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Query: UNIPROT:Q9NXG6 (
PH4
)
87
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Computer simulation analysis of the experimental data showed that Cl'-keto
PH4
and C2'-keto
PH4
were sequential intermediates of the reduction of PPH4 to
BH4
by SPR and that the reaction in the last step of the
BH4
biosynthesis proceeds as follows: PPH4-->Cl'-keto
PH4
-->C2'-keto
PH4
-->
BH4
Cl'-keto
PH4
is not detectable in the reduction of PPH4 by the purified SPR at neutral pH since isomerization (-->) [8] may occur far more rapidly than the first reduction (-->).
...
PMID:Role of enzymes in tetrahydrobiopterin biosynthesis: computer analysis of the sequential reaction of the last step. 129 96
The chiral specificities of bovine striatal tyrosine hydroxylase (TH) (unphosphorylated and phosphorylated by cAMP-dependent protein kinase) and rat liver phenylalanine hydroxylase (PH) were examined at physiological pH using the pure C6 stereoisomers of 6-methyl- and 6-propyl-5,6,7,8-tetrahydropterin (6-methyl-
PH4
and 6-propyl-
PH4
) and (6R)- and (6S)-tetrahydrobiopterin (
BH4
). Both PH and phosphorylated TH have substantially higher Vmax values with the unnatural (6R)-propyl-
PH4
than the natural (6S)-propyl-
PH4
(approximately 6- and 11-fold, respectively). However, the Km's are also higher such that Vmax/Km is almost unaffected by C6 chirality. Unphosphorylated TH has equal Km values for both isomers of 6-propyl-
PH4
, but has about a 6 times greater Vmax with the unnatural isomer, making it the fastest cofactor yet for this form of the enzyme. With the shorter 6-methyl group, chiral differences are still recognized by phosphorylated TH but hardly at all by PH. Inhibition of both PH and TH by amino acid substrate which occurs with (6R)-
BH4
as cofactor is also observed with (6S)-propyl-
PH4
but not with (6S)-
BH4
, (6R)-propyl-
PH4
, or (6R)- or (6R,S)-methyl-
PH4
. The Km for (6S)-
BH4
with phosphorylated TH is nearly 3 times higher than with (6R)-
BH4
, but Vmax is unchanged. With unphosphorylated TH, (6S)-
BH4
produces very low decelerating rates, which was shown not to be due to irreversible inactivation of the enzyme. The Km for (6R)-
BH4
with either hydroxylase is 10 times higher than for the equivalently configured (6S)-propyl-
PH4
. Comparison of these two cofactors reveals that the 1' and 2' side-chain hydroxyl groups of the natural cofactor promote different regulatory functions in PH than in TH.
...
PMID:Role of C6 chirality of tetrahydropterin cofactor in catalysis and regulation of tyrosine and phenylalanine hydroxylases. 168 99
The structure of the cofactor binding domain of tyrosine hydroxylase (TH) was examined at physiological pH by determining kinetic parameters of (R)-tetrahydrobiopterin [(R)-
BH4
] and a series of tetrahydropterin (
PH4
) derivatives (6-R1-6-R2-
PH4
: R1 = H and R2 = methyl, hydroxymethyl, ethyl, methoxymethyl, phenyl, and cyclohexyl; R1 = methyl and R2 = methyl, ethyl, propyl, phenyl, and benzyl). A minimally purified TH preparation that was not specifically phosphorylated (designated as "unphosphorylated") was compared with enzyme phosphorylated with cAMP-dependent protein kinase. The Km for tyrosine with most tetrahydropterin analogues ranged between 20 and 60 microM with little decrease upon phosphorylation. Two exceptions were an unusually low Km of 7 microM with 6-ethyl-
PH4
and a high Km of 120 microM with 6-phenyl-6-methyl-
PH4
, both with phosphorylated TH. Tyrosine substrate inhibition was elicited only with (R)-
BH4
and 6-hydroxymethyl-
PH4
. With unphosphorylated TH (with the exception of 6-benzyl-6-methyl-
PH4
, Km = 4 mM) an inverse correlation between cofactor Km and side-chain hydrophobicity was observed ranging from a high with (R)-
BH4
(5 mM) to a low with 6-cyclohexyl-
PH4
(0.3 mM). An 8-fold span of Vmax was seen overall. Phosphorylation caused a 0.6-4-fold increase in Vmax and a 35-2000-fold decrease in Km for cofactor, ranging from a high of 60 microM with 6-methyl-
PH4
to a low of 0.6 microM with 6-cyclohexyl-
PH4
. A correlation of the size of the hydrocarbon component of the side chain with affinity is strongly evident with phosphorylated TH, but in contrast to unphosphorylated enzyme, the hydroxyl groups in hydroxymethyl-
PH4
(20 microM) and (R)-
BH4
(3 microM) decrease Km in comparison to that of 6-methyl-
PH4
. Although 6,6-disubstituted analogues were found with affinities near that of (R)-
BH4
(e.g., 6-propyl-6-methyl-
PH4
, 4 microM), they were frequently more loosely associated with phosphorylated TH than their monosubstituted counterparts (6-phenyl-
PH4
, 0.8 microM; cf. 6-phenyl-6-methyl-
PH4
, 8 microM). A model of the cofactor side-chain binding domain is proposed in which a limited region of nonpolar protein residue(s) capable of van der Waals contact with the hydrocarbon backbone of the (R)-
BH4
dihydroxypropyl group is opposite to a recognition site for hydroxyl(s). Although interaction with either the hydrophilic or hydrophobic regions of unphosphorylated tyrosine hydroxylase is possible, phosphorylation by cAMP-dependent protein kinase appears to optimize the simultaneous operation of both forces.
