mRNA Display is an in vitro selection and directed-evolution technology that physically couples a peptide (or protein) to the mRNA sequence that encodes it through a covalent bond. This genotype–phenotype “fusion” allows researchers to screen enormous molecular libraries and then recover the winning sequences by amplification, enabling fast, iterative optimization under tightly controlled experimental conditions. 1) The Core Idea: Genotype–Phenotype Coupling Without Cells Every selection technology needs a reliable way to keep “what a molecule does” attached to “the information that made it.” In mRNA Display, that attachment is literal: the newly made peptide becomes covalently linked to its own mRNA, producing a stable fusion that survives stringent washing and enrichment steps. This is a major conceptual advantage over systems where the linkage is non-covalent or depends on living cells for propagation. Because the entire workflow is performed in vitro, the experimenter can tune conditions (buffers, salts, temperature, denaturants, competitors) to match the target biology and the selection pressure they want to apply. 2) How the Covalent Link Is Formed: Puromycin at the 3′ End The “magic” reagent behind classic mRNA Display is puromycin, a molecule that mimics the 3′ end of an aminoacyl-tRNA. When puromycin is physically…
We possess particular expertise in developing aptamers for a wide range of complex protein targets—such as membrane proteins, kinases, cytokines, and antibodies. By optimizing screening strategies, we overcome challenges that are difficult to resolve with traditional methods, delivering highly specific aptamers with performance comparable to or even surpassing that of monoclonal antibodies. For small molecules—including hormones, toxins, and antibiotics—we employ unique library construction and screening technologies. These effectively address the challenge of limited epitopes in small-molecule targets, providing clients with key recognition elements for applications in small-molecule detection, environmental monitoring, food safety, and beyond.
We offer one-stop peptide screening services, ranging from library design and high-throughput screening to functional validation. Leveraging our diverse peptide libraries (including random libraries, phage display libraries, cyclic peptide libraries, etc.), we can rapidly identify functional peptides with high affinity and specificity for specific targets. These peptide molecules hold broad application potential in areas such as drug lead compound development, cell-penetrating peptides, and core raw materials for diagnostic reagents.
High-throughput screening (HTS) has become one of the most influential technologies in modern biochemical research, especially in the field of peptide discovery. By integrating robotics, automated liquid handling, and advanced detection systems, HTS enables researchers to rapidly evaluate thousands to millions of peptide candidates in a short period of time. This knowledge-based overview explains how HTS works, why it is essential for peptide studies, and what scientific advantages it brings. What Is High-Throughput Screening (HTS)? High-throughput screening is an automated experimental approach used to test large libraries of biological or chemical samples — such as peptides — for specific biological activities. HTS platforms combine robotics, multi-well plates, imaging systems, and computational tools to perform parallel experiments at exceptional speed and accuracy. For peptide research, HTS allows scientists to investigate binding affinity, enzyme activity, structural behavior, or therapeutic potential across massive sample sets. What would traditionally require months of manual experiments can now be completed within hours or days. How HTS Works in Peptide Research HTS follows a structured workflow designed for consistency and automation: 1. Library Preparation Researchers first assemble a peptide library, which may include: Synthetic peptide variants Sequence-modified analogs Naturally derived peptide fragments…
In molecular biology and biotherapeutic design, specificity refers to a peptide’s ability to bind only to its intended target while avoiding interactions with unrelated molecules. This property is a cornerstone of precision medicine, enabling researchers to create compounds that influence biological processes with minimal unintended effects. What Specificity Means in Peptide–Target Interactions Specificity arises from the precise arrangement of a peptide’s amino acids. These structural features allow the peptide to recognize a unique three-dimensional pattern—such as a receptor pocket, an exposed protein domain, or a biochemical motif—on its target. Even minor variations in peptide shape, charge distribution, or hydrophobic patterns can dramatically alter the binding profile. This molecular “fit” principle ensures that effective peptides interact only with their designated targets. Why Specificity Matters in Research and Therapeutic Development High specificity offers several critical advantages in scientific and clinical applications: Reduced Off-Target Effects When a peptide binds only to its intended molecule, the likelihood of unintended interactions decreases, improving safety and reliability. Enhanced Experimental Clarity Researchers can interpret results more accurately because the peptide affects a single biological component. Improved Drug Precision Therapeutic peptides with strong specificity can modulate disease-related pathways without disturbing healthy tissues, supporting the development of…
