INTRINSIC TRYPTOPHAN FLUORESCENCE OF BOVINE LIVER ADENOSINE KINASE, CHARACTERIZATION OF LIGAND-BINDING SITES AND CONFORMATIONAL-CHANGES

被引：20

作者：

ELALAOUI, A

DIVITA, G

MAURY, G

IMBACH, JL

GOODY, RS

机构：

[1] MAX PLANCK INST MED RES,BIOPHYS ABT,D-69120 HEIDELBERG,GERMANY

[2] UNIV MONTPELLIER 2,CNRS,URA 488,MONTPELLIER,FRANCE

来源：

EUROPEAN JOURNAL OF BIOCHEMISTRY | 1994年 / 221卷 / 02期

关键词：

D O I：

10.1111/j.1432-1033.1994.tb18798.x

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：

Bovine liver adenosine kinase is a 45-KDa monomeric protein which exhibits a characteristic intrinsic tryptophan fluorescence with a maximal excitation at 284 nm and an emission peak centered at 335 nm. A total of three tryptophan residues/molecule has been estimated by using a fluorescence titration method. Low values of Stern-Volmer quenching constants in the presence of either acrylamide or iodide (4.2 M(-1) or 1.5 M(-1), respectively) indicated that the tryptophan residues are relatively buried in the native molecule. Tryptophan residues also showed a high heterogeneity, with a fractional accessible fluorescence value for iodide of 0.65. The enzyme fluorescence was very sensitive to substrate binding, which induced a marked fluorescence quenching, a lower tryptophan accessibility to acrylamide and iodide, and an increase in the tryptophan heterogeneity. ADP or ATP showed a monophasic saturation curve consistent with the existence of one binding site. In contrast, adenosine and AMP gave biphasic saturation curves, suggesting the existence of at least two binding sites, with a high and a low affinity. The presence of MgCl2 increased the affinity of ATP or ADP, whereas the binding of adenosine or AMP was not affected.

引用

页码：839 / 846

页数：8

共 32 条

[1] ANDRES CM, 1979, J BIOL CHEM, V254, P1388
[2] ACTIVITIES AND SOME PROPERTIES OF 5'-NUCLEOTIDASE, ADENOSINE KINASE AND ADENOSINE-DEAMINASE IN TISSUES FROM VERTEBRATES AND INVERTEBRATES IN RELATION TO CONTROL OF CONCENTRATION AND PHYSIOLOGICAL-ROLE OF ADENOSINE
ARCH, JRS
NEWSHOLME, EA
[J]. BIOCHEMICAL JOURNAL, 1978, 174 (03) : 965 - 977
[3] MECHANISMS OF ELEVATION OF ADENOSINE LEVELS IN ANOXIC HEPATOCYTES
BONTEMPS, F
VINCENT, MF
VANDENBERGHE, G
[J]. BIOCHEMICAL JOURNAL, 1993, 290 : 671 - 677
[4] BRADFORD MM, 1976, ANAL BIOCHEM, V72, P248, DOI 10.1016/0003-2697(76)90527-3
[5] FLUORESCENCE AND LOCATION OF TRYPTOPHAN RESIDUES IN PROTEIN MOLECULES
BURSTEIN, EA
VEDENKINA, NS
IVKOVA, MN
[J]. PHOTOCHEMISTRY AND PHOTOBIOLOGY, 1973, 18 (04) : 263 - 279
[6] PENETRATION OF SMALL MOLECULES INTO PROTEINS STUDIED BY QUENCHING OF PHOSPHORESCENCE AND FLUORESCENCE
CALHOUN, DB
VANDERKOOI, JM
ENGLANDER, SW
[J]. BIOCHEMISTRY, 1983, 22 (07) : 1533 - 1539
[7] KINETICS OF INTERACTION OF HIV REVERSE-TRANSCRIPTASE WITH PRIMER TEMPLATE
DIVITA, G
MULLER, B
IMMENDORFER, U
GAUTEL, M
RITTINGER, K
RESTLE, T
GOODY, RS
[J]. BIOCHEMISTRY, 1993, 32 (31) : 7966 - 7971
[8] INTRINSIC TRYPTOPHAN FLUORESCENCE OF SCHIZOSACCHAROMYCES-POMBE MITOCHONDRIAL F1-ATPASE - A POWERFUL PROBE FOR PHOSPHATE AND NUCLEOTIDE INTERACTIONS
DIVITA, G
DIPIETRO, A
DELEAGE, G
ROUX, B
GAUTHERON, DC
[J]. BIOCHEMISTRY, 1991, 30 (13) : 3256 - 3262
[9] EXPOSURE OF TRYPTOPHANYL RESIDUES IN PROTEINS - QUANTITATIVE-DETERMINATION BY FLUORESCENCE QUENCHING STUDIES
EFTINK, MR
GHIRON, CA
[J]. BIOCHEMISTRY, 1976, 15 (03) : 672 - 680
[10] DOES THE FLUORESCENCE QUENCHER ACRYLAMIDE BIND TO PROTEINS
EFTINK, MR
GHIRON, CA
[J]. BIOCHIMICA ET BIOPHYSICA ACTA, 1987, 916 (03) : 343 - 349

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