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通过单分子显微镜测量 PETase 酶动力学。

Measuring PETase enzyme kinetics by single-molecule microscopy.

机构信息

Department of Biomedical Engineering, Pennsylvania State University, University Park, Pennsylvania.

Department of Biomedical Engineering, Pennsylvania State University, University Park, Pennsylvania; Department of Chemistry, Pennsylvania State University, University Park, Pennsylvania.

出版信息

Biophys J. 2024 Nov 5;123(21):3669-3677. doi: 10.1016/j.bpj.2024.09.016. Epub 2024 Sep 19.

Abstract

Polyethylene terephthalate (PET) is one of the most widely produced man-made polymers and is a significant contributor to microplastics pollution. The environmental and human health impacts of microplastics pollution have motivated a concerted effort to develop microbe- and enzyme-based strategies to degrade PET and similar plastics. A PETase derived from the bacteria Ideonella sakaiensis was previously shown to enzymatically degrade PET, triggering multidisciplinary efforts to improve the robustness and activity of this and other PETases. However, because these enzymes only erode the surface of the insoluble PET substrate, it is difficult to measure standard kinetic parameters, such as k, k, and k, complicating interpretation of the activity of mutants using traditional enzyme kinetics frameworks. To address this challenge, we developed a single-molecule microscopy assay that quantifies the landing rate and binding duration of quantum dot-labeled PETase enzymes interacting with a surface-immobilized PET film. Wild-type PETase binding durations were well fit by a biexponential with a fast population having a 2.7 s time constant, interpreted as active binding events, and a slow population interpreted as nonspecific binding interactions that last tens of seconds. A previously described hyperactive mutant, S238F/W159H had both a faster apparent on-rate and a slower off-rate than wild-type PETase, potentially explaining its enhanced activity. Because this single-molecule approach provides a more detailed mechanistic picture of PETase enzymatic activity than standard bulk assays, it should aid future efforts to engineer more robust and active PETases to combat global microplastics pollution.

摘要

聚对苯二甲酸乙二醇酯(PET)是最广泛生产的人造聚合物之一,也是微塑料污染的主要贡献者。微塑料污染对环境和人类健康的影响促使人们共同努力开发基于微生物和酶的策略来降解 PET 和类似的塑料。先前已经证明,来源于细菌 Ideonella sakaiensis 的 PETase 能够酶促降解 PET,这引发了多学科的努力来提高这种和其他 PETase 的稳健性和活性。然而,由于这些酶只能侵蚀不溶性 PET 基质的表面,因此很难测量标准的动力学参数,如 kcat、Kcat/Km 和 Km,这使得使用传统的酶动力学框架来解释突变体的活性变得复杂。为了解决这个挑战,我们开发了一种单分子显微镜测定法,该方法可量化与表面固定的 PET 膜相互作用的量子点标记的 PETase 酶的着陆率和结合持续时间。野生型 PETase 的结合持续时间很好地符合双指数拟合,其中快速种群的时间常数为 2.7 s,解释为活性结合事件,而慢速种群解释为持续数十秒的非特异性结合相互作用。以前描述的超活性突变体 S238F/W159H 比野生型 PETase 具有更快的表观结合速率和更慢的解离速率,这可能解释了其增强的活性。由于这种单分子方法提供了比标准批量测定法更详细的 PETase 酶活性的机械图,因此它应该有助于未来努力设计更稳健和更活跃的 PETase 来对抗全球微塑料污染。

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