Aptamer affinity optimization refers to the process of improving the binding strength and specificity of an aptamer—a short, single-stranded DNA or RNA molecule—to its target molecule (protein, small molecule, or cell surface marker). Higher affinity aptamers result in better sensitivity and selectivity in diagnostic, therapeutic, and research applications. Key Concepts Affinity vs. Specificity Affinity: How tightly an aptamer binds to its target (quantified by dissociation constant, K_d). Lower K_d indicates higher affinity. Specificity: Aptamer’s ability to distinguish the target from similar molecules. Factors Affecting Aptamer Affinity Sequence composition and length. Secondary and tertiary structures (e.g., stem-loops, G-quadruplexes). Target-binding site accessibility. Ionic conditions (Mg²⁺, Na⁺) and pH. Optimization Strategies In vitro Evolution Methods SELEX (Systematic Evolution of Ligands by EXponential enrichment) Iterative rounds of selection and amplification to enrich high-affinity sequences. Variants: High-stringency SELEX: Lower target concentrations or harsher washing steps. Counter-SELEX: Remove sequences binding to similar molecules to enhance specificity. Truncation and Structural Optimization Remove non-essential nucleotides to reduce size while retaining binding. Stabilize key secondary structures (e.g., adding stem loops or G-quadruplex motifs). Chemical Modifications 2’-Fluoro, 2’-O-methyl nucleotides: Enhance stability and sometimes affinity. PEGylation or LNA (locked nucleic acids): Improve folding and binding. Rational Design & Mutagenesis Identify and…
