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Reexamination of Alcohol Dehydrogenase Structural Mutants in Drosophila Using Protein Blotting
Hope Hollocher 1 and Allen R. Place 1
1 Department of Biology, Leidy Laboratories, University of Pennsylvania,
Philadelphia, Pennsylvania 19104
Using protein blotting and an immuno-overlay procedure, we have reexamined the cross-reacting material produced by ADH null-activity mutants generated with ethyl methanesulfonate (EMS). Of the 13 mutants, 11 have an immunodetectable polypeptide of wild-type size. The native and urea denatured isoelectric points (pI) establish that 7 of 13 of the mutations have no effect on protein charge. The electrophoretic mobilities of each variant on increasing percent acrylamide gels (Ferguson analysis), reveal that 9 of the 11 immunodetectable mutants have retained the ability to form dimers under native conditions. None of the inactive mutant proteins has the ability to form the "adduct-bound" isozyme. We have found no correlation between protein pI and in vivo stability. The observed frequencies of specific charge class alterations do not dispute the propensity of G:A transitions previously found for EMS mutagenesis.
Submitted on October 16, 1986Accepted on March 10, 1987