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Published April 1985 | public
Journal Article Open

Protein stabilization explains the gag requirement for transformation of lymphoid cells by Abelson murine leukemia virus

Abstract

The single protein encoded by Abelson murine leukemia virus is a fusion of sequence from the retroviral gag genes with the v-abl sequence. Deletion of most of the gag region from the transforming protein results in a virus capable of transforming fibroblasts but no longer capable of transforming lymphoid cells. Smaller deletions in gag reveal that p15 gag sequences are responsible for this effect, whereas deletion of p12 sequences had no effect on lymphoid transformation. In transformed fibroblasts, p15-deleted and normal proteins had similar activities and subcellular localization. When the p15-deleted genome was introduced into previously transformed lymphoid lines, its protein product exhibited a marked instability. The tyrosine-specific autophosphorylation activity per cell was less than 1/20th that of the nondeleted protein. Although pulse-Ia-beling showed that the p15-deleted protein was synthesized efficiently, immunoblotting demonstrated that its steady-state level was less than 1/10th that of the nondeleted Abelson protein. The specific instability of the p15-deleted protein in lymphoid cells explains the requirement of these sequences for lymphoid but not fibroblast transformation.

Additional Information

Copyright © 1985 by the American Society for Microbiology. Received 22 October 1984/Accepted 28 December 1984 This work was supported by Public Health Service grants CA26717 (to D.B.) and CA24220 (to N.R.) from the National Cancer Institute and grant MV171 from the American Cancer Society (to N.R.). N.R. is a recipient of a research career development award from the National Cancer Institute.

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August 22, 2023
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October 13, 2023