The Affinity of Pyridoxal 5′-Phosphate for Folding Intermediates of Escherichia coli Serine Hydroxymethyltransferase

The reaction catalyzed by serine hydroxymethyltransferase (SHMT), the transfer of C␤ of serine to tetrahydropteroylglutamate, represents in Eucarya and Eubacteria a major source of one-carbon (C 1 ) units for several essential biosynthetic processes. In many Archaea, C 1 units are carried by modified pterin-containing compounds, which, although structurally related to tetrahydropteroylglutamate, play a distinct functional role. Tetrahydromethanopterin, and a few variants of this compound, are the modified folates of methanogenic and sulfate-reducing Archaea. Little information on SHMT from Archaea is available, and the metabolic role of the enzyme in these organisms is not clear. This contribution reports on the purification and characterization of recombinant SHMT from the hyperthermophilic methanogen Methanococcus jannaschii. The enzyme was characterized with respect to its catalytic, spectroscopic, and thermodynamic properties. Tetrahydromethanopterin was found to be the preferential pteridine substrate. Tetrahydropteroylglutamate could also take part in the hydroxymethyltransferase reaction, although with a much lower efficiency. The catalytic features of the enzyme with substrate analogues and in the absence of a pteridine substrate were also very similar to those of SHMT isolated from Eucarya or Eubacteria. On the other hand, the M. jannaschii enzyme showed increased thermoactivity and resistance to denaturating agents with respect to the enzyme purified from mesophilic sources. The results reported suggest that the active site structure and the mechanism of SHMT are conserved in the enzyme from M. jannaschii, which appear to differ only in its ability to bind and use a modified folate as substrate and increased thermal stability.Serine hydroxymethyltransferase (SHMT, 1 EC 2.1.2.1) catalyzes the reversible transfer of C␤ of serine to tetrahydropteroylglutamate (H 4 PteGlu) to form glycine and 5,10-methylene-H 4 PteGlu. In Eukarya and Eubacteria, H 4 PteGlu functions as a carrier of C 1 units in several oxidation states, which are used in the biosynthesis of important cellular components, such as purines and thymidylate, in the regeneration of methionine from homocysteine or, in acetogenic bacteria, in the synthesis of acetyl-CoA. The reaction catalyzed by SHMT represents in these organisms one of the major loading routes of C 1 units onto the folate carrier (1). In methanogens and several other Archaea, C 1 fragments from formyl to methyl oxidation levels are carried by tetrahydromethanopterin (H 4 MPT), a pterin-containing compound involved in methanogenesis. Although H 4 PteGlu and H 4 MPT are structurally similar in their pterin-like portion (Fig. 1) and in the role as C 1 units carriers, they are functionally distinct. H 4 MPT does not appear to be suited to most of the biosynthetic functions of H 4 PteGlu. Moreover, the biosynthetic pathways of the two carriers have few, if any, homologies, suggesting the possibility of separate evolutionary origins (2). In the metabolism of folates, SHMT represents a...

Section: Resultsmentioning

confidence: 54%

Catalytic and Thermodynamic Properties of Tetrahydromethanopterin-dependent Serine Hydroxymethyltransferase from Methanococcus jannaschii

Angelaccio¹,

Chiaraluce²,

Consalvi³

et al. 2003

“…7, a and b) exhibit a different composition of secondary structure elements for apo-compared with holo-OASS. In contrast, other PLP-dependent enzymes, including serine hydroxymethyltransferase (39,40), mitochondrial aspartate aminotransferase (41) (fold type I), and tryptophan synthase (42) (fold type II), exhibit similar spectra for the apo-and holoenzyme. Despite the well known uncertainty in the quantitative evaluation of secondary structure content from CD spectra, the calculated values for holo-OASS are in good agreement with the crystallographic data (Table II).…”

Section: Discussionmentioning

confidence: 99%

Role of Pyridoxal 5′-Phosphate in the Structural Stabilization of O-Acetylserine Sulfhydrylase

