| Literature DB >> 26992786 |
Ankit P Sudhir1, Viplove V Agarwaal1, Bhaumik R Dave1, Darshan H Patel2, R B Subramanian3.
Abstract
L-Asparaginase (3.5.1.1) being antineoplastic in nature are used in the treatment of acute lymphoblastic leukemia (ALL). However glutaminase activity is the cause of various side effects when used as a drug against acute lymphoblastic leukemia (ALL). Therefore, there is a need of a novel L-asparaginase (L-ASNase) with low or no glutaminase activity. Such a property has been observed with L-ASNase from B. licheniformis (BliA). The enzyme being glutaminase free in nature paved the way for its improvement to achieve properties similar to or near to the commercially available L-ASNases. Rational enzyme engineering approach resulted in four mutants: G238N, E232A, D103V and Q112H. Among these the mutant enzyme, D103V, had a specific activity of 597.7IU/mg, which is higher than native (rBliA) (407.65IU/mg). Moreover, when the optimum temperature and in vitro half life were studied and compared with native BliA, D103V mutant BliA was better, showing tolerance to higher temperatures and a 3 fold higher half life. Kinetic studies revealed that the mutant D103V L-ASNase has increased substrate affinity, with Km value of 0.42mM and Vmax of 2778.9μmolmin(-1).Entities:
Keywords: B. licheniformis; Enhanced catalysis; Site directed mutagenesis; l-asparaginase
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Year: 2016 PMID: 26992786 DOI: 10.1016/j.enzmictec.2015.11.010
Source DB: PubMed Journal: Enzyme Microb Technol ISSN: 0141-0229 Impact factor: 3.493