RNASE-E ACTIVITY IS CONFERRED BY A SINGLE POLYPEPTIDE - OVEREXPRESSION, PURIFICATION, AND PROPERTIES OF THE AMS RNE HMP1 GENE-PRODUCT

被引：80

作者：

CORMACK, RS ^{[1
]}

GENEREAUX, JL ^{[1
]}

MACKIE, GA ^{[1
]}

机构：

[1] UNIV WESTERN ONTARIO,DEPT BIOCHEM,LONDON N6A 5C1,ONTARIO,CANADA

来源：

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA | 1993年 / 90卷 / 19期

关键词：

ENDORIBONUCLEASE; RNA PROCESSING;

D O I：

10.1073/pnas.90.19.9006

中图分类号：

O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];

学科分类号：

07 ; 0710 ; 09 ;

摘要：

Ribonuclease E, an enzyme that processes pre-5S rRNA from its precursor, is now believed to be the major endoribonuclease participating in mRNA turnover in Escherichia coli. The product of the ams/rne/hmp1 gene, which is required for RNase E activity, was overexpressed, purified to near homogeneity by electroelution from an SDS/polyacrylamide gel, and renatured. The purified polypeptide possesses nucleolytic activity in vitro with a specificity identical to that observed for crude RNase E preparations. In addition, both UV crosslinking and RNA-protein blotting unambiguously showed that the Ams/Rne/Hmp1 polypeptide has a high affinity for RNA. Our results demonstrate that RNase E activity is directly attributable to, and is an inherent property of, an RNA-binding protein, the ams/rne/hmp1 gene product.

引用

页码：9006 / 9010

页数：5

共 27 条

[1] THE AMS (ALTERED MESSENGER-RNA STABILITY) PROTEIN AND RIBONUCLEASE-E ARE ENCODED BY THE SAME STRUCTURAL GENE OF ESCHERICHIA-COLI [J].

BABITZKE, P ;

KUSHNER, SR .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1991, 88 (01) :1-5

[2] MECHANISMS OF MESSENGER-RNA DECAY IN BACTERIA - A PERSPECTIVE [J].

BELASCO, JG ;

HIGGINS, CF .

GENE, 1988, 72 (1-2) :15-23

[3] CONTROL OF RNASE-E-MEDIATED RNA DEGRADATION BY 5'-TERMINAL BASE-PAIRING IN ESCHERICHIA-COLI [J].

BOUVET, P ;

BELASCO, JG .

NATURE, 1992, 360 (6403) :488-491

[4] CLONING AND ANALYSIS OF THE ENTIRE ESCHERICHIA-COLI-AMS GENE - AMS IS IDENTICAL TO HMP1 AND ENCODES A 114 KDA PROTEIN THAT MIGRATES AS A 180 KDA PROTEIN [J].

CASAREGOLA, S ;

JACQ, A ;

LAOUDJ, D ;

MCGURK, G ;

MARGARSON, S ;

TEMPETE, M ;

NORRIS, V ;

HOLLAND, IB .

JOURNAL OF MOLECULAR BIOLOGY, 1992, 228 (01) :30-40

[5] SEQUENCING AND EXPRESSION OF THE RNE GENE OF ESCHERICHIA-COLI [J].

CHAUHAN, AK ;

MICZAK, A ;

TARASEVICIENE, L ;

APIRION, D .

NUCLEIC ACIDS RESEARCH, 1991, 19 (01) :125-129

[6]

CLAVERIEMARTIN F, 1991, J BIOL CHEM, V266, P2843

[7] CLONING OF THE ALTERED MESSENGER-RNA STABILITY (AMS) GENE OF ESCHERICHIA-COLI K-12 [J].

CLAVERIEMARTIN, F ;

DIAZTORRES, MR ;

YANCEY, SD ;

KUSHNER, SR .

JOURNAL OF BACTERIOLOGY, 1989, 171 (10) :5479-5486

[8] STRUCTURAL REQUIREMENTS FOR THE PROCESSING OF ESCHERICHIA-COLI 5-S RIBOSOMAL-RNA BY RNASE-E INVITRO [J].

CORMACK, RS ;

MACKIE, GA .

JOURNAL OF MOLECULAR BIOLOGY, 1992, 228 (04) :1078-1090

[9] RNASE PH - AN ESCHERICHIA-COLI PHOSPHATE-DEPENDENT NUCLEASE DISTINCT FROM POLYNUCLEOTIDE PHOSPHORYLASE [J].

DEUTSCHER, MP ;

MARSHALL, GT ;

CUDNY, H .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1988, 85 (13) :4710-4714

[10] EFFECTS OF THE MODIFICATION OF TRANSFER BUFFER COMPOSITION AND THE RENATURATION OF PROTEINS IN GELS ON THE RECOGNITION OF PROTEINS ON WESTERN BLOTS BY MONOCLONAL-ANTIBODIES [J].

DUNN, SD .

ANALYTICAL BIOCHEMISTRY, 1986, 157 (01) :144-153

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