Loschmidt Laboratories, Department of Experimental Biology and RECETOX, Masaryk University, Brno, Czech Republic.
International Clinical Research Center, St. Anne's Universty Hospital, Brno, Czech Republic.
Appl Environ Microbiol. 2020 Aug 18;86(17). doi: 10.1128/AEM.02820-19.
Haloalkane dehalogenases can cleave a carbon-halogen bond in a broad range of halogenated aliphatic compounds. However, a highly conserved catalytic pentad composed of a nucleophile, a catalytic base, a catalytic acid, and two halide-stabilizing residues is required for their catalytic activity. Only a few family members, e.g., DsaA, DmxA, or DmrB, remain catalytically active while employing a single halide-stabilizing residue. Here, we describe a novel haloalkane dehalogenase, DsvA, from a mildly thermophilic bacterium, strain DSM 43017, possessing one canonical halide-stabilizing tryptophan (W125). At the position of the second halide-stabilizing residue, DsvA contains the phenylalanine F165, which cannot stabilize the halogen anion released during the enzymatic reaction by a hydrogen bond. Based on the sequence and structural alignments, we identified a putative second halide-stabilizing tryptophan (W162) located on the same α-helix as F165, but on the opposite side of the active site. The potential involvement of this residue in DsvA catalysis was investigated by the construction and biochemical characterization of the three variants, DsvA01 (F165W), DsvA02 (W162F), and DsvA03 (W162F and F165W). Interestingly, DsvA exhibits a preference for the ()- over the ()-enantiomers of β-bromoalkanes, which has not been reported before for any characterized haloalkane dehalogenase. Moreover, DsvA shows remarkable operational stability at elevated temperatures. The present study illustrates that protein sequences possessing an unconventional composition of catalytic residues represent a valuable source of novel biocatalysts. The present study describes a novel haloalkane dehalogenase, DsvA, originating from a mildly thermophilic bacterium, strain DSM 43017. We report its high thermostability, remarkable operational stability at high temperatures, and an ()-enantiopreference, which makes this enzyme an attractive biocatalyst for practical applications. Sequence analysis revealed that DsvA possesses an unusual composition of halide-stabilizing tryptophan residues in its active site. We constructed and biochemically characterized two single point mutants and one double point mutant and identified the noncanonical halide-stabilizing residue. Our study underlines the importance of searching for noncanonical catalytic residues in protein sequences.
卤代烷烃脱卤酶能够在广泛的卤代脂肪族化合物中切割碳-卤键。然而,它们的催化活性需要一个高度保守的催化五肽,由亲核试剂、催化碱、催化酸和两个卤化物稳定残基组成。只有少数家族成员,如 DsaA、DmxA 或 DmrB,在仅使用一个卤化物稳定残基的情况下仍然具有催化活性。在这里,我们描述了一种来自中度嗜热细菌 菌株 DSM 43017 的新型卤代烷烃脱卤酶 DsvA,它具有一个典型的卤化物稳定色氨酸(W125)。在第二个卤化物稳定残基的位置,DsvA 含有苯丙氨酸 F165,它不能通过氢键稳定酶促反应中释放的卤素阴离子。基于序列和结构比对,我们在同一α-螺旋上鉴定出一个假定的第二个卤化物稳定色氨酸(W162),但位于活性位点的相反侧。通过构建和生化表征三种变体 DsvA01(F165W)、DsvA02(W162F)和 DsvA03(W162F 和 F165W),研究了该残基在 DsvA 催化中的潜在作用。有趣的是,DsvA 对 β-溴代烷烃的()-对映体表现出偏好,这在以前任何一种表征的卤代烷烃脱卤酶中都没有报道过。此外,DsvA 在高温下表现出显著的操作稳定性。本研究表明,具有非常规催化残基组成的蛋白质序列是新型生物催化剂的宝贵来源。本研究描述了一种新型卤代烷烃脱卤酶 DsvA,它源自中度嗜热细菌 菌株 DSM 43017。我们报告了它的高热稳定性、在高温下的显著操作稳定性和()-对映体偏好,这使该酶成为有吸引力的实用生物催化剂。序列分析表明,DsvA 在其活性位点具有不寻常的卤化物稳定色氨酸残基组成。我们构建并生化表征了两个单点突变体和一个双点突变体,并鉴定了非典型的卤化物稳定残基。我们的研究强调了在蛋白质序列中寻找非典型催化残基的重要性。
