An aptamer library is a diverse pool of nucleic acid sequences (DNA or RNA) from which specific aptamers—short oligonucleotides that bind to target molecules with high affinity—can be selected. Constructing a high-quality library is the foundation of aptamer screening technologies like SELEX. 2. Key Components of an Aptamer Library Randomized Region The central portion of the aptamer, typically 20–60 nucleotides, is randomized to generate diversity. Example: N20–N40 where N = A, T/U, G, or C. The diversity determines the probability of finding high-affinity binders. Flanking Constant Regions Short sequences (~15–25 nt) at both ends of the randomized region. Functions: Primer binding sites for PCR amplification. Stability and structural constraints. Overall Length Usually 40–100 nucleotides, balancing structural complexity and amplification efficiency. 3. Steps of Library Construction Design of Oligonucleotides Include random regions flanked by known primer sequences. Example structure:5'-[Primer]-N40-[Primer]-3' Chemical Synthesis Use solid-phase DNA/RNA synthesis to generate the oligonucleotides. Random nucleotides are incorporated using a controlled mixture of A, T/U, G, C. Amplification (for DNA libraries) PCR amplifies the synthesized sequences. RNA libraries require in vitro transcription from DNA templates. Purification Remove truncated or incomplete sequences. Methods: PAGE purification or HPLC. Quality Control Ensure correct length, diversity, and absence of biases.…
