The amino acid sequence of each of the E. coli lysine (DAP), leucine, and T. thermophilus lysine (AAA) biosynthetic enzymes, was used as a query to probe the completely sequenced genomes database of KEGG (Kyoto Encyclopaedia of Genes and Genomes) consisting of 29 Archaea, 423 Bacteria and 35 Eucaryotes. The bidirectional best-hit (BBH) criterion (see Methods) was used to retrieve orthologous sequences. Data obtained, schematically reported in Figure 2 and representative of a dataset of 68 bacterial and 15 archaeal genomes, revealed that:

i) Lysine (AAA) biosynthetic genes are very rarely represented in Bacteria, in that just two organisms harbour the complete set of AAA biosynthetic genes, i.e. T. thermophilus and D. radiodurans. No other bacterium possesses the complete set of enzymes required to synthesize lysine via the AAA route. Six Archaea display a complete set of lysine (AAA) biosynthetic genes, namely Pyrococcus and Sulfolobus strains, and Thermococcus kodakaraensis.

ii) Lysine (DAP) biosynthetic genes are widespread among Bacteria. Among them, 18 (micro)organisms possess a complete set of genes (9) for lysine biosynthesis through the DAP route. The small number of lysine (DAP) biosynthetic genes in some bacterial strains is very likely due to the absence of the corresponding metabolic route, which, in turn, is related to the parasitic lifestyle of these organisms. Such a lifestyle may allow these bacteria to acquire essential compounds directly from the metabolic activities of their host and the adaptation to this environmental condition might have caused the loss of entire metabolic routes or parts thereof.

Although some Archaea are known to synthesize lysine through the DAP pathway 232425262728, it is not still completely clear which of the possible variants they use. Nonetheless, no archaeon possesses a number of genes compatible with the number required by the succinylasic variant. When the ddh sequence of Corynebacterium glutamicum, whose product is involved in the dehydrogenasic variant of lysine (DAP) pathway, was used in a BLAST probing, the only ddh archaeal homolog sequence was found in Archaeoglobus fulgidus genome (data not shown).

iii) The complete set of leucine biosynthetic genes is present in most of Bacteria and Archaea that possess either all the five leucine biosynthetic genes or four of them (lacking the last gene of leucine biosynthetic route, ilvE). This different distribution of ilvE, had already been observed by Velasco et al. 19.

iv) Arginine biosynthetic genes are widespread among Archaea and Bacteria. Even though a complete set is found only in a restricted number of organisms, most of them possess more than half (from five up to eight) of the enzymes required for the biosynthesis of ornithine and arginine, confirming the previous observation that they are synthesized through N-acetylated intermediates both in Bacteria and in Archaea 29.

A comparative analysis of the lysine, leucine, and arginine biosynthetic routes of completely sequenced organisms belonging to the three cellular domains (Eucarya, Bacteria, and Archaea) was carried out. Data obtained for some representative organisms belonging to the three cellular domains are shown in Figures 3, 4, and 5 and can be summarised as reported below.

In most of archaeal, bacterial, and eukaryotic (micro)organisms each of the three amino acid is synthesized through a specific metabolic route and each enzyme catalyzes a single step of the metabolic pathway it belongs to. The only exception is represented by the archaeon Pyrococcus horikoshii (see below); moreover a bifunctional enzyme, coded for by argD, interconnecting arginine and lysine biosyntheses was identified and characterized in Escherichia coli (see below).

In all of the organisms analyzed, leucine is synthesized through the typical biosynthetic pathway, consisting of the enzymatic steps catalyzed by 3-isopropylmalate synthase, 2-isopropylmalate isomerase, 3-isopropylmalate dehydrogenase, and α-ketoisocaproate transaminase, respectively. The four enzymes are coded for by the procaryotic leuA, leuCD, leuB, and ilvE genes, or by the eucaryotic LEU9\4, LEU1, LEU2, and BAT1\2 (Figures 3, 4, 5).

Similarly, arginine biosynthesis proceeds through the same steps in all the organisms taken into account (Figures 3, 4, 5).

