Gel electrophoretic separation of globin chains
- PMID: 7279969
Gel electrophoretic separation of globin chains
Abstract
The globin chains of human embryonic, fetal, and adult hemoglobins can be separated by electrophoresis on gels containing polyacrylamide, acid, urea, and Triton X-100. Whole hemolysates are used, and only microgram quantities are required. The order of the major human erythrocyte proteins, from anode to cathode, is zeta, epsilon, carbonic anhydrase, A gamma, delta and G gamma together, beta, and alpha. Protein composition can be measured on Coomassie blue-stained disc gels, and protein synthesis on fluorograms of slab gels containing 3H-leucine-labelled material. These gels have been used to examine the ratio of G gamma to A gamma in blood from fetuses and newborn infants, and to suggest that the switch from A gamma to G gamma during ontogeny may not be linked to the switch from gamma to beta production. beta/gamma synthetic ratios were determined in fetuses at risk for thalassemia. Embryonic and fetal globin synthesis ratios were measured in hemin-induced human erythroleukemia cells K562 in tissue culture. Fetal globin synthesis and the proportion that was of the "fetal" type (G gamma approximately 70%) was studied in erythroid colonies grown in plasma clot cultures from adult, newborn, and 6 month infant specimens. The gels provide a rapid, simple, and inexpensive approach to many problems of globin composition and synthesis.
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