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一个M13噬菌体展示文库中的与靶标无关的肽可追溯到基因II核糖体结合位点的一个有利突变。

A target-unrelated peptide in an M13 phage display library traced to an advantageous mutation in the gene II ribosome-binding site.

作者信息

Brammer Leighanne A, Bolduc Benjamin, Kass Jessica L, Felice Kristin M, Noren Christopher J, Hall Marilena Fitzsimons

机构信息

Department of Chemistry, Stonehill College, Easton, MA 02375, USA.

出版信息

Anal Biochem. 2008 Feb 1;373(1):88-98. doi: 10.1016/j.ab.2007.10.015. Epub 2007 Oct 14.

DOI:10.1016/j.ab.2007.10.015
PMID:17976366
Abstract

Screening of the commercially available Ph.D.-7 phage-displayed heptapeptide library for peptides that bind immobilized Zn2+ resulted in the repeated selection of the peptide HAIYPRH, although binding assays indicated that HAIYPRH is not a zinc-binding peptide. HAIYPRH has also been selected in several other laboratories using completely different targets, and its ubiquity suggests that it is a target-unrelated peptide. We demonstrated that phage displaying HAIYPRH are enriched after serial amplification of the library without exposure to target. The amplification of phage displaying HAIYPRH was found to be dramatically faster than that of the library itself. DNA sequencing uncovered a mutation in the Shine-Dalgarno (SD) sequence for gIIp, a protein involved in phage replication, imparting to the SD sequence better complementarity to the 16S ribosomal RNA (rRNA). Introducing this mutation into phage lacking a displayed peptide resulted in accelerated propagation, whereas phage displaying HAIYPRH with a wild-type SD sequence were found to amplify normally. The SD mutation may alter gIIp expression and, consequently, the rate of propagation of phage. In the Ph.D.-7 library, the mutation is coincident with the displayed peptide HAIYPRH, accounting for the target-unrelated selection of this peptide in multiple reported panning experiments.

摘要

对市售的Ph.D.-7噬菌体展示七肽文库进行筛选,寻找与固定化Zn²⁺结合的肽段,结果反复筛选出肽段HAIYPRH,尽管结合试验表明HAIYPRH不是锌结合肽。在其他几个实验室使用完全不同的靶标时也筛选出了HAIYPRH,其普遍性表明它是一种与靶标无关的肽。我们证明,展示HAIYPRH的噬菌体在文库连续扩增后富集,而未接触靶标。发现展示HAIYPRH的噬菌体扩增速度比文库本身显著加快。DNA测序揭示了参与噬菌体复制的蛋白质gIIp的Shine-Dalgarno(SD)序列中的一个突变,使SD序列与16S核糖体RNA(rRNA)具有更好的互补性。将此突变引入缺乏展示肽的噬菌体中导致增殖加速,而具有野生型SD序列的展示HAIYPRH的噬菌体扩增正常。SD突变可能会改变gIIp的表达,从而改变噬菌体的增殖速度。在Ph.D.-7文库中,该突变与展示的肽段HAIYPRH一致,这解释了在多个报道的淘选实验中该肽段与靶标无关的筛选结果。

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