And YHK participated inside the discussion from the outcomes and writing of your manuscript. All authors read and approved the final manuscript.Fig. six Interaction among A242D and its surrounding residues: a hydrogen bonding and b charge harge interaction. Numbers aligned with arrows indicate the pKa shift effect on A242DAuthor particulars 1 School of Energy and Chemical Engineering, UNIST, 50 UNIST-gil, Ulju-gun, Ulsan 44919, Republic of Korea. 2 Life Ingredient Material Analysis Institute, CJ Enterprise, 42 Gwanggyo-ro, Yeongtong-gu, Suwon-si, Gyeonggi-do, Republic of Korea. Acknowledgements We gratefully acknowledge the MOTIEKEIT (10049675), KCRC (2014M1A8A1049296), KCGRC (2015M3D3A1A01064919), and UNIST Start-Up Grant 2016 for their support of this perform. We also thank Dr. Youn Min Hye (Korea Institute Power Investigation) for help in performing transient kinetics and Dr. Joo Jeong Chan, Oh Joon Young (Korea Research Institute of Chemical Technology) for technical assistance in enzyme purification. Competing interests The authors declare that they’ve no competing interests. Availability of supporting information All information generated or analyzed in the course of this study are included in this published write-up and its additional files. Consent for publication All authors agree to publication. Funding MOTIEKEIT (10049675), KCRC (2014M1A8A1049296), KCGRC (2015M3D3A1A01064919), UNIST Start-Up Grant 2016. Received: 29 September 2016 Diethyl succinate site Accepted: 9 NovemberFig. 7 Proposed multistep tunneling process in LRET among W171 and Heme via W251 and FPham et al. Biotechnol Biofuels (2016) 9:Page 10 ofReferences 1. Tien M, Kirk TK. Lignin-degrading enzyme in the Hymenomycete Phanerochaete chrysosporium Burds. Science. 1983;221:661. two. Fern dez-Fueyo E, Ruiz-Due s FJ, Mart ez MJ, Romero A, Hammel KE, Medrano FJ, Mart ez AT. Ligninolytic peroxidase genes in the oyster mushroom genome CDPPB In Vitro heterologous expression, molecular structure, catalytic and stability properties, and lignin-degrading capability. Biotechnol Biofuels. 2014;7(1):two. 3. Smith AT, Doyle WA, Dorlet P, Ivancich A. Spectroscopic proof for an engineered, catalytically active Trp radical that creates the distinctive reactivity of lignin peroxidase. Proc Natl Acad Sci USA. 2009;106:16084. four. Saez-Jimenez V, Baratto MC, Pogni R, Rencoret J, Gutierrez A, Santos JI, Martinez AT, Ruiz-Duenas FJ. Demonstration of lignin-to-peroxidase direct electron transfer: a transient-state kinetics, directed mutagenesis, EPR and NMR study. J Biol Chem. 2015;290:232013. 5. Semba Y, Ishida M, Yokobori S, Yamagishi A. Ancestral amino acid substitution improves the thermal stability of recombinant lignin-peroxidase from white-rot fungi, Phanerochaete chrysosporium strain UAMH 3641. Protein Eng Des Sel. 2015;28:2210. six. Saez-Jimenez V, Fernandez-Fueyo E, Medrano FJ, Romero A, Martinez AT, Ruiz-Duenas FJ. Improving the pH-stability of versatile peroxidase by comparative structural analysis with a naturally-stable manganese peroxidase. PLoS 1. 2015;10:e0140984. 7. Pham LTM, Eom MH, Kim YH. Inactivating impact of phenolic unit structures on the biodegradation of lignin by lignin peroxidase from Phanerochaete chrysosporium. Enzyme Microb Technol. 2014;612:484. 8. Doyle WA, Smith AT. Expression of lignin peroxidase H8 in Escherichia coli: folding and activation on the recombinant enzyme with Ca2+ and haem. Biochem J. 1996;315:15. 9. Urban A, Neukirchen S, Jaeger KE. A fast and effective method for sitedirected mutagenesis making use of one-step overlap extensio.