Graduate Program of Biotechnology and Environmental Monitoring, Federal University of São Carlos (UFSCar), Rodovia João Leme dos Santos, km 110, Itinga, Sorocaba, SP, Brazil.
Biochemistry. 2013 Jun 11;52(23):3963-73. doi: 10.1021/bi400141u. Epub 2013 May 30.
The origin of luciferases and of bioluminescence is enigmatic. In beetles, luciferases seem to have evolved from AMP-CoA-ligases. How the new oxygenase luminogenic function originated from AMP-ligases leading to luciferases is one of the most challenging mysteries of bioluminescence. Comparison of the cloned luciferase-like enzyme from the nonluminescent Zophobas morio mealworm and beetle luciferases showed that the oxygenase activity may have emerged as a stereoselective oxidative drift with d-luciferin, a substrate that cannot be easily thioesterified to CoA as in the case of the l-isomer. While the overall kcat displayed by beetle luciferases is orders of magnitude greater than that of the luciferase-like enzyme, the respective oxidation rates and quantum yields of bioluminescence are roughly similar, suggesting that the rate constant of the AMP-ligase activity exerted on the new d-luciferin substrate in beetle protoluciferases was the main enzymatic property that suffered optimization during the evolution of luciferases. The luciferase-like enzyme and luciferases boost the rate of luciferyl-adenylate chemiluminescent oxidation by factors of 10(6) and 10(7), respectively, as compared to the substrate spontaneous oxidation in buffer. A similar enhancement of luciferyl-adenylate chemiluminescence is provided by nucleophilic aprotic solvents, implying that the peptide bonds in the luciferin binding site of beetle luciferase could provide a similar catalytically favorable environment. These data suggest that the luciferase-like enzyme and other similar AMP-ligases are potential alternative oxygenases. Site-directed mutagenesis studies of the luciferase-like enzyme and the red light-producing luciferase of Phrixotrix hirtus railroadworm confirm here a critical role for T/S345 in luciferase function. Mutations such as I327T/S in the luciferase-like enzyme, which simultaneously increases luciferase activity and promotes blue shifts in the emission spectrum, could have been critical for evolving functional bioluminescence from red-emitting protoluciferases. Through the combination of I327T/S mutations and N-terminal fusion, the luminescence activity of this enzyme was increased to visible levels, with the development of a totally new orange-emitting luciferase. These results open the possibility of engineering luciferase activity in a set of AMP-CoA-ligases.
荧光素酶和生物发光的起源是一个谜。在甲虫中,荧光素酶似乎是从 AMP-CoA 连接酶进化而来的。新的加氧酶发光功能是如何从 AMP 连接酶产生导致荧光素酶的,这是生物发光最具挑战性的奥秘之一。从非发光的 Zophobas morio 黄粉虫和甲虫荧光素酶中克隆的类似荧光素酶的比较表明,加氧酶活性可能是一种立体选择性的氧化漂移,与 d-荧光素不同,d-荧光素不能像 l-异构体那样容易硫酯化到 CoA。虽然甲虫荧光素酶的总 kcat 显示出数量级的差异,但各自的氧化速率和生物发光量子产率大致相似,这表明在甲虫原荧光素酶中,对新 d-荧光素底物的 AMP 连接酶活性的速率常数是在荧光素酶进化过程中主要优化的酶学特性。与缓冲液中底物的自发氧化相比,类似荧光素酶和荧光素酶分别将 luciferyl-adenylate 化学发光氧化的速率提高了 10(6)和 10(7)倍。亲核非质子溶剂提供了类似的 luciferyl-adenylate 化学发光增强,这表明甲虫荧光素酶中荧光素结合位点的肽键可以提供类似的催化有利环境。这些数据表明,类似荧光素酶和其他类似的 AMP 连接酶可能是潜在的替代加氧酶。对类似荧光素酶和 Phrixotrix hirtus 铁路虫红光产生荧光素酶的定点突变研究在这里证实了 T/S345 在荧光素酶功能中的关键作用。类似荧光素酶中的 I327T/S 等突变同时提高了荧光素酶的活性,并促进了发射光谱的蓝移,这对于从红色发射原荧光素酶进化出功能性生物发光可能是至关重要的。通过 I327T/S 突变和 N 端融合的组合,该酶的发光活性增加到可见水平,产生了一种全新的橙色发光荧光素酶。这些结果为在一组 AMP-CoA 连接酶中设计荧光素酶活性提供了可能性。
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