Max Planck Institute for Dynamics of Complex Technical Systems, Bioprocess Engineering, Magdeburg, Germany.
Martin Luther University Halle-Wittenberg, Institute of Pharmacy, Department of Downstream Processing, Halle (Saale), Germany.
J Biotechnol. 2018 Oct 10;283:120-129. doi: 10.1016/j.jbiotec.2018.07.027. Epub 2018 Jul 22.
In spite of huge endeavors in cell line engineering to produce glycoproteins with desired and uniform glycoforms, it is still not possible in vivo. Alternatively, in vitro glycoengineering can be used for the modification of glycans. However, in vitro glycoengineering relies on expensive nucleotide sugars, such as uridine 5'-diphospho-N-acetylglucosamine (UDP-GlcNAc) which serves as GlcNAc donor for the synthesis of various glycans. In this work, we present a systematic study for the cell-free de novo synthesis and regeneration of UDP-GlcNAc from polyphosphate, UMP and GlcNAc by a cascade of five enzymes (N-acetylhexosamine kinase (NahK), Glc-1P uridyltransferase (GalU), uridine monophosphate kinase (URA6), polyphosphate kinase (PPK3), and inorganic diphosphatase (PmPpA). All enzymes were expressed in E. coli BL21 Gold (DE3) and purified using immobilized metal affinity chromatography (IMAC). Results from one-pot experiments demonstrate the successful production of UDP-GlcNAc with a yield approaching 100%. The highest volumetric productivity of the cascade was about 0.81 g L h of UDP-GlcNAc. A simple model based on mass action kinetics was sufficient to capture the dynamic behavior of the multienzyme pathway. Moreover, a design equation based on metabolic control analysis was established to investigate the effect of enzyme concentration on the UDP-GlcNAc flux and to demonstrate that the flux of UDP-GlcNAc can be controlled by means of the enzyme concentrations. The effect of temperature on the UDP-GlcNAc flux followed an Arrhenius equation and the optimal co-factor concentration (Mg) for high UDP-GlcNAc synthesis rates depended on the working temperature. In conclusion, the study covers the entire engineering process of a multienzyme cascade, i.e. pathway design, enzyme expression, enzyme purification, reaction kinetics and investigation of the influence of basic parameters (temperature, co-factor concentration, enzyme concentration) on the synthesis rate. Thus, the study lays the foundation for future cascade optimization, preparative scale UDP-GlcNAc synthesis and for in situ coupling of the network with UDP-GlcNAc transferases to efficiently regenerate UDP-GlcNAc. Hence, this study provides a further step towards cost-effective in vitro glycoengineering of antibodies and other glycosylated proteins.
尽管在细胞系工程方面做出了巨大努力,以生产具有所需和均匀糖型的糖蛋白,但在体内仍然无法实现。或者,可以使用体外糖基工程来修饰聚糖。然而,体外糖基工程依赖于昂贵的核苷酸糖,例如尿苷 5'-二磷酸-N-乙酰氨基葡萄糖(UDP-GlcNAc),它是合成各种聚糖的 GlcNAc 供体。在这项工作中,我们通过一系列五种酶(N-乙酰己糖胺激酶(NahK)、Glc-1P 尿苷酰转移酶(GalU)、尿苷单磷酸激酶(URA6)、多磷酸激酶(PPK3)和无机二磷酸酶(PmPpA))从多磷酸盐、UMP 和 GlcNAc 中进行无细胞从头合成和 UDP-GlcNAc 的再生进行了系统研究。所有酶均在 E. coli BL21 Gold(DE3)中表达,并使用固定化金属亲和层析(IMAC)进行纯化。一锅法实验的结果表明 UDP-GlcNAc 的产量接近 100%。级联的最高比体积产率约为 0.81g L-1 h-1 UDP-GlcNAc。基于质量作用动力学的简单模型足以捕获多酶途径的动态行为。此外,建立了基于代谢控制分析的设计方程,以研究酶浓度对 UDP-GlcNAc 通量的影响,并证明可以通过酶浓度来控制 UDP-GlcNAc 的通量。UDP-GlcNAc 通量对温度的影响遵循阿仑尼乌斯方程,高 UDP-GlcNAc 合成速率的最佳辅酶浓度(Mg)取决于工作温度。总之,该研究涵盖了多酶级联的整个工程过程,即途径设计、酶表达、酶纯化、反应动力学以及基本参数(温度、辅酶浓度、酶浓度)对合成速率的影响的研究。因此,该研究为未来的级联优化、制备规模 UDP-GlcNAc 合成以及与 UDP-GlcNAc 转移酶的原位偶联奠定了基础,以有效再生 UDP-GlcNAc。因此,这项研究朝着具有成本效益的抗体和其他糖基化蛋白的体外糖基工程又迈进了一步。
