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肽库:竞争性偶联中受保护氨基酸相对反应速率的测定

Peptide libraries: determination of relative reaction rates of protected amino acids in competitive couplings.

作者信息

Ostresh J M, Winkle J H, Hamashin V T, Houghten R A

机构信息

Torrey Pines Institute for Molecular Studies, San Diego, California 92121.

出版信息

Biopolymers. 1994 Dec;34(12):1681-9. doi: 10.1002/bip.360341212.

DOI:10.1002/bip.360341212
PMID:7849229
Abstract

In the solid phase preparation of synthetic peptide libraries, equimolarity of the resultant peptides in the mixture simplifies the identification of active compounds. Two primary methods for the preparation of combinatorial peptide mixtures are currently used. In the first method, the starting resin is divided into equal aliquots, individual amino acids are coupled to each aliquot, and the resin is then recombined. This process is repeated for each position. However, due to the physical process, each resin bead contains only one peptide sequence. Statistically, for mixtures of longer sequences, an ever-increasing amount of resin is necessary to ensure complete representation of each peptide in the library. Thus, each peptide will be represented in the library if a sufficient number of resin beads are used. In addition, the concentration of each peptide in the library depends on both the number of mixture positions in the library and the amount of resin used. In the second method, mixtures of amino acids are coupled simultaneously at each addition step. The proportion of each amino acid in the reaction mixture is varied inversely to its reaction rate such that, ideally, an equimolar mixture of each peptide is synthesized. An advantage of this method over the previous method is that each peptide is ensured to be represented in the library, although not necessarily in equimolar amounts. It is known that not only do the coupling rates of each amino acid vary, but the coupling rates of individual amino acids also change when coupled to different amino acid resins.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在合成肽库的固相制备中,混合物中所得肽的等摩尔性简化了活性化合物的鉴定。目前使用两种主要方法来制备组合肽混合物。在第一种方法中,将起始树脂分成相等的等分试样,将单个氨基酸偶联到每个等分试样上,然后将树脂重新组合。对每个位置重复此过程。然而,由于物理过程,每个树脂珠仅包含一个肽序列。从统计学上讲,对于较长序列的混合物,需要越来越多的树脂来确保文库中每个肽的完整代表性。因此,如果使用足够数量的树脂珠,每个肽将在文库中得到体现。此外,文库中每个肽的浓度取决于文库中混合物位置的数量和所用树脂的量。在第二种方法中,在每个添加步骤同时偶联氨基酸混合物。反应混合物中每种氨基酸的比例与其反应速率成反比变化,从而理想地合成每种肽的等摩尔混合物。该方法相对于前一种方法的一个优点是,确保每个肽在文库中得到体现,尽管不一定是等摩尔量。已知不仅每种氨基酸的偶联速率不同,而且单个氨基酸与不同氨基酸树脂偶联时的偶联速率也会改变。(摘要截断于250字)

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