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利用基因改良方法提高地衣芽孢杆菌菌株对虾壳的脱蛋白效率,生产高分子质量的壳聚糖。

Genetic improvement of Bacillus licheniformis strains for efficient deproteinization of shrimp shells and production of high-molecular-mass chitin and chitosan.

机构信息

Westfälische Wilhelms-Universität Münster, Institut für Molekulare Mikrobiologie und Biotechnologie, D-48149 Münster, Germany.

出版信息

Appl Environ Microbiol. 2010 Dec;76(24):8211-21. doi: 10.1128/AEM.01404-10. Epub 2010 Oct 22.

DOI:10.1128/AEM.01404-10
PMID:20971870
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3008253/
Abstract

By targeted deletion of the polyglutamate operon (pga) in Bacillus licheniformis F11, a derivative form, F11.1 (Δpga), was obtained that, along with lacking polyglutamate (PGA) formation, displayed enhanced proteolytic activities. The phenotypic properties were maintained in a strain in which the chiBA operon was additionally deleted: F11.4 (ΔchiBA Δpga). These genetically modified strains, carrying the Δpga deletion either alone (F11.1) or together with the ΔchiBA (F11.4) deletion, were used in fermentations (20-liter scale) aiming at the deproteinization of shrimp shells in order to obtain long-chain chitin. After chemical deacetylation, the resulting chitosan samples were analyzed by nuclear magnetic resonance spectroscopy, size exclusion chromatography, and viscometry and compared to a chitosan preparation that was produced in parallel by chemical methods by a commercial chitosan supplier (GSRmbH). Though faint lipid impurities were present in the fermented polysaccharides, the viscosity of the material produced with the double-deletion mutant F11.4 (Δpga ΔchiBA) was higher than that of the chemically produced and commercially available samples (Cognis GmbH). Thus, enhanced proteolytic activities and a lack of chitinase activity render the double mutant F11.4 a powerful tool for the production of long-chain chitosan.

摘要

通过靶向敲除地衣芽孢杆菌 F11 中的多聚谷氨酸操纵子(pga),获得了一个衍生形式,F11.1(Δpga),它不仅缺乏多聚谷氨酸(PGA)的形成,而且显示出增强的蛋白水解活性。在另外缺失 chiBA 操纵子的菌株中保持了这种表型特性:F11.4(ΔchiBA Δpga)。这些经过基因改造的菌株,要么单独携带 Δpga 缺失(F11.1),要么与 ΔchiBA(F11.4)缺失一起,用于发酵(20 升规模),旨在从虾壳中脱蛋白,以获得长链壳聚糖。经过化学脱乙酰化后,用核磁共振波谱、尺寸排阻色谱和粘度计对所得壳聚糖样品进行分析,并与商业壳聚糖供应商(GSRmbH)通过化学方法平行生产的壳聚糖制剂进行比较。尽管发酵多糖中存在微弱的脂质杂质,但具有双重缺失突变体 F11.4(Δpga ΔchiBA)的材料的粘度高于化学生产和市售样品(Cognis GmbH)。因此,增强的蛋白水解活性和缺乏几丁质酶活性使双突变体 F11.4 成为生产长链壳聚糖的有力工具。

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