Conserved Nucleotides of 23 S rRNA Located at the Ribosomal Peptidyltransferase Center

Spahn, C.M.T.; Schäfer, Markus A.; Krayevsky, Alexander A.; Nierhaus, Knud H.

doi:10.1074/jbc.271.51.32857

Cited by 27 publications

(21 citation statements)

References 25 publications

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“…It is therefore likely that the effects of the helix 90 mutations on poly(Phe) synthesis are caused by a severe distortion of the active center of the ribosomal PTF (28). The data clearly indicate that not only the single-stranded 23 S rRNA regions in the central loop of domain V are of high importance for ribosomal function but also the nucleotides at the top of helix 90.…”

Section: Discussionmentioning

confidence: 53%

“…Poly(Phe) synthesis is severely impaired. In the following paper, we were able to demonstrate that the helix 90 mutations G2581A, C2507U/G2581A, and C2507⌬/G2581A completely block the puromycin reaction, and the mutation ⌿2580C drastically impairs this reaction (28). Also C2507U reduces the AcPhe-puromycin formation by approximately 50%.…”

Section: Discussionmentioning

confidence: 77%

“…For example, the G2661C mutation of 23 S rRNA has no effect on bacterial growth until expressed in a mutant S12 background (46), but the 23 S rRNA mutation alone significantly reduces the translational efficiency (47). As shown in the following paper (28), the mutations introduced in helix 80 only slightly reduce the puromycin reaction. Therefore, none of the changed bases is essential for peptide bond formation.…”

Section: Discussionmentioning

confidence: 92%

“…Therefore, a normal tRNA binding to the A and P sites and a block in the PTF activity would be important indications for the specificity of the provoked ribosomal defect. Various functional tests were performed in this and the accompanying study (28) that require a tRNA at a specific site but differ in their ionic conditions. Therefore, 70 S ribosomes were isolated from all mutants and analyzed for binding of AcPhetRNA under the various conditions.…”

Section: Construction Of Mutants In Vivo Effects and Distribution Ofmentioning

confidence: 99%

“…One of these UGG sequences is U2249 to G2251 at the helix-loop 80, and the other is ⌿2580 to G2582 at helix 90, adjacent to the PTF ring. The U (⌿) and the middle G were mutated in both sequences, and the effects on growth, expression, ribosomal assembly, and functions were studied in this and the accompanying paper (28).…”

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confidence: 99%

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Mutational Analysis of Two Highly Conserved UGG Sequences of 23 S rRNA from Escherichia coli

Spahn

Rèmme

Schäfer

et al. 1996

Journal of Biological Chemistry

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The 23 S-type rRNA contains two phylogenetically conserved UGG sequences, which have the potential to bind the universal CCA-3-ends of tRNAs at the ribosomal peptidyltransferase center by base pairing. The first two positions, UG, of these sequences at the helix-loop 80 (U2249G2250) and helix-loop 90 (⌿2580G2581) and some related nucleotides were tested by site-directed mutagenesis for their involvement in ribosomal function, i.e. peptidyltransferase. The plasmid-derived mutated 23 S rRNA comprised about 50% of the total 23 S rRNA. None of the single mutations caused an assembly defect, and all 50 S subunits carrying an altered 23 S rRNA could freely exchange with the pools of 70S ribosomes and polysomes. The mutations at the helix-loop 80 region hardly affected bacterial growth. However, mutations at the helix 90 caused severe growth effects and severely impaired the in vitro protein synthesis, showing that this 23 S rRNA region is of high importance for ribosomal function.The central enzymatic activity of ribosomes is the formation of peptide bonds. The corresponding peptidyltransferase (PTF) 1 center is located on the large ribosomal subunit (1, 2). Reconstitution analyses have identified the ribosomal proteins L2, L3, and L4, and the 23 S rRNA as PTF candidates in Escherichia coli ribosomes (3-5). A complex derived from the large subunit of Thermus aquaticus ribosomes consisting of 23 S rRNA and only 3-8 proteins had significant PTF activity (6, 7). This observation underscores the possible involvement of 23 S rRNA in this activity.An impressive wealth of data points to a distinct feature of the secondary structure map of 23 S rRNA, the so-called "peptidyltransferase ring" of domain V (8, 9) as a component at or near the PTF center. The PTF ring comprises about 40 nucleotides and represents a cluster of universally conserved nucleotides (10, 11). It is satisfying that a highly divergent array of methods correspondingly identifies the same region of 23 S rRNA, methods such as cross-linking studies with substrates of the PTF center (12-15), mutations of the 23 S rRNA gene conferring resistance against inhibitors of the PTF activity (for review, see Refs. 16 and 17), and protection studies (18 -20).Some studies aimed to identify nucleotides at the PTF center. The nucleotides G2252 and G2253, which are at the helixloop 80, were protected against kethoxal by the 3Ј-terminal CCA of P-site bound tRNA (19). Mutation of G2252 generated a dominant lethal phenotype (21). A double mutant having both Gs altered was lethal and showed a reduced activity of peptide bond formation by approximately 50% (22). A recent analysis presented evidence that G2252 is involved in canonical base pairing with C74 at the acceptor end of tRNA, thus obviously playing a role in the binding of the donor substrate at the P site region of the PTF center (23).Another study applied a random mutagenesis of the "Southern half" of the PTF ring (residues 2493-2606). With an elegant screening procedure, 21 mutations of 18 positions were found. Mutatio...

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Section: Discussionmentioning

confidence: 53%

Section: Discussionmentioning

confidence: 77%