Affinity—commonly described as the strength of binding between a peptide and its biological target—is a foundational concept in molecular biology, biochemistry, drug discovery, and biomedical engineering. For researchers, clinicians, and biotechnology developers, understanding affinity helps predict how effectively a peptide can recognize, bind, and influence a specific molecule within complex biological systems. This article provides a clear, search-optimized, and fully original explanation of affinity, how it is measured, and why it matters. What Is Affinity? Affinity refers to the quantitative strength of the interaction between a peptide and its target, such as a protein, receptor, enzyme, or other biomolecule. When a peptide binds strongly to its target, the system is said to have high affinity; when the binding is weak or transient, it exhibits low affinity. In molecular terms, affinity represents the balance between: Association (binding) Dissociation (unbinding) A high-affinity interaction favors stable attachment, often requiring only a small amount of peptide to achieve effective binding. Why Affinity Matters in Peptide Science 1. Precision in Drug Design Peptide-based therapeutics rely heavily on affinity to determine: How well a peptide recognizes a disease-related target Whether the binding is strong enough to produce a therapeutic effect…
Introduction In molecular biology, chemistry, and drug discovery, the term ligand appears everywhere. A ligand is commonly defined as a molecule—often a peptide—that binds specifically and reversibly to a biological target, such as a receptor, enzyme, or ion channel. This binding event can trigger downstream biological effects, regulate cellular pathways, or act as a signal for further molecular interactions. Understanding ligands is crucial for fields like pharmacology, biotechnology, diagnostics, and protein engineering, making the concept a cornerstone of modern life science knowledge. 1. The Core Definition of a Ligand A ligand is a molecule capable of forming a stable complex by binding to a specific site on a target, typically a biomolecule such as a protein. While ligands vary widely in structure, peptides are frequently used due to their versatility, specificity, and ease of engineering. Key Features: Specificity: A ligand binds only to a particular molecular site, similar to a lock-and-key mechanism. Reversibility: Many ligand–target interactions are non-covalent and reversible, allowing dynamic biological regulation. Functionality: Binding can activate, inhibit, stabilize, or signal biological processes. 2. Peptide Ligands: Why They Matter Peptides are short chains of amino acids that naturally fold into shapes favorable…
In biological and biomedical sciences, the term “target” refers to a specific molecule or structure within a living system that researchers aim to observe, influence, or regulate. Although often discussed in the context of drug discovery, targets extend far beyond that domain and include proteins, receptors, enzymes, nucleic acids, and even cell-surface markers that influence physiological and pathological processes. Understanding how targets function provides essential insight into cellular signaling, disease mechanisms, and therapeutic innovation. 1. What Is a Biological Target? A biological target is any molecular entity that participates in a measurable biological activity. It may act as a signal transmitter, structural component, metabolic regulator, or interaction hub within a biochemical pathway. Researchers identify and characterize targets to understand how biological responses are initiated and how they can be modulated to achieve desired outcomes. Common categories of targets include: Proteins – structural proteins, transport proteins, transcription factors Receptors – membrane-bound or intracellular sensors that respond to chemical signals Enzymes – catalysts that regulate metabolic reactions Cell surface markers – characteristic molecules on the external cell membrane used to identify and classify cell types Ion channels – regulators of cellular electrical activity Nucleic acids – DNA or RNA sequences involved…
Amino acids are essential organic molecules that serve as the primary building blocks of peptides and proteins—structures at the core of nearly every biological process. Their unique chemical properties allow them to assemble into countless configurations, enabling life to grow, repair, and operate with extraordinary precision. What Are Amino Acids? Amino acids are small, nitrogen-containing compounds composed of an amino group, a carboxyl group, and a distinct side chain. This side chain—also called the R-group—defines each amino acid’s characteristics, dictating how it interacts with others and influencing the structure of peptides and proteins. Amino Acids as the Basis of Peptides Peptides form when amino acids link together through peptide bonds. This occurs via a condensation reaction, where the carboxyl group of one amino acid connects to the amino group of another. As more amino acids join the chain, they develop into polypeptides, which eventually fold into complex, three-dimensional protein structures. These proteins then serve roles in catalysis, structure, signaling, immunity, and metabolism. Types of Amino Acids Amino acids can be classified into several categories based on their chemical characteristics: Essential amino acids: Cannot be synthesized by the body and must be obtained through diet. Non-essential amino acids:…
The One-Bead-One-Compound (OBOC) Library technique is a powerful combinatorial chemistry strategy used to generate vast molecular libraries for screening and discovery. By anchoring a single, unique compound onto each solid bead, researchers can rapidly explore structural diversity across peptides, peptidomimetics, small molecules, and other bioactive scaffolds. This method has become instrumental in drug discovery, diagnostics, biomolecular engineering, and materials science due to its scalability and efficiency. What Is an OBOC Library? An OBOC library is a collection of beads—typically made of resin or polymer—where each bead carries millions of copies of the same compound. The core idea is that every bead is a microreactor that produces one unique molecular variant. This allows researchers to screen thousands to millions of compounds simultaneously while maintaining clarity on bead-specific identities. The OBOC method was designed to overcome the limitations of traditional combinatorial chemistry, offering a route for high-throughput synthesis without the need for separate reaction vessels for each individual compound. How OBOC Libraries Are Constructed The construction of an OBOC library usually follows a split–mix synthesis approach: Starting Material Distribution Beads are split into multiple reaction vessels. Chemical Coupling Different building blocks (such as amino acids) are coupled to…