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重组乳酸乳球菌无法分泌牛凝乳酶。

Recombinant Lactococcus lactis fails to secrete bovine chymosine.

作者信息

Luerce Tessália Diniz, Azevedo Marcela Santiago Pacheco, LeBlanc Jean Guy, Azevedo Vasco, Miyoshi Anderson, Pontes Daniela Santos

机构信息

a Department of General Biology; Institute of Biological Sciences ; Federal University of Minas Gerais (UFMG-ICB) ; Belo Horizonte , Brazil.

出版信息

Bioengineered. 2014;5(6):363-70. doi: 10.4161/bioe.36327.

Abstract

Bovine chymosin is an important milk-clotting agent used in the manufacturing of cheeses. Currently, the production of recombinant proteins by genetically modified organisms is widespread, leading to greatly reduced costs. Lactococcus (L.) lactis, the model lactic acid bacterium, was considered a good candidate for heterologous chymosin production for the following reasons: (1) it is considered to be a GRAS (generally regarded as safe) microorganism, (2) only one protease is present on its surface, (3) it can secrete proteins of different sizes, and (4) it allows for the direct production of protein in fermented food products. Thus, three genetically modified L. lactis strains were constructed to produce and target the three different forms of bovine chymosin, prochymosin B, chymosin A and chymosin B to the extracellular medium. Although all three proteins were stably produced in L. lactis, none of the forms were detected in the extracellular medium or showed clotting activity in milk. Our hypothesis is that this secretion deficiency and lack of clotting activity can be explained by the recombinant protein being attached to the cell envelope. Thus, the development of other strategies is necessary to achieve both production and targeting of chymosin in L. lactis, which could facilitate the downstream processing and recovery of this industrially important protein.

摘要

牛凝乳酶是用于奶酪制造的一种重要的凝乳剂。目前,通过转基因生物生产重组蛋白的方式已广泛应用,使得成本大幅降低。乳酸乳球菌作为典型的乳酸菌,因其以下原因被认为是异源生产凝乳酶的良好候选菌株:(1)它被认为是一种公认安全的微生物;(2)其表面仅存在一种蛋白酶;(3)它能够分泌不同大小的蛋白质;(4)它允许在发酵食品中直接生产蛋白质。因此,构建了三种转基因乳酸乳球菌菌株,用于生产牛凝乳酶的三种不同形式,即前凝乳酶B、凝乳酶A和凝乳酶B,并将它们靶向分泌到细胞外培养基中。尽管所有这三种蛋白质都在乳酸乳球菌中稳定产生,但在细胞外培养基中均未检测到任何一种形式,且它们在牛奶中也未表现出凝乳活性。我们的假设是,这种分泌缺陷和缺乏凝乳活性可以通过重组蛋白附着在细胞膜上来解释。因此,有必要开发其他策略来实现乳酸乳球菌中凝乳酶的生产和靶向分泌,这将有助于这种具有重要工业价值的蛋白质的下游加工和回收。

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