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Genome-wide analysis in vivo of translation with nucleotide resolution using ribosome profiling.

Science (New York, N.Y.), Vol. 324, No. 5924. (10 April 2009), pp. 218-223.

X Abstract

Techniques for systematically monitoring protein translation have lagged far behind methods for measuring messenger RNA (mRNA) levels. Here, we present a ribosome-profiling strategy that is based on the deep sequencing of ribosome-protected mRNA fragments and enables genome-wide investigation of translation with subcodon resolution. We used this technique to monitor translation in budding yeast under both rich and starvation conditions. These studies defined the protein sequences being translated and found extensive translational control in both determining absolute protein abundance and responding to environmental stress. We also observed distinct phases during translation that involve a large decrease in ribosome density going from early to late peptide elongation as well as widespread regulated initiation at non-adenine-uracil-guanine (AUG) codons. Ribosome profiling is readily adaptable to other organisms, making high-precision investigation of protein translation experimentally accessible.

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This article has been bookmarked 23 times, initially on 2009-02-13.

2010-01-31 User chrisvanlang
2009-11-13 User hzoltan
2009-11-04 User jwfoley
2009-10-13 User yyfwuhan
2009-08-07 User gbloeb , 1 note

A novel approach to "proteomics." By mapping ribosome binding to transcripts in yeast using an "RNAse hypersensitivity" approach, were able to produce a much better prediction of protein levels in cells than by mRNA alone R^2=.6 v. R^2=.17 for mRNA. More to the point for miRNA studies, this technique gives a snapshot of translation occurring in cells, the main step thought to be regulated by miRNA.

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