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Updated protocols for the detection of Sotatercept and Luspatercept in human serum

机译:更新了人类血清Sotatercept和Luspatercept的检测的协议

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We recently published two protocols for the detection of Sotatercept (ACE-011, ACVR2A-Fc) and Luspatercept (ACE-536, ACVR2B-Fc) in human serum. Both methods used covalently immobilized antibodies on agarose beads for immunoprecipitation and SAR-PAGE/Western blotting for detection. Disadvantages were the relatively high amount of antibody required per sample (10 mu g) and the need of a secondary antibody for the final detection. The updated protocols overcome these limitations by antigen-antibody complex formation in solution followed by capture of the complex with anti-antibody-coated magnetic beads. They also omit the secondary antibody incubation step by usage of biotinylated primary antibodies, which can be directly incubated with streptavidin-HRP. Thus, the new protocols are faster, simpler, and cheaper and offer comparable sensitivities.
机译:我们最近公布了两种用于检测人血清中的Sotatercept(ACE-011,ACVR2A-FC)和Luspatercept(ACE-536,ACVR2B-Fc)的两种协议。 两种方法使用共价固定的抗体对琼脂糖珠的免疫沉淀和SAR-PAGE / Western印迹进行检测。 缺点是每个样品(10μg)所需的抗体量的相对大量的抗体以及用于最终检测的二抗的需要。 更新的方案通过溶液中的抗原 - 抗体复合物形成克服了这些限制,然后用抗抗体涂覆的磁珠捕获复合物。 它们还通过使用生物素化的原发性抗体省略二次抗体孵育步骤,其可以直接与链霉抗生物素蛋白-HRP温育。 因此,新协议更快,更简单,更便宜,并提供可比的敏感性。

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