />

HPLC, 581–583<br />

mass spectrometry, 585–587<br />

disruption of, 133<br />

estimation with Ellman’s reagent,<br />

483–484, 595–596<br />

Dithiothreitol, 133<br />

Double replica blotting, 222<br />

DTNB (see Ellman’s reagent)<br />

E<br />

E64, 1099<br />

ECL, 218–219, 223, 429–436<br />

immunoassay, 1089–1094<br />

Edman degradation, 736<br />

Electroblotting, 217-218, 317–319,<br />

321–333, 337–340<br />

Electroelution, 299–304

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