Enhancing Recombinant Protein Quality and Yield by Protein Stability Profiling

蛋白质稳定性 蛋白质纯化 靶蛋白 重组DNA 蛋白质工程 化学 产量(工程) 计算生物学 蛋白质表达 生物化学 生化工程 色谱法 生物 材料科学 基因 工程类 冶金
作者
Tara M. Mezzasalma,James K. Kranz,Winnie Chan,Geoffrey T. Struble,Céline Schalk‐Hihi,Ingrid C. Deckman,Barry A. Springer,Matthew J. Todd
标识
DOI:10.1177/1087057106297984
摘要

The reliable production of large amounts of stable, high-quality proteins is a major challenge facing pharmaceutical protein biochemists, necessary for fulfilling demands from structural biology, for high-throughput screening, and for assay purposes throughout early discovery. One strategy for bypassing purification challenges in problematic systems is to engineer multiple forms of a particular protein to optimize expression, purification, and stability, often resulting in a nonphysiological sub-domain. An alternative strategy is to alter process conditions to maximize wild-type construct stability, based on a specific protein stability profile (PSP). ThermoFluor, a miniaturized 384-well thermal stability assay, has been implemented as a means of monitoring solution-dependent changes in protein stability, complementing the protein engineering and purification processes. A systematic analysis of pH, buffer or salt identity and concentration, biological metals, surfactants, and common excipients in terms of an effect on protein stability rapidly identifies conditions that might be used (or avoided) during protein production. Two PSPs are presented for the kinase catalytic domains of Akt-3 and cFMS, in which information derived from a ThermoFluor PSP led to an altered purification strategy, improving the yield and quality of the protein using the primary sequences of the catalytic domains.

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