Volume 41, Issue 3, Pages (February 2011)

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Volume 41, Issue 3, Pages 321-330 (February 2011) Nascent Peptide in the Ribosome Exit Tunnel Affects Functional Properties of the A-Site of the Peptidyl Transferase Center  Haripriya Ramu, Nora Vázquez-Laslop, Dorota Klepacki, Qing Dai, Joseph Piccirilli, Ronald Micura, Alexander S. Mankin  Molecular Cell  Volume 41, Issue 3, Pages 321-330 (February 2011) DOI: 10.1016/j.molcel.2010.12.031 Copyright © 2011 Elsevier Inc. Terms and Conditions

Molecular Cell 2011 41, 321-330DOI: (10.1016/j.molcel.2010.12.031) Copyright © 2011 Elsevier Inc. Terms and Conditions

Figure 1 Ribosome Stalling at ermAL1 (A) Schematic map of the regulatory region of the ermA gene. The amino acid sequences encoded in the regulatory ORFs ermAL1 and ermAL2 are shown. The sequence of the peptide encoded in the ermCL regulatory ORF is presented for comparison. (B) Primer extension inhibition analysis of the site of ribosome stalling at ermAL1. The ermAL1 ORF was translated in vitro (Shimizu et al., 2001) in the absence (-) or presence (+) of erythromycin (Ery). A primer was annealed to the 3′end of mRNA and extended with reverse transcriptase (Vazquez-Laslop et al., 2008; Vázquez-Laslop et al., 2010). The same primer was used to generate sequencing lanes (U, C). The sequence of the ermAL1 gene and the encoded amino acids are shown to the left of the gel. Reverse transcriptase stops are indicated by arrowheads. The codon located in the P-site of the stalled ribosome is boxed. (C) The effect of mutations of codons 2–10 of ermAL1 on ribosome stalling. The amino acid changes associated with the codon mutations are indicated in the cartoon and over the corresponding lanes of the gel. The primer extension bands representing the ribosome stalled at the eighth ermAL1 codon are shown by arrowheads next to the gel. The lanes representing mutations at codons located in the P- and A-sites of the stalled ribosomes are boxed. In the cartoon, the star represents erythromycin bound in the tunnel. Molecular Cell 2011 41, 321-330DOI: (10.1016/j.molcel.2010.12.031) Copyright © 2011 Elsevier Inc. Terms and Conditions

Figure 2 The Role of the A-Site Codon in SRC Formation (A) The A-site amino acid is not incorporated in the nascent peptide. The cartoon shows possible versions of peptidyl-tRNA in SRC containing the eighth codon of ermAL1 in the P-site. The A-site amino acid (Glu) is shown by a filled circle and the erythromycin molecule bound in the exit tunnel is represented by a star. The gel represents northern blot analysis of tRNA associated with the stalled ribosome. Positions of aminoacyl-tRNAs and peptidyl-tRNA are indicated. (B) Effects of mutations in the ninth codon of ermAL1 on ribosome stalling. The control (no erythromycin) lane is shown only for the wild-type ermAL1 sequence. The bar diagram represents the results of quantitation of the intensity of the stalled ribosome bands (an average of three independent experiments). Error bars represent the standard deviation of the mean. (C) Testing the effects of A-site codons decoded by different tRNA isoacceptors on ribosome stalling. Note that a single nucleotide shift in the position of the band observed with tRNAArg isoacceptors apparently reflects change in the ribosome geometry in response to binding of different tRNAs, which affects the precise site where reverse transcriptase stops. This effect was also seen when binding of different tRNAs was directed to the A-site (see gel in panel B). Molecular Cell 2011 41, 321-330DOI: (10.1016/j.molcel.2010.12.031) Copyright © 2011 Elsevier Inc. Terms and Conditions

