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      Transcription Termination Defective Mutants of Rho: Role of Different Functions of Rho in Releasing RNA from the Elongation Complex

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          Abstract

          The transcription termination factor Rho of Escherichia coli is a RNA binding protein which can translocate along the RNA and unwind the RNA:DNA hybrid using the RNA-dependent ATPase activity. In order to investigate the involvement of each of these functions in releasing RNA from the elongation complex, we have isolated different termination defective mutants of Rho by random mutagenesis, characterized them for their different functions and established the structure–function correlations from the available structural data of Rho. These mutations are located within the two domains; the N-terminal RNA binding domain (G51V, G53V, and Y80C) and in the C-terminal ATP binding domain (Y274D, P279S, P279L, G324D, N340S, I382N) including the two important structural elements, the Q-loop (P279S, P279L) and R-loop (G324D). Termination defects of the mutants in primary RNA binding domain and Q-loop could not be restored under any conditions that we tested and these were also defective for most of the other functions of Rho. The termination defects of the mutants (Y274D, G324D and N340S), which were mainly defective for secondary RNA binding and likely defective for translocase activity, could be restored under relaxed in vitro conditions. We also show that a mutation in a primary RNA binding domain (Y80C) can cause a defect in ATP binding and induce distinct conformational changes in the distal C-terminal domain, and these allosteric effects are not predictable from the crystal structure. We conclude that the interactions in the primary RNA binding domain and in the Q-loop are mandatory for RNA release to occur and propose that the interactions in the primary RNA binding modulate most of the other functions of Rho allosterically. The rate of ATP hydrolysis regulates the processivity of translocation along the RNA and is directly correlated with the efficiency of RNA release. NusG improves the speed of RNA release and is not involved in any other step.

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          Mapping and sequencing of mutations in the Escherichia coli rpoB gene that lead to rifampicin resistance.

          Ding Jun Jin, Carol A. Gross (1988)
          Rifampicin is an antibiotic that inhibits the function of RNA polymerase in eubacteria. Mutations affecting the beta subunit of RNA polymerase can confer resistance to rifampicin. A large number of rifampicin-resistant (hereafter called Rifr) mutants have been isolated in Escherichia coli to probe the involvement of RNA polymerase in a variety of physiological processes. We have undertaken a comprehensive analysis of Rifr mutations to identify their structural and functional effects on RNA polymerase. Forty-two Rifr isolates with a variety of phenotypes were mapped to defined intervals within the rpoB gene using a set of deletions of the rpoB gene. The mutations were sequenced. Seventeen mutational alterations affecting 14 amino acid residues were identified. These alleles are located in three distinct clusters in the center of the rpoB gene. We discuss the implications of our results with regards to the structure of the rifampicin binding site.
          Article 0 comments Cited 113 times – based on 0 reviews     Review now
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            Mechanism of intrinsic transcription termination and antitermination.

            John W. Yarnell, David Roberts (1999)
            Gene expression is modulated by regulatory elements that influence transcription elongation by RNA polymerase: terminators that disrupt the elongation complex and release RNA, and regulators that overcome termination signals. RNA release from Escherichia coli RNA polymerase can be induced by a complementary oligonucleotide that replaces the upstream half of the RNA hairpin stem of intrinsic terminator transcripts, implying that RNA hairpins act by extracting RNA from the transcription complex. A transcription antiterminator inhibits this activity of oligonucleotides and therefore protects the elongation complex from destabilizing attacks on the emerging transcript. These effects illuminate the structure of the complex and the mechanism of transcription termination.
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              Basic mechanisms of transcript elongation and its regulation.

              Jeremy Kane, William Chamberlin, Susan M Uptain (1996)
              Ternary complexes of DNA-dependent RNA polymerase with its DNA template and nascent transcript are central intermediates in transcription. In recent years, several unusual biochemical reactions have been discovered that affect the progression of RNA polymerase in ternary complexes through various transcription units. These reactions can be signaled intrinsically, by nucleic acid sequences and the RNA polymerase, or extrinsically, by protein or other regulatory factors. These factors can affect any of these processes, including promoter proximal and promoter distal pausing in both prokaryotes and eukaryotes, and therefore play a central role in regulation of gene expression. In eukaryotic systems, at least two of these factors appear to be related to cellular transformation and human cancers. New models for the structure of ternary complexes, and for the mechanism by which they move along DNA, provide plausible explanations for novel biochemical reactions that have been observed. These models predict that RNA polymerase moves along DNA without the constant possibility of dissociation and consequent termination. A further prediction of these models is that the polymerase can move in a discontinuous or inchworm-like manner. Many direct predictions of these models have been confirmed. However, one feature of RNA chain elongation not predicted by the model is that the DNA sequence can determine whether the enzyme moves discontinuously or monotonically. In at least two cases, the encounter between the RNA polymerase and a DNA block to elongation appears to specifically induce a discontinuous mode of synthesis. These findings provide important new insights into the RNA chain elongation process and offer the prospect of understanding many significant biological regulatory systems at the molecular level.
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                Author and article information

                Journal
                Journal ID (nlm-ta): J Mol Biol
                Title: Journal of Molecular Biology
                Publisher: Elsevier
                ISSN (Print): 0022-2836
                ISSN (Electronic): 1089-8638
                Publication date PMC-release: 24 August 2007
                Publication date (Print): 24 August 2007
                Volume: 371
                Issue: 4
                Pages: 855-872
                Affiliations
                Laboratory of Transcription Biology, Centre for DNA Fingerprinting and Diagnostics, ECIL Road, Nacharam, Hyderabad-500076, India
                Author notes
                [* ]Corresponding author. rsen@ 123456cdfd.org.in
                [†]

                S.B. and I.B. contributed equally to the work.

                Article
                Publisher ID: YJMBI59496
                DOI: 10.1016/j.jmb.2007.06.013
                PMC ID: 1950744
                PubMed ID: 17599352
                SO-VID: ce878c0f-996c-49cb-92c3-ec60913b58ad
                Copyright © © 2007 Elsevier Ltd.
                License:

                This document may be redistributed and reused, subject to certain conditions.

                History
                Date received : 4 April 2007
                Date revision received : 1 June 2007
                Date accepted : 1 June 2007
                Categories
                Subject: Article

                ScienceOpen disciplines: Molecular biology
                Keywords: transcription termination,%rt, read-through efficiency,ec, elongation complex,nusg,rho,mutagenesis,rnap, rna polymerase,rna polymerase
                Data availability:
                ScienceOpen disciplines: Molecular biology
                Keywords: transcription termination, %rt, read-through efficiency, ec, elongation complex, nusg, rho, mutagenesis, rnap, rna polymerase, rna polymerase

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