Fig. 6.
Fig. 6. 2D gels of tryptic peptides from spectrin dimers and α dimerization site recombinant peptides. Isofocusing was in the horizontal direction (basic side on the left) followed by separation on a 12% SDS gel that was stained with Coomassie Brilliant Blue. (A) Two hundred micrograms of spectrin digested with trypsin from a normal donor; (B) 200 μg of spectrin digested with trypsin from a donor homozygous for the αLELY mutation; (C through E) 20 μg of each recombinant spectrin peptide digested with trypsin. (C) α18-21; (D) α18-211857; (E) α18-211857-Δ46. Arrows indicate the position of the normal αV 41-kD tryptic domain in all panels. The arrowheads indicate the major αIV domain peptides in (A) and (B).

2D gels of tryptic peptides from spectrin dimers and α dimerization site recombinant peptides. Isofocusing was in the horizontal direction (basic side on the left) followed by separation on a 12% SDS gel that was stained with Coomassie Brilliant Blue. (A) Two hundred micrograms of spectrin digested with trypsin from a normal donor; (B) 200 μg of spectrin digested with trypsin from a donor homozygous for the αLELY mutation; (C through E) 20 μg of each recombinant spectrin peptide digested with trypsin. (C) α18-21; (D) α18-211857; (E) α18-211857-Δ46. Arrows indicate the position of the normal αV 41-kD tryptic domain in all panels. The arrowheads indicate the major αIV domain peptides in (A) and (B).

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