Definition of regions in human c-myc that are involved in transformation and nuclear localization.

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Mol Cell Biol. 1987 May; 7(5): 1697-1709

Definition of regions in human c-myc that are involved in transformation and nuclear localization.

J Stone, T de Lange, G Ramsay, E Jakobovits, J M Bishop, H Varmus and W Lee

ABSTRACT

To study the relationship between the primary structure of thec-myc protein and some of its functional properties, we madein-frame insertion and deletion mutants of the normal humanc-myc coding domain that was expressed from a retroviral promoter-enhancer.We assessed the effects of these mutations on the ability ofc-myc protein to cotransform normal rat embryo cells with amutant ras gene, induce foci in a Rat-1-derived cell line (Rat-1a),and localize in nuclei. Using the cotransformation assay, wefound two regions of the protein (amino acids 105 to 143 and321 to 439) where integrity was critical: one region (aminoacids 1 to 104) that tolerated insertion and small deletionmutations, but not large deletions, and another region (aminoacids 144) to 320) that was largely dispensable. Comparisonwith regions that were important for transformation of Rat-1acells revealed that some are essential for both activities,but others are important for only one or the other, suggestingthat the two assays require different properties of the c-mycprotein. Deletion of each of three regions of the c-myc protein(amino acids 106 to 143, 320 to 368, and 370 to 412) resultedin partial cytoplasmic localization, as determined by immunofluorescenceor immunoprecipitation following subcellular fractionation.Some abnormally located proteins retained transforming activity;most proteins lacking transforming activity appeared to be normallylocated.

Mol Cell Biol. 1987 May; 7(5): 1697-1709

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