A novel method to clean protein G agarose for affinity column matrix with renewed binding capacity and high IgG selectivity.

Owuor BO; Remarque EJ; Faber BW; Thomas AW

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A novel method to clean protein G agarose for affinity column matrix with renewed binding capacity and high IgG selectivity.

机译：一种具有新的结合能力和高IgG选择性的清洁亲和柱基质蛋白质G琼脂糖的新方法。

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Attempts have been made at finding ways of cleaning used protein G agarose to revive their efficiency and make them reusable for purifying immunoglobulin G (IgG) in affinity column chromatography. A successful cleaning procedure that involved the use of 4-mol/L urea with 0.1-mol/L sodium hydroxide has been previously evaluated although it had some deleterious effect on the column binding capacity and compromised the resin efficiency. Efforts to develop base-tolerant affinity columns by using genetically engineered ligands such as the recombinant protein A from GE Healthcare have achieved some progress, with the column efficiency getting compromised to a lesser extent. However, genetically engineered ligands are even more expensive and may not be readily affordable in modest laboratory settings, especially if large-scale purchases are needed in routine use. We report here a novel and simple cleaning method involving the use of polyethylene glycol (PEG8000) that renews matrix-binding capacity comparable to a new resin while retaining high selectivity for IgG.

机译：已经尝试寻找清洁用过的蛋白G琼脂糖以恢复其效率并使它们可重复使用以在亲和柱色谱中纯化免疫球蛋白G（IgG）的方法。先前曾评估过成功的清洗程序，其中涉及将4-mol / L尿素与0.1-mol / L氢氧化钠一起使用，尽管它对色谱柱的结合能力有一定的有害影响，并损害了树脂的效率。通过使用基因工程配体（例如GE Healthcare的重组蛋白A）开发耐碱亲和柱的努力已取得一些进展，但柱效受到的影响较小。然而，基因工程配体甚至更昂贵，并且在中等实验室条件下可能无法轻易负担得起，尤其是在常规使用中需要大规模购买的情况下。我们在这里报告了一种新颖而简单的清洁方法，其中涉及到使用聚乙二醇（PEG8000），它可以更新与新树脂相当的基质结合能力，同时保留对IgG的高选择性。

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《Journal of Immunological Methods》 |2010年第2期|共3页
作者
Owuor BO; Remarque EJ; Faber BW; Thomas AW;
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中图分类医学免疫学;
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1. A novel method to clean protein G agarose for affinity column matrix with renewed binding capacity and high IgG selectivity. [J] . Owuor BO, Remarque EJ, Faber BW, Journal of Immunological Methods . 2010,第1a2期

机译：一种具有新的结合能力和高IgG选择性的清洁亲和柱基质蛋白质G琼脂糖的新方法。
2. Application of green fluorescent protein to affinity electrophoresis; affinity of IgG-binding domain C from streptococcal protein G to mouse IgG1. [J] . Kazama H, Yamada K, Aoki T, Biological & pharmaceutical bulletin . 2002,第2期

机译：绿色荧光蛋白在亲和电泳中的应用;链球菌蛋白G的IgG结合结构域C对小鼠IgG1的亲和力。
3. A high-capacity column for affinity purification of sequence-specific DNA-binding proteins [J] . Nucleic acids research . 1992,第13期

机译：高容量色谱柱，用于亲和纯化序列特异性DNA结合蛋白
4. Increase in IgG-binding Capacity of Recombinant Protein a Immobilized on Heterofunctional Amino and Epoxy Agarose [C] . Xufeng Zhang, Ya Duan, Nanyu Han Annual International Workshop on Materials Science and Engineering . 2018

机译：增加重组蛋白A固定在异官能氨基和环氧琼脂糖上的IgG结合能力
5. Towards the prediction of protein-ligand binding affinities: A new class of methods for free energy calculations. [D] . Luo, Rui. 1998

机译：迈向蛋白质-配体结合亲和力的预测：一类用于自由能计算的新方法。
6. A high-capacity column for affinity purification of sequence-specific DNA-binding proteins. [O] . C J Larson, G L Verdine 1992

机译：用于亲和纯化序列特异性DNA结合蛋白的大容量色谱柱。
7. A high-capacity column for affinity purification of sequence-specific DNA-binding proteins. [O] . Larson, C J, Verdine, G L 1992

机译：用于亲和纯化序列特异性DNA结合蛋白的大容量色谱柱。
8. Adsorbent with Enhanced Protein Binding Capacity and Selectivity. [R] . Willson, R. C., Balan, S., Potty, A. S. H. 2005

机译：具有增强的蛋白质结合能力和选择性的吸附剂。

A novel method to clean protein G agarose for affinity column matrix with renewed binding capacity and high IgG selectivity.

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