Two pathways have been identified in nature for the synthesis of lysine. The
diaminopimelate (DAP) pathway belongs to the
aspartate derived biosynthetic family, which is also involved in the synthesis of
threonine,
methionine and
isoleucine, whereas the
α-aminoadipate (AAA) pathway is part of the
glutamate biosynthetic family.
DAP pathway The DAP pathway is found in both
prokaryotes and plants and begins with the
dihydrodipicolinate synthase (DHDPS) (E.C 4.3.3.7)
catalysed condensation reaction between the aspartate derived, L-aspartate semialdehyde, and
pyruvate to form (4
S)-4-hydroxy-2,3,4,5-tetrahydro-(2
S)-dipicolinic acid (HTPA). The product is then
reduced by
dihydrodipicolinate reductase (DHDPR) (E.C 1.3.1.26), with
NAD(P)H as a proton donor, to yield 2,3,4,5-tetrahydrodipicolinate (THDP). From this point on, four pathway variations have been found, namely the acetylase, aminotransferase, dehydrogenase, and succinylase pathways. Both the acetylase and succinylase variant pathways use four
enzyme catalysed steps, the aminotransferase pathway uses two enzymes, and the dehydrogenase pathway uses a single enzyme. These four variant pathways converge at the formation of the penultimate product,
meso‑diaminopimelate, which is subsequently enzymatically
decarboxylated in an irreversible reaction catalysed by
diaminopimelate decarboxylase (DAPDC) (E.C 4.1.1.20) to produce L-lysine. The DAP pathway is regulated at multiple levels, including upstream at the enzymes involved in aspartate processing as well as at the initial DHDPS catalysed condensation step. Lysine imparts a strong
negative feedback loop on these enzymes and, subsequently, regulates the entire pathway. It has also been reported that an alternative variant of the AAA route has been found in
Thermus thermophilus and
Pyrococcus horikoshii, which could indicate that this pathway is more widely spread in prokaryotes than originally proposed. The first and
rate-limiting step in the AAA pathway is the condensation reaction between acetyl-CoA and α‑ketoglutarate catalysed by
homocitrate-synthase (HCS) (E.C 2.3.3.14) to give the intermediate homocitryl‑CoA, which is
hydrolysed by the same enzyme to produce
homocitrate. Homocitrate is enzymatically
dehydrated by
homoaconitase (HAc) (E.C 4.2.1.36) to yield
cis-homoaconitate. HAc then catalyses a second reaction in which
cis-homoaconitate undergoes
rehydration to produce
homoisocitrate. The resulting product undergoes an
oxidative decarboxylation by
homoisocitrate dehydrogenase (HIDH) (E.C 1.1.1.87) to yield α‑ketoadipate. AAA is then formed via a
pyridoxal 5′-phosphate (PLP)-dependent
aminotransferase (PLP-AT) (E.C 2.6.1.39), using glutamate as the amino donor. From this point on, the AAA pathway varies with [something is missing here ? -> at the very least, section header! ] on the kingdom. In fungi, AAA is reduced to α‑aminoadipate-semialdehyde via AAA reductase (E.C 1.2.1.95) in a unique process involving both
adenylation and reduction that is activated by a
phosphopantetheinyl transferase (E.C 2.7.8.7). Once the semialdehyde is formed,
saccharopine reductase (E.C 1.5.1.10) catalyses a condensation reaction with glutamate and NAD(P)H, as a proton donor, and the
imine is reduced to produce the penultimate product, saccharopine. The final step of the pathway in fungi involves the
saccharopine dehydrogenase (SDH) (E.C 1.5.1.8) catalysed oxidative
deamination of saccharopine, resulting in L-lysine. In a variant AAA pathway found in some prokaryotes, AAA is first converted to
N‑acetyl-α-aminoadipate, which is
phosphorylated and then reductively
dephosphorylated to the ε-aldehyde. The aldehyde is then
transaminated to
N‑acetyllysine, which is deacetylated to give L-lysine. However, the enzymes involved in this variant pathway need further validation. ==Catabolism==