Pentaerithrityl tetranitrate

The target chemical pentaerithrityl tetranitrate is predicted as not ready biodegradable by Catalogic 301F. The predicted BOD at 28 is 7%. Pentaerithrityl tetranitrate was found to be out of structural domain for the Catalogic biodegradation model 301F. The compound has 94.24% unknown structural fragments (-C-CH2-NO3) and 4.76% correct fragments (C(CH2)(CH2)(CH2)(CH2)). Nevertheless, the observed metabolic map of pentaerithrityl tetranitrate was found in the database with documented metabolism data. Sensitivity of the prediction of metabolism is 100%. Therefore, the prediction of the degradation pathway should be considered as an indication for a reliable prediction of BOD.

A mixed microbial culture capable of metabolizing the explosive pentaerythritol tetranitrate (PETN) was obtained from soil enrichments under aerobic and nitrogen-limiting conditions. A strain of Enterobacter cloacae, designated PB2, was isolated from this culture and was found to use PETN as a sole source of nitrogen for growth. Growth yields suggested that 2 to 3 mol of nitrogen was utilized per mol of PETN. The metabolites pentaerythritol dinitrate, 3-hydroxy-2,2-bis-[(nitrooxy)methyl]propanal, and 2,2-bis-[(nitrooxy)methyl]-propanedial were identified by mass spectrometry and 1H-nuclear magnetic resonance. An NADPH-dependent PETN reductase was isolated from cell extracts and shown to liberate nitrite from PETN, producing pentaerythritol tri- and dinitrates which were identified by mass spectrometry. PETN reductase was purified to apparent homogeneity by ion-exchange and affinity chromatography. The purified enzyme was found to be a monomeric flavoprotein with a Mr of approximately 40,000, binding flavin mononucleotide noncovalently.

A resting-cell suspension of A. radiobacter grown on GTN as the nitrogen source metabolized 0.1 mM PETN rapidly, within 1.5 h; this was accompanied by a rapid increase in the concentration of a UV-detectable metabolite (designated M3). M3 was transient, and its disappearance was accompanied by the formation of a second metabolite, M2, which achieved its maximum concentration after 3 h. Thereafter, M2 slowly disappeared, and a third metabolite peak (M1; not shown) was observed in HPLC traces; its elution in the water dip precluded accurate peak integration. Without standard compounds to calibrate the HPLC system, the identities of metabolites M1 to M3 remain uncertain. However, by analogy with the sequential denitration of GTN in this bacterium, it is a reasonable working hypothesis that M3, M2, and M1 are the tri-, di-, and mononitrates of pentaerythritol, respectively.