The lysine biosynthesis is much more intriguing; the amino acid can be synthesized through either the AAA or the DAP pathway (see Background). The AAA pathway was found in T. thermophilus and D. radiodurans, and a modified version of it was found in S. cerevisiae (Figure 4a and Figure 5a). The first four metabolic steps are shared by the two organisms and are evolutionarily related to the corresponding ones of leucine biosynthesis 819. The second moiety of these two AAA versions is different. In T. thermophilus lysine biosynthesis is achieved by the products of lysZ, Y, J, and K, whose sequences are homologous to argB, C, D, and E, respectively, whereas in S. cerevisiae lysine biosynthesis is completed by LYS2, LYS9, LYS1, that have no homolog among the genes of the biosynthetic pathways we took into account.

In the other Bacteria and in some Archaea, lysine is synthesized through the DAP pathway. Even in this case, several alternatives are possible. In the γ-proteobacterium E. coli (Figure 4c) the product of DapB is converted in LL-meso-diaminopimelate through four sequential enzymatic steps, known as the succinylate variant, and performed by DapD, ArgD, DapE, and DapF. Moreover, the enzyme coded for by argD exhibits both N-acetyl-ornithine and N-succinyl-L,L-diaminopimelate aminotransferase activities, with a very similar catalytic efficiency and identical kinetic mechanism, suggesting that this enzyme can play a role in both lysine and arginine biosynthesis 30. In C. glutamicum (Figure 4b) another version of the pathway has been disclosed: tetrahydrodipicolinate can be converted into meso-diaminopimelate by the activity of diaminopimelate dehydrogenase (ddh) in a single metabolic step. It is highly likely that this catalytic step is present also in the DAP pathway of the archaeon Haloarcula hispanica (Figure 3a) 23. Interestingly, in C. glutamicum two distinct enzymes (ArgD and DapC) can perform the reaction that in E. coli is carried out by a single one. Thus, the enzymes encoded by argD and dapC in C. glutamicum can be considered specific for the biosynthetic routes of arginine and lysine, respectively.

Arabidopsis thaliana is known to synthesize lysine through the DAP pathway 1531. A DAP variant has been recently identified in this plant that utilizes a novel transaminase (LL-aminoadipate aminotransferase, the product of ORF At4g33680) that specifically catalyzes the conversion of tetrahydrodipicolinate to LL-diaminopimelate, a reaction requiring three enzymes in the DAP-pathway variant found in E. coli 32.

The archaeon P. horikoshii represents the main exception. In fact, in this organism just one pathway for the biosynthesis of all these three amino acids has been identified so far (Figure 3b). On the basis of sequence comparison and phylogenetic analyses, it has been suggested 9 that ORF PH1722, PH1724, PH1726, and PH1727 (see Figure 3b) from P. horikoshii might be involved in leucine biosynthesis as well as in the AAA variant of lysine biosynthesis, and that ORF PH1720, PH1718, PH1716, and PH1715 (Figure 3b) might be involved in the biosynthesis of both lysine (through the AAA one) and arginine. Even though it cannot be ruled a priori out the possibility that other uncharacterized routes for the biosynthesis of these amino acids may exist 33, it has been suggested that P. horikoshii possesses a unique amino acid biosynthetic system by which several amino acids are synthesized by a limited number of enzymes with broad substrate specificity 8.

Data shown in Figures 3, 4 and 5 reveal that some steps of lysine, leucine, and arginine biosynthetic pathways are strongly conserved among the organisms we have taken into account. These steps are the first three of leucine route (performed by LeuA, LeuCD, and LeuB), the central ones of the arginine route (performed by ArgB, ArgC, ArgD, and ArgE), and the first two of lysine (DAP) route (performed by Ask and Asd). Moreover, these enzymes, share a significant degree of sequence similarity with some of those involved in the AAA lysine biosynthesis 19. As shown in Figure 1, leuA, leuCD, and leuB appeared to be paralogous to lysS, lysTU, and homoisocitrate dehydrogenase coding gene, respectively. A similar paralogy exists between argB, ask, and lysZ, as well as among argC, asd, and lysY. Velasco et al. 19 suggested that all of them are the outcome of one or more duplication events of an ancestral set of genes. According to the patchwork hypothesis 2, these ancestral genes might have encoded enzymes possessing broad substrate specificity and have been involved in different metabolic pathways.

