Abstract

Translation of mRNA sequences by the ribosome is normally a faithful process, yet mistakes occur. Sequences in mRNAs have evolved that modulate the accuracy of translation to increase the frequency of translational frameshifting errors. Such sites are termed programmed translational frameshift sites. The yeast Ty elements, a class of retrotransposons, express the enzymes needed for retrotransposition using a programmed+1 frameshifting mechanism. We find evidence that frameshifting occurs because the mRNA disrupts the function of the ribosomal accuracy center by inserting peptidyl-tRNAs into the ribosomal P site that Make a non-canonical interaction with the mRNA. The unusual codon*anticodon complex formed disrupts the ability of the ribosome to accurately recognize in-frame cognate tRNAs in the A site. Also, a sequence derived from the Ty3 retrotransposon appears to directly interact with a structure in the rRNA necessary for accurate decoding in the A site. This sequence, termed the Ty3 stimulator, appears to base pair with part of the loop of Helix 18. A nucleotide in that base paired region, G530, directly contacts both mRNA and tRNA nucleotides in the A site codon*anticodon complex to assure that they are correctly paired. By sequestering that nucleotide in an rnRNA*rRNA complex, the Ty3 stimulator could reduce overall discrimination in the A site. Recently, detailed molecular structures of the 30S, 50S and 70S ribosomes were solved. These structures provide an unprecedented level of detail about the structure of the ribosome, and can be used to predict the mechanisms used during translation, including the error correction mechanisms. The structures clearly show how cognate, in-frame tRNAs are recognized, but gives little direct information about how the ribosome avoids errors leading to changes in translational frame. Arguably, maintenance of frame is the most critical role for the ribosome, since frame errors almost always result in production of inactive protein products while missense errors rarely do. To address how the ribosome maintains reading frame we have been using the tools provided by the programmed translational frameshift sites. We will continue that work attempting to determine how error-correcting elements of the ribosome function in this process. Recently, we found that mRNA sequences that stimulate frame errors also induce errors during translational initiation. This suggests that the accuracy of these processes has shared aspects. We will use the twin tools afforded by frameshifting and translation initiation to dissect the ribosomal functions insuring accuracy.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM029480-24
Application #
6868887
Study Section
Cell Development and Function Integrated Review Group (CDF)
Program Officer
Rhoades, Marcus M
Project Start
1989-08-01
Project End
2007-03-31
Budget Start
2005-04-01
Budget End
2007-03-31
Support Year
24
Fiscal Year
2005
Total Cost
$323,104
Indirect Cost

  Institution

Name
University of Maryland Balt CO Campus
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
061364808
City
Baltimore
State
MD
Country
United States
Zip Code
21250

  Publications

Manickam, Nandini; Joshi, Kartikeya; Bhatt, Monika J et al. (2016) Effects of tRNA modification on translational accuracy depend on intrinsic codon-anticodon strength. Nucleic Acids Res 44:1871-81
Nord, Stefan; Bhatt, Monika J; Tükenmez, Hasan et al. (2015) Mutations of ribosomal protein S5 suppress a defect in late-30S ribosomal subunit biogenesis caused by lack of the RbfA biogenesis factor. RNA 21:1454-68
Manickam, Nandini; Nag, Nabanita; Abbasi, Aleeza et al. (2014) Studies of translational misreading in vivo show that the ribosome very efficiently discriminates against most potential errors. RNA 20:9-15
Turkel, Sezai; Kaplan, Guliz; Farabaugh, Philip J (2011) Glucose signalling pathway controls the programmed ribosomal frameshift efficiency in retroviral-like element Ty3 in Saccharomyces cerevisiae. Yeast 28:799-808
Kramer, Emily B; Vallabhaneni, Haritha; Mayer, Lauren M et al. (2010) A comprehensive analysis of translational missense errors in the yeast Saccharomyces cerevisiae. RNA 16:1797-808
Vallabhaneni, Haritha; Fan-Minogue, Hua; Bedwell, David M et al. (2009) Connection between stop codon reassignment and frequent use of shifty stop frameshifting. RNA 15:889-97
Vallabhaneni, Haritha; Farabaugh, Philip J (2009) Accuracy modulating mutations of the ribosomal protein S4-S5 interface do not necessarily destabilize the rps4-rps5 protein-protein interaction. RNA 15:1100-9
Kramer, Emily B; Farabaugh, Philip J (2007) The frequency of translational misreading errors in E. coli is largely determined by tRNA competition. RNA 13:87-96
Guarraia, Carla; Norris, Laura; Raman, Ana et al. (2007) Saturation mutagenesis of a +1 programmed frameshift-inducing mRNA sequence derived from a yeast retrotransposon. RNA 13:1940-7
Taliaferro, Dwayne L; Farabaugh, Philip J (2007) Testing constraints on rRNA bases that make nonsequence-specific contacts with the codon-anticodon complex in the ribosomal A site. RNA 13:1279-86

Showing the most recent 10 out of 29 publications