首页> 外文期刊>Journal of microbiology and biotechnology >Isolation, Cloning and Co-Expression of Lipase and Foldase Genes of Burkholderia territorii GP3 from Mount Papandayan Soil
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Isolation, Cloning and Co-Expression of Lipase and Foldase Genes of Burkholderia territorii GP3 from Mount Papandayan Soil

机译:巴布尼亚山土丘脑脂肪酶GP3的脂肪酶和脂肪酶基因的分离,克隆和共表达

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摘要

Lipases are industrial enzymes that catalyze both triglyceride hydrolysis and ester synthesis. The overexpression of lipase genes is considered one of the best approaches to increase the enzymatic production for industrial applications. Subfamily I.2. lipases require a chaperone or foldase in order to become a fully-activated enzyme. The goal of this research was to isolate, clone, and co-express genes that encode lipase and foldase from Burkholderia territorii GP3, a lipolytic bacterial isolate obtained from Mount Papandayan soil via growth on Soil Extract Rhodamine Agar. Genes that encode for lipase (lipBT) and foldase (lifBT) were successfully cloned from this isolate and co-expressed in the E. coli BL21 background. The highest expression was shown in E. coli BL21 (DE3) pLysS, using pET15b expression vector. LipBT was particulary unique as it showed highest activity with optimum temperature of 80 degrees C at pH 11.0. The optimum substrate for enzyme activity was C-10, which is highly stable in methanol solvent. The enzyme was strongly activated by Ca2+, Mg2+, and strongly inhibited by Fe2+ and Zn2+. In addition, the enzyme was stable and compatible in non-ionic surfactant, and was strongly incompatible in ionic surfactant.
机译:脂肪酶是催化甘油三酯水解和酯合成的工业酶。脂肪酶基因的过表达被认为是增加工业应用酶促生产的最佳方法之一。亚家族I.2。脂肪酶需要伴侣或重叠,以成为完全活化的酶。该研究的目标是分离,克隆和共同表达基因编码缅因力李克希尔菌GP3的脂肪酶和复合酶,通过土壤提取物罗丹明琼脂的生长从粉孢盐山土壤中获得的脂肪溶解细菌分离物。从该分离物中成功地克隆了编码用于脂肪酶(LIPBT)和重组(LIVBT)的基因,并在大肠杆菌BL21背景中共同表达。使用PET15B表达载体,在大肠杆菌BL21(DE3)帘布层中显示了最高表达。 LIMBT是颗粒状独特的,因为它在pH 11.0下显示出最佳温度为80℃的最高活性。用于酶活性的最佳基质是C-10,其在甲醇溶剂中是高度稳定的。通过Ca2 +,Mg 2 +强烈地激活酶,并受到Fe2 +和Zn2 +的强烈抑制。此外,酶在非离子表面活性剂中稳定并相容,并且在离子表面活性剂中强烈不相容。

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