ISOLATION AND CHARACTERIZATION OF A GENE CODING FOR A NOVEL ASPARTATE-AMINOTRANSFERASE FROM RHIZOBIUM-MELILOTI

被引：27

作者：

ALFANO, JR

KAHN, ML

机构：

[1] WASHINGTON STATE UNIV, INST BIOL CHEM, PULLMAN, WA 99164 USA

[2] WASHINGTON STATE UNIV, DEPT MICROBIOL, PULLMAN, WA 99164 USA

来源：

JOURNAL OF BACTERIOLOGY | 1993年 / 175卷 / 13期

关键词：

D O I：

10.1128/JB.175.13.4186-4196.1993

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

Aspartate aminotransferase (AAT) is an important enzyme in aspartate catabolism and biosynthesis and, by converting tricarboxylic acid cycle intermediates to amino acids, AAT is also significant in linking carbon metabolism with nitrogen metabolism. To examine the role of AAT in symbiotic nitrogen fixation further, plasmids encoding three different aminotransferases from Rhizobium meliloti 104A14 were isolated by complementation of an Escherichia coli auxotroph that lacks three aminotransferases. pJA10 contained a gene, aatB, that coded for a previously undescribed AAT, AatB. pJA30 encoded an aromatic aminotransferase, TatA, that had significant AAT activity, and pJA20 encoded a branched-chain aminotransferase designated BatA. Genes for the latter two enzymes, tatA and batA, were previously isolated from R. meliloti. aatB is distinct from but hybridizes to aatA, which codes for AatA, a protein required for symbiotic nitrogen fixation. The DNA sequence of aatB contained an open reading frame that could encode a protein 410 amino acids long and with a monomer molecular mass of 45,100 Da. The amino acid sequence of aatB is unusual, and AatB appears to be a member of a newly described class of AATs. AatB expressed in E. coli has a K(m) for aspartate of 5.3 mM and a K(m) for 2-oxoglutarate of 0.87 mM. Its pH optimum is between 8.0 and 8.5. Mutations were constructed in aatB and tatA and transferred to the genome of R. meliloti 104A14. Both mutants were prototrophs and were able to carry out symbiotic nitrogen fixation.

引用

页码：4186 / 4196

页数：11

共 68 条

[1] GLUTAMATE OXALOACETATE TRANSAMINASE IN PEA ROOT-NODULES - PARTICIPATION IN A MALATE/ASPARTATE SHUTTLE BETWEEN PLANT AND BACTEROID
APPELS, MA
HAAKER, H
[J]. PLANT PHYSIOLOGY, 1991, 95 (03) : 740 - 747
[2] ACQUISITION OF NEW METABOLIC CAPABILITIES - MULTICOPY SUPPRESSION BY CLONED TRANSAMINASE GENES IN ESCHERICHIA-COLI K-12
BERG, CM
WANG, MD
VARTAK, NB
LIU, L
[J]. GENE, 1988, 65 (02) : 195 - 202
[3] THE GENBANK GENETIC SEQUENCE DATA-BANK
BILOFSKY, HS
BURKS, C
FICKETT, JW
GOAD, WB
LEWITTER, FI
RINDONE, WP
SWINDELL, CD
TUNG, CS
[J]. NUCLEIC ACIDS RESEARCH, 1986, 14 (01) : 1 - 4
[4] THE ACTIVE-SITE OF SULFOLOBUS-SOLFATARICUS ASPARTATE-AMINOTRANSFERASE
BIROLO, L
ARNONE, MI
CUBELLIS, MV
ANDREOTTI, G
NITTI, G
MARINO, G
SANNIA, G
[J]. BIOCHIMICA ET BIOPHYSICA ACTA, 1991, 1080 (03) : 198 - 204
[5] DICARBOXYLIC-ACID TRANSPORT IN RHIZOBIUM-MELILOTI - ISOLATION OF MUTANTS AND CLONING OF DICARBOXYLIC-ACID TRANSPORT GENES
BOLTON, E
HIGGISSON, B
HARRINGTON, A
OGARA, F
[J]. ARCHIVES OF MICROBIOLOGY, 1986, 144 (02) : 142 - 146
[6] BRADFORD MM, 1976, ANAL BIOCHEM, V72, P248, DOI 10.1016/0003-2697(76)90527-3
[7] COOPER AJL, 1985, TRANSAMINASES, P533
[8] CLONING AND SEQUENCING OF THE GENE CODING FOR ASPARTATE-AMINOTRANSFERASE FROM THE THERMOACIDOPHILIC ARCHAEBACTERIUM SULFOLOBUS-SOLFATARICUS
CUBELLIS, MV
ROZZO, C
NITTI, G
ARNONE, MI
MARINO, G
SANNIA, G
[J]. EUROPEAN JOURNAL OF BIOCHEMISTRY, 1989, 186 (1-2): : 375 - 381
[9] DAY DA, 1991, PLANT PHYSIOL BIOCH, V29, P185
[10] THE USE OF TRANSPOSON TN5 MUTAGENESIS IN THE RAPID GENERATION OF CORRELATED PHYSICAL AND GENETIC MAPS OF DNA SEGMENTS CLONED INTO MULTICOPY PLASMIDS - A REVIEW
DEBRUIJN, FJ
LUPSKI, JR
[J]. GENE, 1984, 27 (02) : 131 - 149

← 1 2 3 4 5 6 7 →