Directed evolution of enzymatic silicon-carbon bond cleavage in siloxanes.
Nicholas S SaraiTyler J FultonRyen L O'MearaKadina E JohnstonSabine Brinkmann-ChenRyan R MaarRon E TecklenburgJohn M RobertsJordan C T ReddelDimitris E KatsoulisFrances H ArnoldPublished in: Science (New York, N.Y.) (2024)
Volatile methylsiloxanes (VMS) are man-made, nonbiodegradable chemicals produced at a megaton-per-year scale, which leads to concern over their potential for environmental persistence, long-range transport, and bioaccumulation. We used directed evolution to engineer a variant of bacterial cytochrome P450 BM3 to break silicon-carbon bonds in linear and cyclic VMS. To accomplish silicon-carbon bond cleavage, the enzyme catalyzes two tandem oxidations of a siloxane methyl group, which is followed by putative [1,2]-Brook rearrangement and hydrolysis. Discovery of this so-called siloxane oxidase opens possibilities for the eventual biodegradation of VMS.