Figure 4 Characterization of the discrete NRPS domains and aminotransferase in vivo. LC-MS analysis (extracted ion chromatograms of m/z [M + H]+ 969.5 corresponding
to PLYA) of Streptomyces sp. MK498-98F14 wild type (WT) and mutants (ΔplyC, ΔplyD, ΔplyQ, ΔplyI, ΔplyS, ΔplyY and ΔplyN). Assembly of the cyclodepsipeptide by NRPSs After the C15 acyl side chain is assembled by 4 modular PKSs, it is transferred to 3-hydroxyleucine via an amide bond formation catalyzed by a NRPS, thus initiating the assembly of the peptide core. Within the biosynthetic gene cluster, there are 4 genes plyFGHX encoding modular NRPS proteins. Both PlyF and PlyG consist of two modules with seven domains (C-A1-PCP-E-C-A2-PCP) (Figure 2B). Active epimerase (E) domains are click here present indicating that the buy BI 10773 amino acids activated by PlyF-A1 and PlyG-A1 should be converted into d-configuration. selleck inhibitor Among the six nonproteinogenic amino acid residues, only two piperazic acid residues are d-configuration, so these two A domains (PlyF-A1 and PlyG-A1) are proposed to recognize and activate l-piperazic acid (4, Figure 2D) that was confirmed to be derived from l-ornithine [37]. This assumption can be supported by the findings
that PlyF-A1 shares 52-59% identity and 64-69% similarity to PlyG-A1, KtzH-A1 [38], and HmtL-A1 [39] (Additional file 1: Figure S4), and as well as the substrate specificity-conferring ten amino acids (DVFSVASYAK for PlyF-A1 and DVFSIAAYAK for PlyG-A1) Calpain are highly analogous to those of KtzH-A1 (DVFSVGPYAK) and HmtL-A1 (DVFSVAAYAK) [40, 41]. Both KtzH-A1 and HmtL-A1 were proposed to recognize and activate l-piperazic acid [38, 39]. PlyH contains five domains (C-A-M-PCP-TE) with a thioesterase (TE) domain present, indicating that PlyH is the last module of PLY NRPS system and responsible for the release and cyclization of the peptide chain via an ester bond formation. It is striking that an active methyltransferase (M) domain (containing the SAM-binding sites EXGXGXG) is present in the PlyH [42], but no N-methyl group
is present in the structure of PLYs. The presence of this M domain remains enigmatic. Based on the PLY structure analysis and NRPS machinery [43], PlyH-A is proposed to recognize N-hydroxyvaline (5, Figure 2E) as its substrate, but not valine because its substrate specificity-conferring codon sequences (DAPFEALVEX) are significantly distinct from those found for valine-specificity (DALWMGGTFK) [44]. Subsequently, the whole sequence of PlyH-A shows 76% identity and 83% similarity to that of PlyF-A2, indicating that PlyF-A2 is specific for N-hydroxyalanine (6, Figure 2E and Additional file 1: Figure S5). These assignments are consistent with the amino acid sequence of the peptide core of PLYs.