Amino acid biosynthesis is discussed most conveniently in the context of
families of amino acids that originate from a common precursor:
1. Glutamate or α-Ketoglutarate Family. Glutamate,
glutamine, glutathione, proline, arginine, putrescine, spermine, spermidine,
and in yeasts and molds, lysine. A tetrapyrrole (heme) precursor, δ-aminolevulinate,
arises from glutamate in some organisms.
2. Aspartate Family. Aspartate, asparagine, threonine,
methionine, isoleucine, and, in bacteria, lysine.
3. Pyruvate Family. Alanine, valine, leucine, and isoleucine.
4. Serine-Glycine or Triose Family. Serine, glycine cysteine, and
cystine.
In yeasts and molds, mammals, and some bacteria, δ-aminolevulinate
is formed by the condensation of glycine and succinate.
5. Aromatic Amino Acid Family. Phenylalanine, tyrosine, and
tryptophan. Additional compounds that can originate from the common aromatic
pathway include enterochelin, p-aminobenzoate, ubiquinone, menaquinone,
and NAD.
6. Histidine. This amino acid originates as an offshoot of the
purine pathway in that a portion of the histidine molecule is derived from the
intact purine ring.
Glutamine and Glutathione Synthesis
The importance of glutamate as one of
the primary amino acids involved in the assimilation of ammonia is N2 Cycle.
Glutamate and glutamine play acentral role in amino acid biosynthesis by the ready transfer of amino
or amide groups, respectively, in the
synthesis of other amino acids by transamination or transamidation reactions. Glutamine is synthesized from glutamate
with the participation of ammonia
and ATP.
Glutathione, a disulfide-containing amino acid whose functions have only recently begun to be understood in detail, is
synthesized in two steps. The coupling
of L-glutamate
and L-cysteine in the presence of ATP to form γ –glutamylcysteine is catalyzed by a specific synthase. In the presence
of glycine and ATP, glutathione synthase forms
glutathione.
 |
Fig.Pathways from glutamate to glutamine, glutathione, proline, ornithine, and ALA.
|
The
Proline Pathway
The pathway to proline
involves formation of γ -glutamylphosphate from L-glutamate and ATP by γ
-glutamyl kinase (ProB).
Aminolevulinate
Synthesis
In S. enterica and E. coli, δ-aminolevulinic acid
(ALA), the first committed precursor to tetrapyrroles, arises from glutamate.
This C5 pathway, which was originally thought to occur primarily in plants and
algae, is now firmly established as a major route to ALA in several bacterial
species. Prior to this discovery, the condensation of glycine and succinyl-CoA by the enzyme ALA synthase (the C4 pathway) was considered
to be the only route of ALA formation. It is still the major route of ALA
formation in mammals, fungi, and certain bacteria, such as Rhodopseudomonas
sphaeroides, R. capsulatus, and Bradyrhizobium japonicum. The C5 pathway
to ALA involves conversion of glutamate to glutamyl-tRNAGlu by glutamyl-tRNA
synthetase, reduction to glutamate γ -semialdehyde (GSA) by an
NADPH-dependent glutamyl-tRNA reductase (HemA), and transamination by glutamate
γ -semialdehyde aminomutase (HemL) to form ALA.
The Arginine Pathway
Bacteria and fungi synthesize ornithine via a series of N-acetyl
derivatives. The function of the N-acetyl group is to
prevent the premature cyclization of 1-pyrroline-5-carboxylate to proline.
There is a divergence in the pathway in differentorganisms depending on the
manner in which the acetyl group is removed. In Enterobacteriaceae and Bacillaceae, N-acetylornithine is deacylated via acetylornithine deacetylase (ArgE). In N. gonorrhoeae, Pseudomonadaceae, cyanobacteria,
photosynthetic bacteria, and yeasts and molds, the acetyl group of
N-acetylornithine is recycled by ornithine acetyltransferase (ArgJ).
Carbamoyl phosphate is a common precursor in the biosynthesis of
arginine and pyrimidines. In E. coli and S. enterica a single carbamoyl
phosphate synthetase catalyzes the reaction
Ammonia can replace glutamine as a nitrogen donor in vitro, but
glutamine is the physiologically
preferred substrate, and K+ and Mg2+ are required participants.
Arginine degradation in E. coli, K. pneumoniae, and P. aeruginosa may
follow yet another catabolic pathway: the arginine succinyltransferase (AST)
pathway. In E. coli the enzymes in this pathway are encoded by genes in the
astCADBE operon representing the structural genes for arginine
succinyltransferase, succinylarginine dihydrolase, succinylornithine
transaminase, succinylglutamic semialdehyde dehydrogenase,
and succinylglutamate desuccinylase.
Disruption of any of the genes in this pathway prevents arginine
catabolism and impairs ornithine utilization. In P. aeruginosa these same genes
are designated aru (for arginine utilization). Arginine metabolism is of
considerable significance in P. aeruginosa as evidenced by the strong
chemotactic activity for this amino acid and the fact that there are four
different catabolic pathways for arginine utilization: arginine deiminase,
arginine succinyltransferase (AST), arginine dehydrogenase, and arginine decarboxylase.
In S. cerevisiae, N. crassa, and in mammalian cells, arginine is degraded via
the arginase pathway. In fungi, the arginine catabolic enzymes arginase
(encoded by CAR1)and ornithine transaminase (encoded by CAR1) work in tandem to
degrade arginine.
