Over the past two decades, various scaffolds have been designed and synthesized to organize enzyme cascades spatially for enhanced enzyme activity based on the concepts of substrate channeling and enhanced stability. The most bio-compatible synthetic scaffolds known for enzyme immobilization are protein and DNA nanostructures. Herein, we examined the utility of the T4 phage capsid to serve as a naturally occurring protein scaffold for the immobilization of a three-enzyme cascade: Amylase, Maltase, and Glucokinase. Covalent constructs between each of the enzymes and the outer capsid protein Hoc were prepared through SpyTag-SpyCatcher pairing and assembled onto phage capsids in vitro with an estimated average of 90 copies per capsid. The capsid-immobilized Maltase has a fourfold higher initial rate relative to Maltase free in solution. Kinetic analysis also revealed that the immobilized three-enzyme cascade has an 18-fold higher converted number of NAD(+) to NADH relative to the mixtures in solution. Our results demonstrate that the T4 phage capsid can act as a naturally occurring scaffold with substantial potential to enhance enzyme activity by spatially organizing enzymes on the capsid Hoc.
Multi-Enzyme Assembly on T4 Phage Scaffold.
在T4噬菌体支架上进行多酶组装
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作者:Liu Jinny L, Zabetakis Daniel, Breger Joyce C, Anderson George P, Goldman Ellen R
| 期刊: | Frontiers in Bioengineering and Biotechnology | 影响因子: | 4.800 |
| 时间: | 2020 | 起止号: | 2020 Jun 24; 8:571 |
| doi: | 10.3389/fbioe.2020.00571 | 研究方向: | 微生物学 |
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