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A purification method for a molecular complex in which a scaffold molecule is fully loaded with heterogeneous molecules.

机译:一种分子复合物的纯化方法,其中支架分子中充满了异质分子。

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摘要

An affinity resin-based pull-down method is convenient for the purification of biochemical materials. However, its use is difficult for the isolation of a molecular complex fully loaded with multiple components from a reaction mixture containing the starting materials and intermediate products. To overcome this problem, we have developed a new purification procedure that depends on sequential elimination of the residues. In practice, two affinity resins were used for purifying a triangular-shaped RNP (RNA-protein complex) consisting of three ribosomal proteins (L7Ae) bound to an RNA scaffold. First, a resin with immobilized L7Ae protein captured the incomplete RNP complexes and the free RNA scaffold. Next, another resin with an immobilized chemically modified RNA of a derivative of Box C/D motif, the binding partner of L7Ae, was used to capture free protein. The complete triangular RNP was successfully purified from the mixture by these two steps. Obviously, the purified triangular RNP displaying three protein-binding peptides exhibited an improved performance when compared with the unrefined product. Conceptually, this purification procedure should be applicable for the purification of a variety of complexes consisting of multiple components other than RNP.
机译:基于亲和树脂的下拉法方便于生化材料的纯化。但是,很难从含有起始原料和中间产物的反应混合物中分离出满载有多种组分的分子复合物。为了克服这个问题,我们开发了一种新的纯化程序,该程序依赖于残留物的顺序消除。在实践中,两种亲和树脂用于纯化三角形RNP(RNA-蛋白质复合物),该RNP由结合到RNA支架上的三种核糖体蛋白质(L7Ae)组成。首先,具有固定L7Ae蛋白的树脂捕获了不完整的RNP复合物和游离的RNA支架。接下来,另一种树脂具有固定的Box C / D基序衍生物(L7Ae的结合伴侣)的化学修饰RNA,用于捕获游离蛋白。通过这两个步骤,可以从混合物中成功纯化出完整的三角形RNP。显然,与未精制的产品相比,展示了三种蛋白质结合肽的纯化的三角RNP表现出更高的性能。从概念上讲,此纯化程序应适用于纯化由RNP以外的多种组分组成的各种复合物。

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