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Nucleic Acids Research, 1978, Vol. 5, No. 10 3715-3730
© 1978


Articles

The turnover of tRNAs microinjected into animal cells

Robert A. Schlegel1, Patrick Iversen and Martin Rechsteiner2

Department of Biology, University of Utah, Salt Lake City UT 84112, USA

2The author to whom correspondence should be sent.

Received August 11, 1978.

Red cell-mediated microinjection has been used to study tRNA turnover in SV3T3 mouse cells and TC7 cells, an African green monkey kidney line. The turnover of endogenous tRNA, measured by labeling with 3H-methionine, was first-order with half-lives of approximately one day in SV3T3 and two days in TC7 cells. 32p-tRNA isolated from E. coil or TC7 cells turned over at the same rate as endogenous tRNA when injected into either SV3T3 or TC7 cells. This demonstrates that cellular processes, not properties inherent to tRNAs, are responsible for the difference in tRNA turnover observed between SV3T3 and TC7 cells. These results further indicate that the mechanism of tRNA turnover in mammalian cells does not distinguish prokaryotic from eukaryotic tRNAs. In contrast to unmodified tRNA, glyoxalated tRNA was rapidly degraded upon injection. Thus altered tRNAs, like altered proteins, are turned over more rapidly in animal cells.


1Present address: Department of Microbiology and Cell Biology, The Pennsylvania State University, University Park, Pa. 16802.


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