Bulk Affinity Assays in Aptamer Selection: Challenges, Theory, and Workflow

Teclemichael, Eden; Le, An T. H.; Krylova, Svetlana M.; Wang, Tong Ye; Krylov, Sergey N.

doi:10.1021/acs.analchem.2c03173

Cited by 3 publications

(3 citation statements)

References 28 publications

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“…In addition, more and more aptamers were discovered with the aptamer selection developed, and EV isolation methods would be more valued when accompanied by the discovery of more EV membrane proteins. 65,66 It has the characteristics of high efficiency, high specicity and friendliness to downstream analysis, and it has broad application prospects. Similar to antibodies, the only weakness of aptamers is that it requires condition optimization, including the types and amount of aptamers on a solid phase matrix.…”

Section: Critical Reviewmentioning

confidence: 99%

Recent research on material-based methods for isolation of extracellular vesicles

Chen,

Li,

Lin

et al. 2024

Anal. Methods

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Section: Critical Reviewmentioning

confidence: 99%

Recent research on material-based methods for isolation of extracellular vesicles

Chen,

Li,

Lin

et al. 2024

Anal. Methods

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“…Instead, our experimental study aimed to test how varying BNR (via varying target concentration) influences the SELEX progress assessed through affinity maturation via a bulk-affinity assay of the output library. This assay relies on optimized measurements of the fraction of unbound library 4 (R), 25 and is deemed to provide accurate comparison of SELEX carried out at different target concentrations.…”

Section: Input Librarymentioning

confidence: 99%

“…To validate BNR as a tool for assessing SELEX progress, we compared BNR values with affinity maturation monitored using the bulk-affinity assay. 25 The results of the bulk affinity assay are summarized in Figure 3b, where R is plotted against the SELEX round number for every target concentration, with Round 0 being the starting library prior to the first partitioning (see Section S4 for the electropherograms and calculations of R values).…”

Section: Input Librarymentioning

confidence: 99%

Quantitative Characterization of Partitioning Stringency in SELEX

Le,

Teclemichael,

Krylova

et al. 2024

Preprint

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Maintaining stringent conditions in SELEX (Systematic Evolution of Ligands by EXponential enrichment) is crucial for obtaining high-affinity aptamers; however, excessive stringency greatly increases the risk of SELEX failure. The control of stringency remains a technical challenge reliant solely on intuition, largely due to the absence of a measure of stringency. Essentially, researchers increase or decrease stringency through its influencers without defining and quantitating it. This study was motivated by our insight that while stringency may not be easily definable via its multiple influencers, it can be delineated by its effect: increasing stringency leads to a decrease in the normalized quantity of binders at the output of partitioning. Building on this insight, we introduce a measure of stringency called the Binder-to-Nonbinder Ratio (BNR) and derive an expression for its experimental determination using a single experimental tool: quantitative PCR. The outcomes of our theoretical analysis and the result of SELEX experiments targeting three distinct protein targets underscore the importance of maintaining a BNR significantly greater than zero to avoid SELEX failure due to excessive stringency – a principle that we term the SELEX non-failure criterion. Utilizing BNR as a measure of stringency alongside this criterion will enable researchers to rationally control SELEX progress.

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