SELEX (Systematic Evolution of Ligands by EXponential enrichment) is a technique used to develop aptamers—single-stranded DNA or RNA oligonucleotides that bind to a specific target molecule with high affinity and specificity, akin to antibodies.
Whole Cell-SELEX is a variant where the target is not a purified protein, but an entire living cell. This is crucial for discovering aptamers against:
Native cell-surface proteins in their natural conformation and modification state.
Complex membrane protein complexes.
Disease-specific cell markers (e.g., on cancer cells, pathogens) without prior knowledge of the specific molecular target.
Specific cell types in a heterogeneous mixture (e.g., cancer stem cells within a tumor).
A service provider performs this technically demanding and iterative process on behalf of researchers or companies.
A typical service workflow involves close collaboration with the client:
1. Project Design & Consultation
Defining Targets: Client specifies the positive selection cell (e.g., human glioblastoma cells) and the critical negative/counter selection cell (e.g., normal astrocytes or a related cell line). This is key to generating selective aptamers.
Library Design: The service provider uses a vast (10^14 – 10^15 sequences) random oligonucleotide library.
2. The SELEX Cycle (Iterative Rounds)
This is the core experimental phase performed by the service provider:
Incubation: The library is incubated with the negative selection cells. Unbound sequences are collected to remove binders to common surface features.
Positive Selection: The pre-cleared library is incubated with target cells.
Washing: Weakly or non-specifically bound sequences are washed away.
Elution: Cell-bound aptamers are recovered (e.g., by heating, trypsinization, or cell lysis).
Amplification: Eluted aptamers are amplified by PCR (for DNA-SELEX) or RT-PCR (for RNA-SELEX).
Purification: The amplified pool is purified for the next round.
Monitoring: Binding enrichment is tracked after several rounds using flow cytometry or qPCR.
8-20 rounds are typically required to enrich for high-affinity, specific aptamers.
3. Post-SELEX Analysis & Delivery
Cloning & Sequencing: The final enriched pool is cloned, and individual aptamers are sequenced.
Bioinformatics: Sequences are analyzed for homology to cluster into families and identify consensus motifs.
Characterization of Candidates: The service often includes basic characterization of top candidate aptamers:
Binding Affinity (Kd): Determined via flow cytometry.
Specificity: Tested against control cell lines.
Confocal Microscopy: To confirm cell surface binding.
Final Report & Delivery: Client receives a detailed report, sequence data, and characterized aptamer candidates.
Expertise & Efficiency: Access to specialized skills and optimized protocols, saving months of labor and troubleshooting.
No Target Identification Needed: Ideal for discovering biomarkers or targeting cells with unknown surfaceome changes.
Native Conformation Targets: Aptamers are selected against proteins as they naturally exist on the cell.
Turnkey Solution: From design to characterized candidates, allowing researchers to focus on downstream applications.
Reduced Infrastructure Cost: Avoids capital investment in specialized equipment (e.g., high-throughput sequencers, FACS).
A complete service package usually includes:
A finalized, project-specific SELEX protocol.
The final enriched aptamer pool.
Sequences and clustering analysis of 50-200 individual aptamer clones.
3-10 lead candidate aptamer sequences.
In vitro binding data (Kd and specificity) for the lead candidates.
A comprehensive project report.
Experience & Track Record: Look for published work or case studies in your field (e.g., oncology, immunology).
Cell Line Expertise: Ensure they can handle your specific cell types (adherent, suspension, primary cells, etc.).
Counter-Selection Strategy: Their approach to negative selection is critical for specificity.
Characterization Depth: Clarify what level of binding validation (Kd, specificity, microscopy) is included.
Intellectual Property (IP) Terms: Clearly define ownership of the discovered aptamer sequences. This is crucial.
Timeline & Cost: A full service can take 3-6 months and cost anywhere from $30,000 to $100,000+, depending on scope and characterization.
Unknown Target: The specific protein target of the aptamer remains unidentified after SELEX (requires separate target identification efforts like protein pull-down/MS).
Complexity: Working with whole cells introduces variables like cell viability, receptor internalization, and batch-to-batch variation.
Service vs. In-House: For labs planning extensive aptamer development, building in-house capacity might be more cost-effective long-term.
The aptamers generated from this service can be used for:
Diagnostics: As detection probes in flow cytometry, imaging, or biosensors.
Targeted Drug Delivery: Conjugated to nanoparticles, drugs, or siRNAs.
Cell Isolation: For magnetic or fluorescence-activated cell sorting (FACS).
Therapeutics: As antagonistic or agonistic agents (e.g., Macugen® for AMD).
Basic Research: As tools to study cell surface biology and protein function.
By outsourcing to a specialized Whole Cell-SELEX Aptamer Screening Service, researchers can rapidly acquire powerful molecular tools for cell-specific targeting, accelerating their diagnostic and therapeutic development pipelines.
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