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Labeled EF-Tus for Rapid Kinetic Studies of Pretranslocation Complex Formation
Author(s) -
Wei Liu,
Darius Kavaliauskas,
Jared M. Schrader,
Kiran Poruri,
Victoria Birkedal,
Emanuel Goldman,
Hieronim Jakubowski,
Włodek Mandecki,
Olke C. Uhlenbeck,
Charlotte R. Knudsen,
Yale E. Goldman,
Barry S. Cooperman
Publication year - 2014
Publication title -
acs chemical biology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.899
H-Index - 111
eISSN - 1554-8937
pISSN - 1554-8929
DOI - 10.1021/cb500409y
Subject(s) - ribosome , transfer rna , ternary complex , translation (biology) , biology , ribosomal rna , ef tu , protein biosynthesis , biochemistry , puromycin , elongation factor , aminoacyl trna , messenger rna , rna , enzyme , gene
The universally conserved translation elongation factor EF-Tu delivers aminoacyl(aa)-tRNA in the form of an aa-tRNA·EF-Tu·GTP ternary complex (TC) to the ribosome where it binds to the cognate mRNA codon within the ribosomal A-site, leading to formation of a pretranslocation (PRE) complex. Here we describe preparation of QSY9 and Cy5 derivatives of the variant E348C-EF-Tu that are functional in translation elongation. Together with fluorophore derivatives of aa-tRNA and of ribosomal protein L11, located within the GTPase associated center (GAC), these labeled EF-Tus allow development of two new FRET assays that permit the dynamics of distance changes between EF-Tu and both L11 (Tu-L11 assay) and aa-tRNA (Tu-tRNA assay) to be determined during the decoding process. We use these assays to examine: (i) the relative rates of EF-Tu movement away from the GAC and from aa-tRNA during decoding, (ii) the effects of the misreading-inducing antibiotics streptomycin and paromomycin on tRNA selection at the A-site, and (iii) how strengthening the binding of aa-tRNA to EF-Tu affects the rate of EF-Tu movement away from L11 on the ribosome. These FRET assays have the potential to be adapted for high throughput screening of ribosomal antibiotics.

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