Abstract
BackgroundRibosome profiling (ribo-seq) provides experimental data on the density of elongating or initiating ribosomes at the whole transcriptome level that can be potentially used for estimating absolute levels of translation initiation at individual Translation Initiation Sites (TISs). These absolute levels depend on the mutual organisation of TISs within individual mRNAs. For example, according to the leaky scanning model of translation initiation in eukaryotes, a strong TIS downstream of another strong TIS is unlikely to be productive, since only a few scanning ribosomes would be able to reach the downstream TIS. In order to understand the dependence of translation initiation efficiency on the surrounding nucleotide context, it is important to estimate the strength of TISs independently of their mutual organisation, i.e. to estimate with what probability a ribosome would initiate at a particular TIS.ResultsWe designed a simple computational approach for estimating the probabilities of ribosomes initiating at individual start codons using ribosome profiling data. The method is based on the widely accepted leaky scanning model of translation initiation in eukaryotes which postulates that scanning ribosomes may skip a start codon if the initiation context is unfavourable and continue on scanning. We tested our approach on three independent ribo-seq datasets obtained in mammalian cultured cells.ConclusionsOur results suggested that the method successfully discriminates between weak and strong TISs and that the majority of numerous non-AUG TISs reported recently are very weak. Therefore the high frequency of non-AUG TISs observed in ribosome profiling experiments is due to their proximity to mRNA 5′-ends rather than their strength. Detectable translation initiation at non-AUG codons downstream of AUG codons is comparatively infrequent. The leaky scanning method will be useful for the characterization of differences in start codon selection between tissues, developmental stages and in response to stress conditions.Electronic supplementary materialThe online version of this article (doi:10.1186/s12859-014-0380-4) contains supplementary material, which is available to authorized users.
Highlights
Ribosome profiling provides experimental data on the density of elongating or initiating ribosomes at the whole transcriptome level that can be potentially used for estimating absolute levels of translation initiation at individual Translation Initiation Sites (TISs)
How to measure the strength of a translation initiation site (TIS)? One way to estimate the strength of a TIS is by counting the ribosomes that initiate at this particular codon
This is the basis of the signal generated in the ribo-seq studies described in the Background section [3,4,5]: the number of RNA fragments protected by the ribosomes arrested at a TIS should reflect the number of ribosomes initiating at this site
Summary
Ribosome profiling (ribo-seq) provides experimental data on the density of elongating or initiating ribosomes at the whole transcriptome level that can be potentially used for estimating absolute levels of translation initiation at individual Translation Initiation Sites (TISs). Despite differences in the experimental approaches and computational techniques, the studies converged in the conclusion that approximately half of the TISs are non-AUGs (Figure 1A “All TISs”). This was unanticipated as the translation initiation machinery was thought to stringently select AUG codons for initiation, whereas non-AUG TISs were thought to be rare and gene-specific. Earlier measurements of translation initiation in mammalian cell free extracts indicated that, even in optimal nucleotide context, non-AUG initiation efficiency is at least 20 times lower than that of AUG [10] and even lower in yeast [11]
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