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分枝杆菌在链霉菌中 O-甘露糖基化和重组 APA(45/47 kDa)蛋白的产生受摇瓶培养条件的影响。

The O-mannosylation and production of recombinant APA (45/47 KDa) protein from Mycobacterium tuberculosis in Streptomyces lividans is affected by culture conditions in shake flasks.

机构信息

Unidad de Bioprocesos, Instituto de Investigaciones Biomédicas, Universidad Nacional Autónoma de México, AP, 70228, México, D,F,, CP, 04510, México.

出版信息

Microb Cell Fact. 2011 Dec 20;10:110. doi: 10.1186/1475-2859-10-110.

Abstract

BACKGROUND

The Ala-Pro-rich O-glycoprotein known as the 45/47 kDa or APA antigen from Mycobacterium tuberculosis is an immunodominant adhesin restricted to mycobacterium genus and has been proposed as an alternative candidate to generate a new vaccine against tuberculosis or for diagnosis kits. In this work, the recombinant O-glycoprotein APA was produced by the non-pathogenic filamentous bacteria Streptomyces lividans, evaluating three different culture conditions. This strain is known for its ability to produce heterologous proteins in a shorter time compared to M. tuberculosis.

RESULTS

Three different shake flask geometries were used to provide different shear and oxygenation conditions; and the impact of those conditions on the morphology of S. lividans and the production of rAPA was characterized and evaluated. Small unbranched free filaments and mycelial clumps were found in baffled and coiled shake flasks, but one order of magnitude larger pellets were found in conventional shake flasks. The production of rAPA is around 3 times higher in small mycelia than in larger pellets, most probably due to difficulties in mass transfer inside pellets. Moreover, there are four putative sites of O-mannosylation in native APA, one of which is located at the carboxy-terminal region. The carbohydrate composition of this site was determined for rAPA by mass spectrometry analysis, and was found to contain different glycoforms depending on culture conditions. Up to two mannoses residues were found in cultures carried out in conventional shake flasks, and up to five mannoses residues were determined in coiled and baffled shake flasks.

CONCLUSIONS

The shear and/or oxygenation parameters determine the bacterial morphology, the productivity, and the O-mannosylation of rAPA in S. lividans. As demonstrated here, culture conditions have to be carefully controlled in order to obtain recombinant O-glycosylated proteins with similar "quality" in bacteria, particularly, if the protein activity depends on the glycosylation pattern. Furthermore, it will be an interesting exercise to determine the effect of shear and oxygen in shake flasks, to obtain evidences that may be useful in scaling-up these processes to bioreactors. Another approach will be using lab-scale bioreactors under well-controlled conditions, and study the impact of those on rAPA productivity and quality.

摘要

背景

结核分枝杆菌中富含丙氨酸-脯氨酸的 O-糖蛋白,即 45/47kDa 或 APA 抗原,是一种免疫优势黏附素,仅限于分枝杆菌属,已被提议作为一种替代候选物,用于开发新的结核病疫苗或诊断试剂盒。在这项工作中,通过非致病性丝状细菌链霉菌生产了重组 O-糖蛋白 APA,并评估了三种不同的培养条件。与结核分枝杆菌相比,该菌株以更短的时间生产异源蛋白而闻名。

结果

使用三种不同的摇瓶几何形状提供不同的剪切和供氧条件;并对这些条件对链霉菌形态和 rAPA 生产的影响进行了表征和评估。在有挡板和螺旋的摇瓶中发现了小的无分支游离丝和菌丝团,但在常规摇瓶中发现了一个数量级更大的颗粒。rAPA 的产量在小菌丝中比在大颗粒中高约 3 倍,这很可能是由于颗粒内部的传质困难所致。此外,天然 APA 中有四个假定的 O-甘露糖基化位点,其中一个位于羧基末端区域。通过质谱分析确定了该位点的碳水化合物组成,结果表明,rAPA 的糖型因培养条件而异。在常规摇瓶中培养时,发现有两个甘露糖残基,而在螺旋和有挡板的摇瓶中培养时,发现有五个甘露糖残基。

结论

剪切和/或供氧参数决定了链霉菌的形态、rAPA 的生产力和 O-甘露糖基化。正如这里所证明的,为了在细菌中获得具有相似“质量”的重组 O-糖基化蛋白,必须仔细控制培养条件,特别是如果蛋白质的活性取决于糖基化模式。此外,在摇瓶中获得剪切和供氧的影响的证据将是一项有趣的练习,这些证据可能对扩大这些过程到生物反应器有用。另一种方法是在可控条件下使用实验室规模的生物反应器,并研究这些条件对 rAPA 生产力和质量的影响。

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