On the basis of the analysis of phylogenetic distribution, Velasco et al. 19 also proposed that the DAP variant of lysine biosynthesis appeared earlier than the AAA one. However, a different scenario can be proposed. The model that we describe here predicts the existence of an ancestral pathway consisting of a set of genes, some of which coding for unspecific enzymes able to react with a wide range of chemically related substrates. This metabolic pathway interconnected lysine, leucine, arginine and also methionine and threonine biosyntheses and nitrogen fixation (Figure 6). According to the model, the first step of the primordial route was catalyzed by the ancestor of the extant isopropylmalate synthase (IPMase, LeuA) and homocitrate synthase (HCase, NifV), that are involved in leucine biosynthesis and nitrogen fixation, respectively. The paralogy existing between their coding genes has not been analyzed in detail up to now, but its description is beyond the scope of the present work. Moreover, the first three steps of this ancestral biosynthetic pathway might have included the reactions that, in the extant organisms, are separately accomplished by the enzymes of leucine and lysine-AAA pathways. Moreover, the last four steps, involving the ancestral copies of the extant ArgB, C, D, and LysZ, Y, J, K, may have been able to recognize different substrates and to catalyze their conversion into ornithine, a fundamental intermediary in arginine biosynthesis.

Even though these ancestral enzymes may have been the backbone of the hypothetical common route, some others might have been necessary to complete the biosynthesis of all the corresponding products. An ancestor of the extant IlvE might have catalyzed the conversion of 2-oxoisocaproate into leucine, the final step of leucine biosynthesis, whereas an unspecific aminotransferase may have accomplished the transamination of α-aminoadipate, the extant role of LysN.

Moreover, an ancestral copy of LysX, which is evolutionarily related to E. coli RimK 34, was probably involved in the modification of α-aminoadipate to N-acetyl-α-aminoadipate, releasing the substrate of LysZ/ArgB/Ask ancestor. As shown in Figure 5, the model proposed does not contemplate the biosynthesis of LL-diaminopimelate in primordial cells, implying that the AAA pathway predated the appearance of the DAP pathway.

In conclusion, ancestral organisms may have been able to synthesize lysine, leucine and ornithine using just one pathway, consisting of a small number of enzymes endowed with a broad substrate specificity, permitting a clear interconnection of different metabolic routes.

On the basis of the structure and the relationships existing in the extant biosynthetic routes leading to lysine, leucine, or arginine we depict a possible evolutionary model that might explain the (complex) extant scenario.

The model predicts the existence of the above described ancestral pathway (Figures 6 and 7a) that appears to be very similar to that responsible for the biosynthesis of lysine, leucine, and ornithine in P. horikoshii (Figure 3b and 6). It has been proposed 8 that P. horikoshii might have developed unique amino acid biosynthetic systems in which several amino acids are synthesized by a limited number of enzymes with broad substrate specificity and that these enzymes might be the ancestors of the extant biosynthetic ones of lysine, leucine, and arginine.

If the idea of an ancestral common pathway for the biosynthesis of lysine, leucine and arginine is correct, this raises the question of how did the extant routes originate. Besides, which was the timing of their appearance? Here we propose a model that is in agreement with the Nishida's idea and predicts that the extant biosynthetic routes might have emerged after a set of duplication events involving the genes of the ancestral common pathway (Figure 7). According to the model, the first step (or one of the first steps) might have been the duplication of the genes encoding the enzymes catalysing the sixth and seventh steps of the route common to lysine and ornithine. These events gave raise to the ancestors of ask and asd genes and to the overall metabolic "grid" that has been found in P. horikoshii (Figures 3b and 7b). This idea is also supported by the phylogenetic analysis (see next section).

Later on, the duplication of the genes encoding the first three steps of the ancestral pathway and the further evolutionary divergence of the new copies might have originated the ancestor of leuA, leuCD, and leuB, which coded for enzymes with a more narrow substrate specificity, rendering the leucine biosynthesis independent from the ancestral common pathway (Figure 7c). The central steps of arginine biosynthesis, catalyzed by ArgB, ArgC, ArgD and ArgE, might have arisen from the duplication and further evolutionary divergence of the corresponding ancestral aspecific genes (Figure 7d). In this way the four metabolic routes leading to leucine, lysine, arginine, and methionine\threonine, respectively, became one independent from each other. This metabolic scheme corresponds to that found in T. thermophilus and D. radiodurans.