...
PMID:Changes in the cofactor binding domain of bovine striatal tyrosine hydroxylase at physiological pH upon cAMP-dependent phosphorylation mapped with tetrahydrobiopterin analogues. 256 33
The 6-lactoyl tetrahydropterin (C1'-keto
PH4
) isomerase activity of sepiapterin reductase, which was found in our recent work (Katoh and Sueoka (1987) J. Biochem. 101, 275-278) as a novel activity of the enzyme, i.e., the conversion of C1'-keto
PH4
to 6-1'-hydroxy-2'-oxopropyl tetrahydropterin (C2'-keto
PH4
) without coenzymes, could be enhanced by a small amount of NADPH or NADP+. The concentration of NADP+ required for the maximal stimulation was approximately the same as the concentration of the enzyme subunit. When NADP+ was added with the enzyme and C1'-keto
PH4
at pH 8.6, the reaction sequence of C1'-keto
PH4
----C2'-keto
PH4
----tetrahydrobiopterin (
BH4
) was observed in the presence of dithioerythritol. These observations suggest that the coenzyme stimulating the isomerase function of sepiapterin reductase may be involved in the two sequential reductions, from pyruvoyl tetrahydropterin to
BH4
, by causing internal rearrangement of the keto group of the first intermediate, C1'-keto
PH4
, to form the second one, C2'-keto
PH4
.
...
PMID:Coenzyme stimulation of isomerase activity of sepiapterin reductase in the biosynthesis of tetrahydrobiopterin. 328 29
Phenylalanine hydroxylase (PAH) is the key enzyme in the catabolism of L-Phe. The natural cofactor of PAH, 6R-tetrahydrobiopterin (
BH4
), negatively regulates the enzyme activity in addition to being an essential cosubstrate for catalysis. The analogue 6-methyltetrahydropterin (6M-
PH4
) is effective in catalysis but does not regulate PAH. Here, the thermodynamics of binding of
BH4
and 6M-
PH4
to human PAH have been studied by isothermal titration calorimetry. At neutral pH and 25 degrees C,
BH4
binds to PAH with higher affinity (Kd = 0.75 +/- 0.18 microM) than 6M-
PH4
(Kd = 16.5 +/- 2.7 microM). While
BH4
binding is a strongly exothermic process (DeltaH = -11.8 +/- 0.4 kcal/mol) accompanied by an entropic penalty (-TDeltaS = 3.4 +/- 0.4 kcal/mol), 6M-
PH4
binding is both enthalpically (DeltaH = -3.3 +/- 0.3 kcal/mol) and entropically (-TDeltaS = -3.2 kcal/mol) driven. No significant changes in binding affinity were observed in the 5-35 degrees C temperature range for both pterins at neutral pH, but the enthalpic contribution increased with temperature rendering a heat capacity change (DeltaCp) of -357 +/- 26 cal/mol/K for
BH4
and -63 +/- 12 cal/mol/K for 6M-
PH4
. Protons do not seem to be taken up or released upon pterin binding. Structure-based energetics calculations applied on the molecular dynamics simulated structures of the complexes suggest that in the case of
BH4
binding, the conformational rearrangement of the N-terminal tail of PAH contribute with favorable enthalpic and unfavorable entropic contributions to the intrinsic thermodynamic parameters of binding. The entropic penalty is most probably associated to the reduction of conformational flexibility at the protein level and disappears for the L-Phe activated enzyme. The calculated energetic parameters aid to elucidate the molecular mechanism for cofactor recognition and the regulation of PAH by the dihydroxypropyl side chain of
BH4
.
...
PMID:Thermodynamic characterization of the binding of tetrahydropterins to phenylalanine hydroxylase. 1549 24
