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NUCLEOLYTIC INACTIVATION AND DEGRADATION OF THE RNASE-III PROCESSED PNP MESSAGE ENCODING POLYNUCLEOTIDE PHOSPHORYLASE OF ESCHERICHIA-COLI

被引:44
作者
HAJNSDORF, E
CARPOUSIS, AJ
REGNIER, P
机构
[1] INST BIOL PHYSICOCHIM,CNRS,URA 1139,F-75005 PARIS,FRANCE
[2] UNIV GENEVA,DEPT MOLEC BIOL,CH-1211 GENEVA 4,SWITZERLAND
来源
JOURNAL OF MOLECULAR BIOLOGY | 1994年 / 239卷 / 04期
关键词
MESSENGER-RNA PROCESSING; MESSENGER-RNA DEGRADATION; RNASE III; RNASE E; POLYNUCLEOTIDE PHOSPHORYLASE;
D O I
10.1006/jmbi.1994.1387
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The two cleavages made by RNase III in the transcripts of the pnp gene of Escherichia coli, 80 nucleotides upstream of the coding sequence of polynucleotide phosphorylase, were previously demonstrated to trigger the rapid degradation of the pnp messenger. In this paper, we demonstrate that the 5' end of the RNase III processed pnp mRNA is attacked by ribonucleases more efficiently than the rest of the molecule. Several 5' extremities resulting from cleavages occurring in the first 500 nucleotides of the pnp transcript have been identified. Three of them referred to as X, Y and W occur in the wild-type strain at the beginning of the coding sequence of the pnp mRNA. The mRNA appears to be cleaved more efficiently at the X site, proximal to the initiation codon, than at sites Y and W located downstream. In vitro, the maturation at X is catalysed by RNase E but not by RNase III. Accumulation of RNA processed at X in RNase E deficient strains leads us to postulate that X is a high affinity primary site which is slowly cleaved by the residual activity of thermosensitive RNase E at non-permissive temperature and that secondary sites located downstream are processed less efficiently than X. Taken together, our results suggest that in wild-type E. coli the degradation of the RNase III processed mRNA is mediated by RNase E. © 1994, Academic Press Limited.
引用
收藏
页码:439 / 454
页数:16
相关论文
共 74 条
[41]   SITE-SPECIFIC ENDONUCLEOLYTIC CLEAVAGES AND THE REGULATION OF STABILITY OF ESCHERICHIA-COLI OMPA MESSENGER-RNA [J].
MELEFORS, O ;
VONGABAIN, A .
CELL, 1988, 52 (06) :893-901
[42]   GENETIC-STUDIES OF CLEAVAGE-INITIATED MESSENGER-RNA DECAY AND PROCESSING OF RIBOSOMAL 9S RNA SHOW THAT THE ESCHERICHIA-COLI-AMS AND RNE LOCI ARE THE SAME [J].
MELEFORS, O ;
VONGABAIN, A .
MOLECULAR MICROBIOLOGY, 1991, 5 (04) :857-864
[43]  
MELEFORS O, 1993, CONTROL MRNA STABILI
[44]   PROCESSING OF UNSTABLE BACTERIOPHAGE-T4 GENE-32 MESSENGER-RNAS INTO A STABLE SPECIES REQUIRES ESCHERICHIA-COLI RIBONUCLEASE-E [J].
MUDD, EA ;
PRENTKI, P ;
BELIN, D ;
KRISCH, HM .
EMBO JOURNAL, 1988, 7 (11) :3601-3607
[45]   ESCHERICHIA-COLI RNASE-E HAS A ROLE IN THE DECAY OF BACTERIOPHAGE-T4 MESSENGER-RNA [J].
MUDD, EA ;
CARPOUSIS, AJ ;
KRISCH, HM .
GENES & DEVELOPMENT, 1990, 4 (05) :873-881
[46]   RNASE-E, AN ENDORIBONUCLEASE, HAS A GENERAL ROLE IN THE CHEMICAL DECAY OF ESCHERICHIA-COLI MESSENGER-RNA - EVIDENCE THAT RNE AND AMS ARE THE SAME GENETIC-LOCUS [J].
MUDD, EA ;
KRISCH, HM ;
HIGGINS, CF .
MOLECULAR MICROBIOLOGY, 1990, 4 (12) :2127-2135
[47]   ESCHERICHIA-COLI ENDORIBONUCLEASE RNASE E - AUTOREGULATION OF EXPRESSION AND SITE-SPECIFIC CLEAVAGE OF MESSENGER-RNA [J].
MUDD, EA ;
HIGGINS, CF .
MOLECULAR MICROBIOLOGY, 1993, 9 (03) :557-568
[48]   EVIDENCE THAT RIFAMPICIN CAN STIMULATE READTHROUGH OF TRANSCRIPTIONAL TERMINATORS IN ESCHERICHIA-COLI, INCLUDING THE ATTENUATOR OF THE RPOBC OPERON [J].
NEWMAN, AJ ;
MA, JC ;
HOWE, KM ;
GARNER, I ;
HAYWARD, RS .
NUCLEIC ACIDS RESEARCH, 1982, 10 (22) :7409-7424
[49]   GROWTH-RATE DEPENDENT REGULATION OF MESSENGER-RNA STABILITY IN ESCHERICHIA-COLI [J].
NILSSON, G ;
BELASCO, JG ;
COHEN, SN ;
VONGABAIN, A .
NATURE, 1984, 312 (5989) :75-77
[50]   CONDITIONAL LETHAL MUTATION IN AN ESCHERICHIA-COLI STRAIN WITH A LONGER CHEMICAL LIFETIME OF MESSENGER-RNA [J].
ONO, M ;
KUWANO, M .
JOURNAL OF MOLECULAR BIOLOGY, 1979, 129 (03) :343-357
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