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Cloned Bacillus subtilis Alkaline Protease (aprA) Gene Showing High Level or Keratinolytic Activity

机译:克隆的枯草芽孢杆菌碱性蛋白酶(aprA)基因显示高水平或角质素分解活性

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The Bacillus subtilis alkaline protease (aprA) gene was previously cloned on a pUB110-derivative plasmid. High levels of expression and gene stability were demonstrated when B. subtilis cells were grown on the laboratory medium 2XSG. B. subtilis cells harboring the multicopy aprA gene were grown on basal medium, supplemented with 1 % chicken feather as a source of energy, carbon, and nitrogen. Proteolytic and kera-tinolytic activities were monitored throughout the cultivation time. A high level of keratinolytic activity was obtained, and this indicates that alkaline protease is acting as a keratinase. Furthermore, considerable amounts of soluble proteins and free amino acids were obtained as a result of the enzymatic hydrolysis of feather. Biodegradation of feather waste using these cells represents an alternative way to improve the nutritional value of feather, since feather waste is currently utilized on a limited basis as a dietary protein supplement for animal feedstuffs. Moreover, the release of free amino acids from feather and the secreted keratinase enzyme would promote industries based on feather waste.
机译:枯草芽孢杆菌碱性蛋白酶(aprA)基因事先克隆在pUB110衍生质粒上。当枯草芽孢杆菌细胞在实验室培养基2XSG上生长时,证明了高水平的表达和基因稳定性。携带多拷贝aprA基因的枯草芽孢杆菌细胞在基础培养基上生长,并补充了1%的鸡毛作为能量,碳和氮的来源。在整个培养过程中监测蛋白水解和角质水解活性。获得了高水平的角蛋白分解活性,这表明碱性蛋白酶起着角蛋白酶的作用。此外,由于羽毛的酶促水解,获得了大量可溶蛋白和游离氨基酸。使用这些细胞对羽毛废料进行生物降解代表了提高羽毛营养价值的另一种方法,因为羽毛废料目前仅在有限的基础上用作动物饲料的膳食蛋白质补充剂。而且,从羽毛和分泌的角蛋白酶释放游离氨基酸将促进基于羽毛废物的工业。

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