| Literature DB >> 28570047 |
Song Li1, Pamela A Diego-Limpin1, Bekim Bajrami1, Santosh Keshipeddy1, Ying-Wai Lam2,3, Bin Deng2,3, Vahid Farrokhi1, Adam J McShane1, Reza Nemati1, Amy R Howell1, Xudong Yao1,4.
Abstract
Unified analysis of complex reactions of an activity-based probe with proteins in a proteome remains an unsolved challenge. We propose a power expression, rate = kobs[Probe]α, for scaling the progress of proteome-wide reactions and use the scaling factor (0 ≤ α ≤ 1) as an apparent, partial order with respect to the probe to measure the "enzyme-likeness" for a protein in reaction acceleration. Thus, α reports the intrinsic reactivity of the protein with the probe. When α = 0, the involved protein expedites the reaction to the maximal degree; when α = 1, the protein reacts with the probe via an unaccelerated, bimolecular reaction. The selectivity (β) of the probe reacting with two proteins is calculated as a ratio of conversion factors (kobs values) for corresponding power equations. A combination of α and β provides a tiered system for quantitatively assessing the probe efficacy; an ideal probe exhibits high reactivity with its protein targets (low in α) and is highly selective (high in β) in forming the probe-protein adducts. The scaling analysis was demonstrated using proteome-wide reactions of HT-29 cell lysates with a model probe of threonine β-lactone.Entities:
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Year: 2017 PMID: 28570047 PMCID: PMC6368408 DOI: 10.1021/acs.analchem.7b01184
Source DB: PubMed Journal: Anal Chem ISSN: 0003-2700 Impact factor: 6.986