Analysis of the puromycin reaction
- 1 December 1986
- journal article
- Published by Wiley in European Journal of Biochemistry
- Vol. 161 (3) , 715-721
- https://doi.org/10.1111/j.1432-1033.1986.tb10498.x
Abstract
The standard technique for determination of the ribosomal site location of bound tRNA, viz. the puromycin reaction, has been analyzed with regard to its applicability under tRNA saturation conditions. The criteria derived have been used to re-examine the exclusion principle for peptidyl-tRNA binding, which states that only one peptidyl-tRNA (AcPhe-tRNA) can be bound per ribosome although in principle two sites (A and P site) are available. The following results were obtained. The puromycin reaction is only appropriate for a site determination if the reaction conditions prevent one ribosome from performing more than one puromycin reaction. With an excess of AcPhe-tRNA over ribosomes, and in the absence of EF-G, this criterion is fulfilled at 0 degree C, where the P-site-bound material reacts with puromycin (quantitative reaction after 50 h), while the A-site-bound material does not. In contrast, at 37 degrees C the extent of the puromycin reaction can exceed the binding values by 2-4-fold ('repetitive reaction'). In the presence of EF-G a repetitive puromycin reaction is seen even at 0 degree C, i.e. EF-G can already promote a translocation reaction at 0 degree C. However, the extent of translocation becomes negligibly low for short incubation times (up to 60 min) at 0 degree C, if only catalytic amounts of EF-G are used. Using the criteria outlined above, the validity of the exclusion principle for Escherichia coli ribosomes was confirmed pursuing two different experimental strategies. Ribosomes were saturated with AcPhe-tRNA at one molecule per 70S ribosome, and a quantitative puromycin reaction demonstrated the exclusive P-site location of the AcPhe-tRNA. The same result was also found in the presence of viomycin, which blocks the translocation reaction. These findings also indicate that here nearly 100% of the ribosomes participate in AcPhe-tRNA binding to the P site. Precharging the P sites of 70S ribosomes with one Ac[14C]Phe-tRNA molecule per ribosome prevented additional Ac[3H]Phe-tRNA binding. In contrast, 70S particles carrying one molecule of [14C]tRNAPhe per ribosome were able to bind up to a further 0.64 molecule Ac[3H]Phe-tRNA per ribosome.Keywords
This publication has 11 references indexed in Scilit:
- Evidence that the three-site model for the ribosomal elongation cycle is also valid in the archaebacterium Halobacterium halobiumMolecular Genetics and Genomics, 1986
- Different conformations of tRNA in the ribosomal P‐site and A‐siteEuropean Journal of Biochemistry, 1985
- tRNA binding sites of ribosomes from Escherichia coliBiochemistry, 1984
- Spontaneous, elongation factor G independent translocation of Escherichia coli ribosomes.Journal of Biological Chemistry, 1983
- The Ribosomal Elongation Cycle: tRNA Binding, Translocation and tRNA ReleaseEuropean Journal of Biochemistry, 1983
- Non‐exclusion principle of Ac‐Phe‐tRNAPhe interaction with the donor and acceptor sites of Escherichia coli ribosomesFEBS Letters, 1982
- Three tRNA binding sites on Escherichia coli ribosomes.Proceedings of the National Academy of Sciences, 1981
- [54] Isolation of the protein synthesis elongation factors EF-Tu, EF-Ts, and EF-G from Escherichia coliPublished by Elsevier ,1979
- The Inhibition of Ribosomal Translocation by ViomycinEuropean Journal of Biochemistry, 1977
- Dual actions of viomycin on the ribosomal functionsBiochemical and Biophysical Research Communications, 1976