Methionyl-tRNA synthetase from E coli - A review

T. Meinnel; Y. Mechulam; F. Dardel; J. M. Schmitter; C. Hountondji; S. Brunie; P. Dessen; G. Fayat; S. Blanquet

doi:10.1016/0300-9084(90)90126-2

Methionyl-tRNA synthetase from E coli - A review

T. Meinnel
, Y. Mechulam
, F. Dardel
, J. M. Schmitter
, C. Hountondji
, S. Brunie
, P. Dessen
, G. Fayat
, S. Blanquet

Institut Polytechnique de Paris

Résultats de recherche: Contribution à un journal › Article › Revue par des pairs

Résumé

Methionyl-tRNA synthetase (MetRS) from E coli is a dimer composed of 2 identical subunits of M_r 76 kDa. A fully active monomeric fragment (64 kDa) could be obtained by mild proteolysis of the native dimer. Earlier studies reviewed in Blanquet et al (1979) have compared the catalytic mechanisms of native and trypsin-modified MetRS. Moreover, the truncated form of the enzyme was crystallized and its 3-D structure solved at low resolution. In the last few years, the availability of the corresponding metG gene has facilitated the development of studies using affinity labelling and site-directed mutagenesis techniques. In parallel, the 3-D structure has been solved at a resolution of 2.5 Å. These convergent approaches have allowed significant progress in the understanding of the structure-function relationships of this enzyme, and, in particular, of the rules governing the recognition of tRNA.

langue originale	Anglais
Pages (de - à)	625-632
Nombre de pages	8
journal	Biochimie
Volume	72
Numéro de publication	8
Les DOIs	https://doi.org/10.1016/0300-9084(90)90126-2
état	Publié - 1 janv. 1990

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10.1016/0300-9084(90)90126-2

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title = "Methionyl-tRNA synthetase from E coli - A review",

abstract = "Methionyl-tRNA synthetase (MetRS) from E coli is a dimer composed of 2 identical subunits of Mr 76 kDa. A fully active monomeric fragment (64 kDa) could be obtained by mild proteolysis of the native dimer. Earlier studies reviewed in Blanquet et al (1979) have compared the catalytic mechanisms of native and trypsin-modified MetRS. Moreover, the truncated form of the enzyme was crystallized and its 3-D structure solved at low resolution. In the last few years, the availability of the corresponding metG gene has facilitated the development of studies using affinity labelling and site-directed mutagenesis techniques. In parallel, the 3-D structure has been solved at a resolution of 2.5 {\AA}. These convergent approaches have allowed significant progress in the understanding of the structure-function relationships of this enzyme, and, in particular, of the rules governing the recognition of tRNA.",

keywords = "3-D structure, affinity labelling, methionyl, neutron scattering, tRNA discrimination, tRNA synthetase",

author = "T. Meinnel and Y. Mechulam and F. Dardel and Schmitter, \{J. M.\} and C. Hountondji and S. Brunie and P. Dessen and G. Fayat and S. Blanquet",

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doi = "10.1016/0300-9084(90)90126-2",

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T1 - Methionyl-tRNA synthetase from E coli - A review

AU - Meinnel, T.

AU - Mechulam, Y.

AU - Dardel, F.

AU - Schmitter, J. M.

AU - Hountondji, C.

AU - Brunie, S.

AU - Dessen, P.

AU - Fayat, G.

AU - Blanquet, S.

PY - 1990/1/1

Y1 - 1990/1/1

N2 - Methionyl-tRNA synthetase (MetRS) from E coli is a dimer composed of 2 identical subunits of Mr 76 kDa. A fully active monomeric fragment (64 kDa) could be obtained by mild proteolysis of the native dimer. Earlier studies reviewed in Blanquet et al (1979) have compared the catalytic mechanisms of native and trypsin-modified MetRS. Moreover, the truncated form of the enzyme was crystallized and its 3-D structure solved at low resolution. In the last few years, the availability of the corresponding metG gene has facilitated the development of studies using affinity labelling and site-directed mutagenesis techniques. In parallel, the 3-D structure has been solved at a resolution of 2.5 Å. These convergent approaches have allowed significant progress in the understanding of the structure-function relationships of this enzyme, and, in particular, of the rules governing the recognition of tRNA.

AB - Methionyl-tRNA synthetase (MetRS) from E coli is a dimer composed of 2 identical subunits of Mr 76 kDa. A fully active monomeric fragment (64 kDa) could be obtained by mild proteolysis of the native dimer. Earlier studies reviewed in Blanquet et al (1979) have compared the catalytic mechanisms of native and trypsin-modified MetRS. Moreover, the truncated form of the enzyme was crystallized and its 3-D structure solved at low resolution. In the last few years, the availability of the corresponding metG gene has facilitated the development of studies using affinity labelling and site-directed mutagenesis techniques. In parallel, the 3-D structure has been solved at a resolution of 2.5 Å. These convergent approaches have allowed significant progress in the understanding of the structure-function relationships of this enzyme, and, in particular, of the rules governing the recognition of tRNA.

KW - 3-D structure

KW - affinity labelling

KW - methionyl

KW - neutron scattering

KW - tRNA discrimination

KW - tRNA synthetase

UR - https://www.scopus.com/pages/publications/0025119614

U2 - 10.1016/0300-9084(90)90126-2

DO - 10.1016/0300-9084(90)90126-2

M3 - Article

C2 - 2126467

AN - SCOPUS:0025119614

SN - 0300-9084

VL - 72

SP - 625

EP - 632

JO - Biochimie

JF - Biochimie

IS - 8

ER -

Methionyl-tRNA synthetase from E coli - A review

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