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Literature DB >> 1309522

Broad-specificity endoribonucleases and mRNA degradation in Escherichia coli.

S K Srivastava¹, V J Cannistraro, D Kennell.

Abstract

Crude extracts from Escherichia coli were screened for any broad-specificity endoribonuclease after the cell proteins were fractionated by size. In a mutant lacking the gene for RNase I (molecular mass, 27,156 Da), the only such activities were also in the size range of 23 to 28 kDa. Fractionation by chromatography on a strong cation-exchange resin revealed only two activities. One of them eluted at a salt concentration expected for RNase M and had the specificity of RNase M. It preferred pyrimidine-adenosine bonds, could not degrade purine homopolymers, and had a molecular mass of approximately 27 kDa (V. J. Cannistraro and D. Kennell, Eur. J. Biochem. 181:363-370, 1989). A second fraction, eluting at a higher salt concentration, was active against any phosphodiester bond but was about 100 times less active than are RNase I and RNase I* (a form of RNase I) in the wild-type cell. On the basis of sizing-gel chromatography, this enzyme had a molecular mass of approximately 24 kDa. We call it RNase R (for residual). RNase R is not an abnormal product of the mutant rna gene; a cell carrying many copies of that gene on a plasmid did not synthesize more RNase R. Our search for broad-specificity endoribonucleases was prompted by the expectation that the primary activities for mRNA degradation are expressed by a relatively small number of broad-specificity RNases. If correct, the results suggest that the endoribonucleases for this major metabolic activity reside in the 24- to 28-kDa size range. Endoribonucleases with much greater specificity must have as primary functions the processing of specific RNA molecules at a very limited number of sites as steps in their biosynthesis. In exceptional cases, these endoribonucleases inactivate a specific message that has such a site, and they can also effect total mRNA metabolism indirectly by a global disturbance of the cell physiology. It is suggested that a distinction be made between these processing and degradative activities.

Entities: Chemical Species

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Year: 1992 PMID： 1309522 PMCID： PMC205676 DOI： 10.1128/jb.174.1.56-62.1992

Source DB: PubMed Journal: J Bacteriol ISSN： 0021-9193 Impact factor: 3.490

47 in total

1. Phage fl mRNA processing in Escherichia coli: search for the upstream products of endonuclease cleavage, requirement for the product of the altered mRNA stability (ams) locus.

Authors: R J Kokoska; K J Blumer; D A Steege
Journal: Biochimie Date: 1990-11 Impact factor: 4.079

2. Specific endonucleolytic cleavage of the mRNA for ribosomal protein S20 of Escherichia coli requires the product of the ams gene in vivo and in vitro.

Authors: G A Mackie
Journal: J Bacteriol Date: 1991-04 Impact factor: 3.490

3. RNase I*, a form of RNase I, and mRNA degradation in Escherichia coli.

Authors: V J Cannistraro; D Kennell
Journal: J Bacteriol Date: 1991-08 Impact factor: 3.490

4. Processing enzyme ribonuclease E specifically cleaves RNA I. An inhibitor of primer formation in plasmid DNA synthesis.

Authors: T Tomcsányi; D Apirion
Journal: J Mol Biol Date: 1985-10-20 Impact factor: 5.469

5. Polynucleotide phosphorylase and ribonuclease II are required for cell viability and mRNA turnover in Escherichia coli K-12.

Authors: W P Donovan; S R Kushner
Journal: Proc Natl Acad Sci U S A Date: 1986-01 Impact factor: 11.205

6. Decay of RNA in RNA processing mutants of Escherichia coli.

Authors: D Apirion; D R Gitelman
Journal: Mol Gen Genet Date: 1980-01

7. Purification and characterization of Escherichia coli RNase I. Comparisons with RNase M.

Authors: J Meador; B Cannon; V J Cannistraro; D Kennell
Journal: Eur J Biochem Date: 1990-02-14

8. Cloning and sequencing the gene encoding Escherichia coli ribonuclease I: exact physical mapping using the genome library.

Authors: J Meador; D Kennell
Journal: Gene Date: 1990-10-30 Impact factor: 3.688

9. Isolating and sequencing the predominant 5'-ends of a specific mRNA in cells. II. End-labeling and sequencing.

Authors: V J Cannistraro; B M Wice; D E Kennell
Journal: J Biochem Biophys Methods Date: 1985-08

10. Cleavages in the 5' region of the ompA and bla mRNA control stability: studies with an E. coli mutant altering mRNA stability and a novel endoribonuclease.

Authors: U Lundberg; A von Gabain; O Melefors
Journal: EMBO J Date: 1990-09 Impact factor: 11.598

10 in total

10. Roles of RNase E, RNase II and PNPase in the degradation of the rpsO transcripts of Escherichia coli: stabilizing function of RNase II and evidence for efficient degradation in an ams pnp rnb mutant.

Authors: E Hajnsdorf; O Steier; L Coscoy; L Teysset; P Régnier
Journal: EMBO J Date: 1994-07-15 Impact factor: 11.598

10 in total

Broad-specificity endoribonucleases and mRNA degradation in Escherichia coli.

1. Phage fl mRNA processing in Escherichia coli: search for the upstream products of endonuclease cleavage, requirement for the product of the altered mRNA stability (ams) locus.

2. Specific endonucleolytic cleavage of the mRNA for ribosomal protein S20 of Escherichia coli requires the product of the ams gene in vivo and in vitro.

3. RNase I*, a form of RNase I, and mRNA degradation in Escherichia coli.

4. Processing enzyme ribonuclease E specifically cleaves RNA I. An inhibitor of primer formation in plasmid DNA synthesis.

5. Polynucleotide phosphorylase and ribonuclease II are required for cell viability and mRNA turnover in Escherichia coli K-12.

6. Decay of RNA in RNA processing mutants of Escherichia coli.

7. Purification and characterization of Escherichia coli RNase I. Comparisons with RNase M.

8. Cloning and sequencing the gene encoding Escherichia coli ribonuclease I: exact physical mapping using the genome library.

9. Isolating and sequencing the predominant 5'-ends of a specific mRNA in cells. II. End-labeling and sequencing.

10. Cleavages in the 5' region of the ompA and bla mRNA control stability: studies with an E. coli mutant altering mRNA stability and a novel endoribonuclease.

Review 1. Processing endoribonucleases and mRNA degradation in bacteria.

2. Decay of ermC mRNA in a polynucleotide phosphorylase mutant of Bacillus subtilis.

3. RNase YI* and RNA structure studies.

Review 4. Trans-acting regulators of ribonuclease activity.

5. Purification and characterization of the bacteriophage P4 delta protein.

6. Cell-Free Protein Synthesis by Diversifying Bacterial Transcription Machinery.

7. Escherichia coli endoribonucleases involved in cleavage of bacteriophage T4 mRNAs.

8. Differential decay of RNA of the CFA/I fimbrial operon and control of relative gene expression.

Review 9. Bacterial ribonucleases and their roles in RNA metabolism.

10. Roles of RNase E, RNase II and PNPase in the degradation of the rpsO transcripts of Escherichia coli: stabilizing function of RNase II and evidence for efficient degradation in an ams pnp rnb mutant.