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在大肠杆菌中过表达来自苋菜种子的改良蛋白及其表达受环境条件的影响。

Overexpression of a modified protein from amaranth seed in Escherichia coli and effect of environmental conditions on the protein expression.

机构信息

Centro de Investigación para el Desarrollo Integral Regional, CIDIIR-IPN, Sinaloa, Mexico.

出版信息

J Biotechnol. 2012 Mar 31;158(1-2):59-67. doi: 10.1016/j.jbiotec.2011.12.012. Epub 2012 Jan 9.

Abstract

Amaranth seeds are considered as an excellent complementary source of food protein due to their balanced amino acid composition. Amarantin acidic subunit has the potential as a functional and nutraceutical protein, and it is structurally a good candidate for modification. The aim of this work was to improve its functionality, then the primary structure was modified into the third variable region of 11S globulins, by inserting antihypertensive peptides: four Val-Tyr in tandem and Arg-Ile-Pro-Pro in the C-terminal region. Modified protein was expressed in Escherichia coli Origami (DE3) and was purified. The culture conditions, including the culture media, temperature, agitation speed and air flow were tested in order to obtain an increased expression levels of the modified protein. A 2(3) factorial design was used for evaluate the effect of environmental conditions on modified protein production. The results indicated that the yield of modified protein could be increased by up 3-fold in bioreactor as compared with flask. In addition, the temperature, the agitation speed and the oxygen were significant factors on the expression of the antihypertensive protein. The maximum production was 99 mg protein-L(-1). The hydrolyzed protein showed a high inhibitory activity of the angiotensin converting enzyme (IC50=0.047 mg mL(-1)).

摘要

苋菜种子因其氨基酸组成平衡而被认为是一种极好的食物蛋白质补充来源。苋菜酸性亚基具有作为功能性和营养蛋白的潜力,并且在结构上是修饰的良好候选物。本工作的目的是改善其功能,然后将一级结构修饰成 11S 球蛋白的第三个可变区,通过插入具有降压作用的肽:四个缬氨酸-酪氨酸串联和精氨酸-异亮氨酸-脯氨酸-脯氨酸在 C 末端区域。修饰后的蛋白质在大肠杆菌 Origami(DE3)中表达并进行了纯化。为了获得修饰蛋白的表达水平提高,测试了包括培养基、温度、搅拌速度和空气流量在内的培养条件。采用 2(3) 因子设计来评估环境条件对修饰蛋白生产的影响。结果表明,与摇瓶相比,在生物反应器中修饰蛋白的产率可提高 3 倍。此外,温度、搅拌速度和氧气是影响降压蛋白表达的重要因素。最大产量为 99mg 蛋白·L(-1)。水解蛋白对血管紧张素转化酶(IC50=0.047mg·mL(-1))具有很高的抑制活性。

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