Naqvi Shoa, Moerschbacher Bruno M
a Institute for Biology and Biotechnology of Plants, WWU Münster University , Münster , Germany.
Crit Rev Biotechnol. 2017 Feb;37(1):11-25. doi: 10.3109/07388551.2015.1104289. Epub 2015 Nov 2.
Chitin is one of the most abundant renewable resources, and chitosans, the partially deacetylated derivatives of chitin, are among the most promising functional biopolymers, with superior material properties and versatile biological functionalities. Elucidating molecular structure-function relationships and cellular modes of action of chitosans, however, it is challenging due to the micro-heterogeneity and structural complexity of polysaccharides. Lately, it has become apparent that many of the biological activities of chitosan polymers, such as in agricultural plant disease protection or in mediating scar-free wound healing, may be attributed to oligomeric break-down products generated by the action of chitosanolytic hydrolases present in the target tissues, such as human chitotriosidase. Consequently, the focus of current research is shifting toward chitosan oligomers so that the availability of well-defined chitosan oligosaccharides (COS) becomes a bottleneck. Well-known ways of producing COS use physical and/or chemical means for the partial depolymerization of chitosan polymers, typically leading to broad mixtures of COS varying in their degrees of polymerization (DP) and acetylation (DA), and with more or less random patterns of acetylation (PAs). Even after chromatographic separation according to DP and DA, such mixtures are of limited value to elucidate structure-function relationships and modes of action. More recently, enzymatic means using chitinases and/or chitosanases, and sometimes chitin deacetylases, have been proposed as these can be more tightly controlled and yield slightly better defined mixtures of COS. An alternative would be chemical synthesis of COS which in principle would allow for full structural control, but protocols for it are lengthy, costly, and not yet well developed, and yields are low. Synthetic biology now allows to develop today's in vitro bio-refinery approaches into in vivo cell factory approaches for the biotechnological production of defined COS using recombinant microbial strains expressing chitin oligomer synthases and chitin oligomer deacetylases. In this review, we will describe the state-of-the-art of this cell factory approach, as a basis for upcoming developments. We will briefly describe traditional chemical protocols and enzymatic production of COS as a background to the more detailed presentation of what has been achieved through in vivo biosynthesis. We will only briefly describe those as a background to the more detailed presentation of what has been achieved through in vivo biosynthesis. We will also touch on the production of COS derivatives that has been achieved in this way, as these oligomers open up another plethora of potential applications when used as building blocks for defined biomaterials.
几丁质是最丰富的可再生资源之一,而壳聚糖作为几丁质的部分脱乙酰衍生物,是最具前景的功能性生物聚合物之一,具有优异的材料性能和多样的生物功能。然而,由于多糖的微不均一性和结构复杂性,阐明壳聚糖的分子结构 - 功能关系和细胞作用模式具有挑战性。最近,很明显壳聚糖聚合物的许多生物活性,如在农业植物病害防治或介导无瘢痕伤口愈合中,可能归因于靶组织中存在的壳聚糖分解水解酶(如人几丁质三糖苷酶)作用产生的低聚降解产物。因此,当前的研究重点正转向壳聚糖低聚物,使得获得明确的壳聚糖寡糖(COS)成为一个瓶颈。生产COS的已知方法使用物理和/或化学手段使壳聚糖聚合物部分解聚,通常会产生聚合度(DP)和乙酰化程度(DA)不同且乙酰化模式(PA)或多或少随机的COS广泛混合物。即使根据DP和DA进行色谱分离,这种混合物对于阐明结构 - 功能关系和作用模式的价值也有限。最近,有人提出使用几丁质酶和/或壳聚糖酶,有时还使用几丁质脱乙酰酶的酶促方法,因为这些方法可以得到更严格的控制,并且产生的COS混合物定义更明确。另一种方法是COS的化学合成,原则上这将允许完全的结构控制,但相关方案冗长、成本高且尚未充分发展,产率也低。合成生物学现在允许将当今的体外生物精炼方法发展为体内细胞工厂方法,用于使用表达几丁质低聚物合成酶和几丁质低聚物脱乙酰酶的重组微生物菌株生物技术生产明确的COS。在本综述中,我们将描述这种细胞工厂方法的最新进展,作为未来发展的基础。我们将简要描述传统的化学方案和COS的酶促生产,作为更详细介绍通过体内生物合成所取得成果的背景。我们只会简要描述这些,作为更详细介绍通过体内生物合成所取得成果的背景。我们还将提及以这种方式实现的COS衍生物的生产,因为这些低聚物用作明确生物材料的构建块时会开辟大量潜在应用。
