A continuous coupled spectrophotometric assay for tyrosine aminotransferase activity with aromatic and other nonpolar amino acids

被引：15

作者：

Luong, TN ^{[1
]}

Kirsch, JF ^{[1
]}

机构：

[1] UNIV CALIF BERKELEY,DEPT MOL & CELL BIOL,BERKELEY,CA 94720

来源：

ANALYTICAL BIOCHEMISTRY | 1997年 / 253卷 / 01期

关键词：

D O I：

10.1006/abio.1997.2344

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

A continuous assay for Escherichia coli tyrosine aminotransferase (TATase) that employs Lactobacillus delbrueckii ssp. bulgaricus hydroxyisocaproate dehydrogenase (HO-HxoDH) as a coupling enzyme is described. alpha-Keto acids, including those formed by TATase-catalyzed transamination of L-phenylalanine, L-tyrosine, L-tryptophan, L-methionine, and L-leucine, are converted to the corresponding alpha-hydroxy acids by the auxiliary enzyme. The concomitant reduction of NADH by this enzyme can be followed as a decrease in absorbance at 340 nm. Importantly, HO-HxoDH-catalyzed reduction of alpha-ketoglutarate (alpha-KG), a cosubstrate of TATase required to regenerate the pyridoxal-5'-phosphate cofactor of this enzyme from pyridoxamine-5'-phosphate, is a poor substrate and does not interfere with the assay, The kinetic parameters determined for the transamination of phenylalanine by TATase (k(cat) = 180 s(-1), KM (L-Phe) = 0.56 mM, KM (alpha-KG) = 5 mM) with HO-HxoDH as a coupling enzyme are comparable to those reported in the literature, which were determined by direct monitoring of the formation of phenylpyruvate at 280 nm, This new assay offers the advantages of increased sensitivity and broad substrate specificity. (C) 1997 Academic Press.

引用

页码：46 / 49

页数：4

共 16 条

[1] NAD+-DEPENDENT D-2-HYDROXYISOCAPROATE DEHYDROGENASE OF LACTOBACILLUS-DELBRUECKII SUBSP BULGARICUS - GENE CLONING AND ENZYME CHARACTERIZATION [J].

BERNARD, N ;

JOHNSEN, K ;

FERAIN, T ;

GARMYN, D ;

HOLS, P ;

HOLBROOK, JJ ;

DELCOUR, J .

EUROPEAN JOURNAL OF BIOCHEMISTRY, 1994, 224 (02) :439-446

[2]

BRAUNSHTEIN AE, 1953, BIOKHIMIYA, V18, P393

[3] CALCULATION OF PROTEIN EXTINCTION COEFFICIENTS FROM AMINO-ACID SEQUENCE DATA [J].

GILL, SC ;

VONHIPPEL, PH .

ANALYTICAL BIOCHEMISTRY, 1989, 182 (02) :319-326

[4] EXAMINING THE STRUCTURAL AND CHEMICAL FLEXIBILITY OF THE ACTIVE-SITE BASE, LYS-258, OF ESCHERICHIA-COLI ASPARTATE-AMINOTRANSFERASE BY REPLACEMENT WITH UNNATURAL AMINO-ACIDS [J].

GLOSS, LM ;

KIRSCH, JF .

BIOCHEMISTRY, 1995, 34 (38) :12323-12332

[5] ESCHERICHIA-COLI AROMATIC AMINO-ACID AMINOTRANSFERASE - CHARACTERIZATION AND COMPARISON WITH ASPARTATE-AMINOTRANSFERASE [J].

HAYASHI, H ;

INOUE, K ;

NAGATA, T ;

KURAMITSU, S ;

KAGAMIYAMA, H .

BIOCHEMISTRY, 1993, 32 (45) :12229-12239

[6] Analysis of the substrate-recognition mode of aromatic amino acid aminotransferase by combined use of quasisubstrates and site-directed mutagenesis: Systematic hydroxy-group addition/deletion studies to probe the enzyme-substrate interactions [J].

Hayashi, H ;

Inoue, K ;

Mizuguchi, H ;

Kagamiyama, H .

BIOCHEMISTRY, 1996, 35 (21) :6754-6761

[7] REVERSIBLE DISSOCIATION AND UNFOLDING OF ASPARTATE-AMINOTRANSFERASE FROM ESCHERICHIA-COLI - CHARACTERIZATION OF A MONOMERIC INTERMEDIATE [J].

HEROLD, M ;

KIRSCHNER, K .

BIOCHEMISTRY, 1990, 29 (07) :1907-1913

[8] BRANCHED-CHAIN AMINO-ACID AMINOTRANSFERASE OF ESCHERICHIA-COLI - OVERPRODUCTION AND PROPERTIES [J].

INOUE, K ;

KURAMITSU, S ;

AKI, K ;

WATANABE, Y ;

TAKAGI, T ;

NISHIGAI, M ;

IKAI, A ;

KAGAMIYAMA, H .

JOURNAL OF BIOCHEMISTRY, 1988, 104 (05) :777-784

[9] PROTONATION STATE OF THE ACTIVE-SITE SCHIFF-BASE OF AROMATIC AMINO-ACID AMINOTRANSFERASE - MODULATION BY BINDING OF LIGANDS AND IMPLICATIONS FOR ITS ROLE IN CATALYSIS [J].

IWASAKI, M ;

HAYASHI, H ;

KAGAMIYAMA, H .

JOURNAL OF BIOCHEMISTRY, 1994, 115 (01) :156-161

[10]

KOHLER E, 1994, BIOCHEMISTRY-US, V33, P90

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