用PCR菌落平行分析人p53蛋白四聚域突变体。

IF 3.5 Q1 EDUCATION & EDUCATIONAL RESEARCH Genomic medicine Pub Date : 2007-01-01 Epub Date: 2007-09-05 DOI:10.1007/s11568-007-9011-8
Joshua Merritt, Kim G Roberts, James A Butz, Jeremy S Edwards
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引用次数: 5

摘要

一种高度平行的酵母功能试验,能够平行筛选大约100- 1000个突变体,并设计用于筛选转录激活蛋白的活性,用于功能表征人类p53转录因子和肿瘤抑制蛋白的四聚域突变体。在酿酒酵母中对人类p53蛋白四聚域3个位置的19个可能的单氨基酸取代(57个突变体)进行了功能筛选。研究发现,氨基酸Leu330和Ile332的侧链构成了稳定活性p53四聚体的疏水袋的一部分,它们可以耐受大多数疏水氨基酸取代,而亲水性取代会导致蛋白质失活。氨基酸Gln331基本上耐受所有突变。重要的是,利用高度平行的诱变和克隆技术,结合最近报道的高度平行的DNA测序方法,将能够增加额外的2-3个数量级的吞吐量。
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Parallel analysis of tetramerization domain mutants of the human p53 protein using PCR colonies.

A highly-parallel yeast functional assay, capable of screening approximately 100-1,000 mutants in parallel and designed to screen the activity of transcription activator proteins, was utilized to functionally characterize tetramerization domain mutants of the human p53 transcription factor and tumor suppressor protein. A library containing each of the 19 possible single amino acid substitutions (57 mutants) at three positions in the tetramerization domain of the human p53 protein, was functionally screened in Saccharomyces cerevisiae. Amino acids Leu330 and Ile332, whose side chains form a portion of a hydrophobic pocket that stabilizes the active p53 tetramer, were found to tolerate most hydrophobic amino acid substitutions while hydrophilic substitutions resulted in the inactivation of the protein. Amino acid Gln331 tolerated essentially all mutations. Importantly, highly parallel mutagenesis and cloning techniques were utilized which, in conjunction with recently reported highly parallel DNA sequencing methods, would be capable of increasing throughput an additional 2-3 orders of magnitude.

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