Figure 3 Differential Acceptor Activity of Stalling and Nonstalling Amino Acids in the Reaction of Peptide Bond Formation in the SRC (A) The ribosome stalled at the end of the truncated ermAL1 mRNA was allowed to react for a specified time at 37°C with 1 mM CCA-N-Ala or CCA-N-Lys, and the remaining unreacted peptidyl-tRNA was resolved by gel electrophoresis. The first two lanes in the gel show samples incubated for 0 or 30 min in the absence of aminoacyl-tRNA analogs. The graph below the gel represents the results of quantitation of the amount of radioactivity in the peptidyl-tRNA bands. (B) Translation in the presence of erythromycin of an extended ermAL1 ORF containing a mutation of the wild-type ninth codon (Glu) to the nonstalling Phe. A frameshift mutation downstream of the stalling site extends the ORF to 72 codons. The codons located in the P- and A-sites of the SRC are boxed. The position of gel bands representing a 72-amino acid full-size translation product and peptidyl-tRNA esterified by an 8 amino acid nascent peptide are marked by filled and contoured arrowheads, respectively. Four-fold less material was loaded onto the no-erythromycin lanes compared with the erythromycin lanes. The bar diagram represents the results of quantitation of the amount of radioactivity in the gel bands in the samples containing erythromycin. Molecular Cell 2011 41, 321-330DOI: (10.1016/j.molcel.2010.12.031) Copyright © 2011 Elsevier Inc. Terms and Conditions

Figure 4 Effects of the Nascent Peptide Sequence on the Properties of the PTC A-Site The gels show the primer extension inhibition signal (bold arrowheads) representing SRC formation at different ORFs (erythromycin was present in all the samples). Bands corresponding to translation initiation sites at the erm ORFs are shown for reference and are indicated by thin arrows. The amino acid sequences corresponding to the ErmCL peptide are red and those representing the ErmAL1 peptide are blue. The Gly mutation at position 7 of ErmCL is shown in green, and the A-site amino acid is black. Amino acids located in the A-site of the PTC in the stalled ribosome are boxed with solid lines. The amino acid position −2 relative to the nascent peptide C terminus is boxed with a dashed line. Molecular Cell 2011 41, 321-330DOI: (10.1016/j.molcel.2010.12.031) Copyright © 2011 Elsevier Inc. Terms and Conditions

Figure 5 Nascent Peptide Controls Properties of the PTC A-Site (A) During normal translation, the PTC A-site (orange) is in the versatile state. (B) In the presence of an inducing antibiotic (ery) and a specific nascent peptide (e.g., ErmAL1), the A-site becomes selective. Peptide bond formation with certain amino acids (red) becomes very slow; the corresponding A-site codons are conducive to SRC formation. (C) Certain peptide sequences (e.g., ErmCL) can render the A-site even more restrictive; the SRC is formed irrespective of the A-site codon. The ErmAL1 and ErmCL sequences essential for stalling are shown in cyan; the amino acid residue in position −2, which apparently controls the A-site properties, is blue. (D) A possible signal relay pathway communicating the information from the ribosomal exit tunnel to the PTC A-site. The eight-amino acid ErmAL1 nascent peptide, attached to the P-site tRNA, was modeled in the structure of Thermus thermophilus 70S ribosome (PDB accession number 2WDL; Voorhees et al., 2009). C-terminal amino acids critical for stalling are colored in cyan; the residue at position −2 is shown in blue. The 23S rRNA residues A2451 and C2452 forming the A-site crevice are orange. Erythromycin shape (ery) is shown as violet sticks and mesh with the cladinose residue highlighted in red. Mutations of residues A2062 and A2503 (purple) prevent stalling. Neighboring residues G2061 and U2504 (pale blue) may participate in communicating the stalling signal to the A-site crevice. The conformational flexibility of the rRNA residues putatively involved in relaying the stalling signal from the exit tunnel to the PTC is illustrated by their varying placements in different ribosomal complexes (Schmeing et al., 2005; Gürel et al., 2009; Schuwirth et al., 2005; Jenner et al., 2005; Petry et al., 2005). Molecular Cell 2011 41, 321-330DOI: (10.1016/j.molcel.2010.12.031) Copyright © 2011 Elsevier Inc. Terms and Conditions