Bettati¹,

Benci²,

Campanini³

et al. 2000

Proteins belonging to the superfamily of pyridoxal 5-phosphate-dependent enzymes are currently classified into three functional groups and five distinct structural fold types. The variation within this enzyme group creates an ideal system to investigate the relationships among amino acid sequences, folding pathways, and enzymatic functions. The number of known three-dimensional structures of pyridoxal 5-phosphate-dependent enzymes is rapidly increasing, but only for relatively few have the folding mechanisms been characterized in detail. The dimeric O-acetylserine sulfhydrylase from Salmonella typhimurium belongs to the ␤-family and fold type II group. Here we report the guanidine hydrochloride-induced unfolding of the apo-and holoprotein, investigated using a variety of spectroscopic techniques. Data from absorption, fluorescence, circular dichroism, 31 P nuclear magnetic resonance, time-resolved fluorescence anisotropy, and photon correlation spectroscopy indicate that the O-acetylserine sulfhydrylase undergoes extensive disruption of native secondary and tertiary structure before monomerization. Also, we have observed that the holo-O-acetylserine sulfhydrylase exhibits a greater conformational stability than the apoenzyme form. The data are discussed in light of the fact that the role of the coenzyme in structural stabilization varies among the pyridoxal 5-phosphate-dependent enzymes and does not seem to be linked to the particular enzyme fold type.

“…The addition of glycine and H 4 PteGlu to every SHMT that has been studied results in an abortive complex that absorbs near 500 nm, which is characteristic of a quinonoid structure known to be on the catalytic pathway. However, the Pro 258 and Pro 264 mutants do not give this complex with glycine and H 4 PteGlu, suggesting that they are blocked in going from the external aldimine to the quinonoid intermediate. A previous study of sheep liver SHMT also showed that the P297R mutant (equivalent to Pro 258 ) resulted in the loss of 85% of its activity (23).…”

Section: Role Of Promentioning

confidence: 99%

“…Double reciprocal plots of initial velocity versus serine concentration was used to determine K m and k cat values with saturating levels of H 4 PteGlu (0.2 mM) used as the cosubstrate. The K d for H 4 PteGlu was determined by a spectrophotometric method involving the formation of an abortive complex with glycine that absorbs uniquely at 495 nm (10). Saturating levels of glycine (50 mM) were used, and the absorbance at 492 nm of the SHMT⅐Gly⅐H 4 PteGlu abortive complex was determined as a function of increasing concentrations of H 4 PteGlu.…”

Section: Methodsmentioning

confidence: 99%

See 1 more Smart Citation

Role of Proline Residues in the Folding of Serine Hydroxymethyltransferase

Boja

Schirch

2003

Self Cite

Previous studies on the folding mechanism of Escherichia coli serine hydroxymethyltransferase (SHMT) showed that the final rate determining folding step was from an intermediate that contained two fully folded domains with N-terminal segments of approximately 55 residues and interdomain segments of approximately 50 residues that were still solvent exposed and subject to proteolysis. The interdomain segment contains 3 Pro residues near its N terminus and 2 Pro residues near its C terminus. The 5 Pro residues were each mutated to both a Gly and Ala residue, and each mutant SHMT was purified and characterized with respect to kinetic properties, stability, secondary structure, and folding mechanism. The results showed that Pro 214 and Pro 218 near the N terminus of the interdomain segment are not critical for folding, stability, or activity. The P216A mutant also retained most of the characteristics of the native enzyme, but its folding rate was altered. However, the P216G mutant was severely compromised in folding into a catalytically competent enzyme. Mutation of both Pro 258 and Pro 264 had altered folding kinetics and resulted in enzymes that expressed little catalytic activity. The Phe 257 -Pro 258 bond is cis in its configuration, and the P258A mutant SHMT showed reduced thermal stability. Pro 216 , Pro 258 , and Pro 264 are conserved in all 53 known sequences of this enzyme. The results are discussed in terms of the role of each Pro residue in maintaining the structure and function of SHMT and a possible role in pyridoxal 5 -phosphate addition to the apo-enzyme.