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从免疫吸附剂释放的抗体:载体、活化及洗脱条件的影响

Antibodies released from immunoadsorbents: effect of support, activation and elution conditions.

作者信息

Ubrich N, Rivat C

机构信息

Centre de Recherche INSERM, CHU de Brabois, Vandoeuvre-les-Nancy, France.

出版信息

Artif Cells Blood Substit Immobil Biotechnol. 1996 Jan;24(1):65-75. doi: 10.3109/10731199609117432.

Abstract

Immunoadsorption is an application of affinity chromatography, as a therapeutic method to specifically deplete biological fluids such as blood plasma from proteins in excess, or to extract a biomolecule from a complex mixture. However, the leakage of small amounts of antibodies covalently immobilized on the support hampers the practical use of this method. In fact, these released antibodies contaminate the purified proteins or depleted media and, when they are of animal nature, they may lead to immunization of patients, or cause an anaphylactic shock when a clinical use is concerned. It is therefore of prime importance that the immunoadsorbents exhibit a satisfactory stability over the whole range of chemical and biochemical conditions involved during their clinical handling. To determine optimal conditions for the preparation of stable immunoadsorbents designed to remove selectively Low Density Lipoproteins (LDLs) from the plasma of patients affected by familial hypercholesterolemia, various immunoadsorbents were prepared by covalent immobilization of goat anti-apolipoprotein B polyclonal antibodies on different supports (Sepharose CL-4B, Sepharose 6 Fast Flow, Sphérodex and Fractogel) previously activated by various chemical reagents (cyanogen bromide, divinyl sulphone, tresyl chloride and trichloro-s-triazine). Their adsorption capacity, specificity, stability and the amount of immobilized antibodies were compared in terms of the activation method and the support used. It turns out that the immunoadsorbents prepared with Sepharose 6 Fast Flow lead to optimal yield of coupling, adsorption capacity, and an excellent stability at neutral pH. TC-activated-Fractogel turns out as well to afford an excellent coupling yield, a good adsorption capacity and an optimal stability in the whole pH range tested.

摘要

免疫吸附是亲和色谱的一种应用,作为一种治疗方法,可特异性去除生物流体(如血浆)中过量的蛋白质,或从复杂混合物中提取生物分子。然而,共价固定在载体上的少量抗体泄漏阻碍了该方法的实际应用。事实上,这些释放的抗体污染了纯化的蛋白质或耗尽的介质,并且当它们是动物源性时,可能导致患者免疫,或在临床使用时引起过敏反应。因此,至关重要的是,免疫吸附剂在其临床处理过程中涉及的整个化学和生化条件范围内表现出令人满意的稳定性。为了确定制备用于从家族性高胆固醇血症患者血浆中选择性去除低密度脂蛋白(LDL)的稳定免疫吸附剂的最佳条件,通过将山羊抗载脂蛋白B多克隆抗体共价固定在先前用各种化学试剂(溴化氰、二乙烯砜、甲苯磺酰氯和三氯-s-三嗪)活化的不同载体(琼脂糖CL-4B、琼脂糖6快速流动、Sphérodex和Fractogel)上制备了各种免疫吸附剂。根据活化方法和所用载体比较了它们的吸附容量、特异性、稳定性和固定化抗体的量。结果表明,用琼脂糖6快速流动制备的免疫吸附剂导致最佳的偶联产率、吸附容量,并且在中性pH下具有优异的稳定性。TC活化的Fractogel也显示出优异的偶联产率、良好的吸附容量和在整个测试pH范围内的最佳稳定性。

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