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一种用于IgA亲和纯化的合成配体。

A synthetic ligand for IgA affinity purification.

作者信息

Palombo G, De Falco S, Tortora M, Cassani G, Fassina G

机构信息

Tecnogen SCpA, Piana di Monte Verna, CE, Italy.

出版信息

J Mol Recognit. 1998 Winter;11(1-6):243-6. doi: 10.1002/(SICI)1099-1352(199812)11:1/6<243::AID-JMR431>3.0.CO;2-#.

Abstract

We reported previously that TG19318, a synthetic ligand deduced from the screening of combinatorial libraries, displays specific and selective recognition properties for immunoglobulins of the G class and can be used conveniently for affinity chromatography purification of monoclonal and polyclonal antibodies. In this study we have extended the ligand characterization, examining its ability to bind IgA from cell culture supernatants and from IgG-deprived serum. Affinity columns prepared by immobilizing TG19318 on Sepharose allowed convenient one-step purification of monoclonal IgA directly from crude feedstocks, in high yield and with full recovery of immunoreactivity. Optimal column adsorption occurred with phosphate buffer at neutral pH, while elution of adsorbed IgA could be accomplished by a buffer pH change to acidic or basic conditions. Column capacity was close to 7 mg IgA/ml support.

摘要

我们之前报道过,TG19318是一种通过组合文库筛选推导出来的合成配体,对G类免疫球蛋白具有特异性和选择性识别特性,可方便地用于单克隆和多克隆抗体的亲和层析纯化。在本研究中,我们扩展了对该配体的表征,研究了其结合细胞培养上清液和去除IgG的血清中IgA的能力。通过将TG19318固定在琼脂糖上制备的亲和柱,能够直接从粗原料中方便地一步纯化单克隆IgA,产量高且免疫反应性完全恢复。在中性pH的磷酸盐缓冲液中柱吸附最佳,而通过将缓冲液pH改变为酸性或碱性条件可实现吸附的IgA的洗脱。柱容量接近7 mg IgA/ml载体。

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