Replying to Wei et al. Nature Communications https://doi.org/10.1038/s41467-019-13492-9 (2019)

The manuscript entitled “Conformational fitting of a flexible oligomeric substrate does not explain the enzymatic PET degradation” by Wei et al.1 raises a question on the conclusion reached in our published work, particularly regarding the docking calculations of PET substrate into the PETase from Ideonella sakaiensis (IsPETase)2. The authors showed the ethylene glycol torsion angle Ψ in an amorphous PET material of 0.25 mm thickness (Goodfellow Cambridge Ltd.) using solid-state nuclear magnetic resonance experiments and determined trans/gauche ratio of 9:91 at 30 °C in good agreement with the previous report on amorphous PET (14 ± 5%)3. Based on the result, they suggested that the conformation of the docked 2-HE(MHET)4 in our published work that showed a trans content of ethylene glycol higher than 25% is rarely present in amorphous PET polymer chains, and claimed that the residues in subsite IIb and IIc we suggested are unlikely to interact with the two MHET moieties of 2-HE(MHET)4. To support the latter statement, they further demonstrated that the transition from gauche to trans conformation is highly restricted in amorphous PET at 30 °C by magic-angle-spinning nuclear magnetic resonance method. They also suggested that, instead of the perfect accommodation, the key factor facilitating the substrate binding seems to be the fragile contact between the phenylene moieties and the surrounding hydrophobic residues. In general, we agree that the comments by Wei et al. provide concrete experimental results showing that ethylene glycol units of amorphous PET polymer do not have the free rotational properties to fit into its substrate binding site as the form of 2-HE(MHET)4 at 30 °C. Thus, the study provides the scientific community with useful information on PET degradation by IsPETase.

However, our previous docking calculations2 were independent of temperature setting and not restricted to the temperature of 30 °C. Although IsPETase cannot maintain its activity at high temperature due to its low thermal stability, efforts to increase thermal stability of the enzyme have already been reported4. Thus, an engineered IsPETase with high thermal stability might be able to accommodate the PET substrate in the manner we presented at temperatures higher than 30 °C as the trans content of the material was increased to 56% at 70 °C1.

Moreover, we did not use the Goodfellow amorphous PET in our published works2,4, which counters the comment that IsPETase showed almost “no” activity against crystalline PET polymer1. It was also previously shown that the semi-crystalline PET material exhibits much higher trans conformation of ethylene glycol than amorphous one at ambient temperature3. Thus, we believe that the authors’ claims regarding the residues in subsite IIb and IIc may not apply under all conditions. In sum, while we agree that Wei et al. provide useful evidences that the used docking calculation is not suitable in amorphous PET at low temperature such as 30 °C, their observations are not necessarily incompatible with the general findings of our previous work2. We anticipate that Wei et al.’s work and our own will inspire future studies aimed at unraveling the exact mechanisms of PET degradation.