A further duplication of the bottom genes of the ancestral pathway led to the appearance of DapC and DapE; during this step the branch of the "DAP pathway" leading to lysine was completely assembled (Figure 7e) with the recruitment of dapC and dapE (that are homolog to the extant lysJ/argD and lysZ/argB, respectively), dapF, and lysA. On the basis of the available data, it is not still possible to discern between the possibility that the product of the reaction catalyzed by Asd directly interacts with DapC, or if other enzymes (possibly the ancestor of the extant dapA, dapB, and dapD) were required to complete the DAP route. However, it is possible that once the assembly of the lysine-branch of the DAP pathway was completed the primordial cells possessed two alternative ways to synthesize lysine. If the model we propose here is correct, it is possible that, in this context, the entire AAA pathway became superfluous. Hence, the fourth step (Figure 7e) of the model predicts that, after the completion of the DAP pathway to lysine, genes belonging to the AAA pathway were progressively lost; therefore those organisms lacking the DAP pathway, maintained the ability to synthesize lysine through the AAA route. The final step of the model (Figure 7f) predicts that lysine (DAP) may have been completely assembled, with the appearance of all the extant variants (deacetylasic, desuccynilasic, and dehydrogenasic), leading to the metabolic patterns found in E. coli and in many other microorganisms. The development of the DAP pathway might allow bacterial cells to acquire the possibility to insert LL-diaminopimelate and meso-diaminopimelate, that are both intermediaries of the DAP route, into their cell wall.

In our opinion, the duplication events from Figure 7a to Figure 7e would have predated the appearance of the Last Universal Common Ancestor (LUCA), which, according to Woese 35, would have been a complex community of progenotes, highly dynamic from a genomic viewpoint, a mix of heterogeneous primordial cells with different metabolic abilities that could be easily exchanged between the different entities of the community. According to this idea, cells with different metabolic grids such as those represented in Figure 7b and 7d might have co-existed in the "LUCA community". The model also predicts, according to Cavalier-Smith 36, that if the primordial cells were surrounded by a cell wall containing peptidoglycan, ornithine should have been one of the first, if not the very first, component of peptidoglycan (see Conclusions).

According to the model proposed, the metabolic pathway leading to methionine and threonine diverged from the ancestral pathway before lysine, leucine, and arginine biosynthetic ones. However, (at least) another plausible scenario can be depicted, involving the previous appearance of the leucine pathway and the further assembly of the others biosynthetic routes. In other words, is it possible to establish the relative timing of the separation of the extant three pairs of genes involved in lysine, arginine, threonine, and methionine biosynthesis, that is lysZ and lysY, argB and argC, and ask and asd?

Useful hints concerning this issue can be obtained by a phylogenetic analysis of the two paralogous triads (LysZ, ArgB, Ask, and LysY, ArgC, and Asd). To this purpose a dataset of all the retrieved LysZ, ArgB, Ask and, LysY, ArgC, and Asd amino acid sequences was aligned using the program ClustalW 37 and the multialignments obtained used to draw the phylogenetic trees shown in Figure 8. This analysis revealed that:

1. Ask sequences form a unique cluster, which is clearly separated from the other one containing all the ArgB and LysZ sequences involved in arginine and lysine (AAA) biosynthesis, respectively (Figure 8a).

2. Asd sequences form a unique cluster separated from ArgC and LysY sequences, involved in arginine and lysine biosynthesis, respectively (Figure 8b).

Hence, the topology of the tree in Figure 8a suggests that ArgB and LysZ sequences share a degree of sequence similarity higher than that exhibited with Ask, respectively. Similarly, the tree shown in Figure 8b, revealed that ArgC and LysY sequences share a degree of similarity higher than that exhibited with Asd. The overall body of phylogenetic data suggests that the first duplication event(s) involving the ancestral common genes might have originated the ancestor of the extant ask and asd genes; hence, argB and argC might be the outcome of a later duplication event of their corresponding ancestral sequences.

Thus, in our opinion, the model proposed in the previous section appeared to be in agreement with both phylogenetic analyses and the metabolic schemes shown in Figures 2, 3, 4.

Amino acid sequences were retrieved from GenBank and KEGG databases and were used to build a local database for BLASTp 44 probing that was performed using default parameters. Orthologs identification was achieved according to the bidirectional best-hit (BBH) criterion 4546. The relationship between gene x in genome A and gene y in genome B is called best-best hit when x is the best hit of query y against all genes in A and vice versa, and it is often used as an operational definition of ortholog 4547.

The ClustalW 37 program in the BioEdit 48 package was used to perform pairwise and multiple amino acid sequences alignments.

Phylogenetic trees were obtained with Mega 3 software 49 using the Neighbor-Joining (NJ) and the Minimum Evolution (ME) methods.