CUT&Tag Technology: A High-Resolution Approach for Protein–DNA Interaction Analysis

Understanding protein–DNA interactions is fundamental to studying gene regulation, epigenetic modifications, and transcriptional control. Traditional methods such as ChIP-seq have long been used for this purpose, but they often face limitations in sensitivity, efficiency, and sample
requirements.

[2025 03 20] cuttag技术解锁比chipseq更精准高效的dna和蛋白质互作研究 3

CUT&Tag (Cleavage Under Targets and Tagmentation) has emerged as an advanced alternative, enabling high-resolution mapping of protein–DNA interactions with improved efficiency and lower input requirements.

Limitations of Conventional ChIP-seq Approaches

While ChIP-seq remains a widely used method, it presents several challenges:

  • Requires large numbers of input cells
  • Involves complex and time-consuming workflows
  • High background noise and lower signal-to-noise ratio
  • Significant sequencing depth required
  • Limited performance in low-input or single-cell applications

These constraints have driven the development of next-generation methods such as CUT&Tag.

How CUT&Tag Works

CUT&Tag leverages antibody-targeted tagmentation to selectively profile protein–DNA
interactions.

[2025 03 20] cuttag技术解锁比chipseq更精准高效的dna和蛋白质互作研究 5

In this approach:

  • Antibodies bind to target proteins (e.g., transcription factors, histone modifications)
  • A Protein A/G–Tn5 transposase fusion is recruited to the binding sites
  • DNA is fragmented and sequencing adapters are inserted directly at target regions
  • Non-target chromatin remains largely intact, reducing background noise

This targeted fragmentation significantly improves signal specificity and simplifies the workflow.

Key Advantages of CUT&Tag

Compared with ChIP-seq, CUT&Tag offers:

  • Higher signal-to-noise ratio
  • Lower sequencing requirements
  • Simplified workflow without crosslinking
  • Compatibility with low-input and single-cell samples
  • Faster library preparation (within one day)

These advantages make CUT&Tag particularly suitable for studies with limited sample
availability or requiring high resolution.

CUT&TagChIP-seqDifferences
Intracellular reaction*Intracellular reaction/
Harvest cells, no special treatment requiredFormaldehyde cross-linkingDifferences in cell processing
Incubate cells with ConA magnetic beadsCell lysis and sonication to fragment genomic DNABackground noise
Primary and secondary antibodies bind to target proteinPrimary antibody binds to target proteinPresence/absence of secondary antibody for epitope amplification
Transposase complex binds to secondary antibody, activating the reactionImmunoprecipitationDifferences in capture method
Magnetic bead recovery of DNA fragmentsElution, reverse cross-linking to obtain DNA fragmentsDifferences in DNA acquisition method and structure
One-step PCR amplification for library preparationMulti-step reactions: end repair + A-tailing, adapter ligation, PCR amplificationDifferences in library amplification workflow
Purify product, proceed to sequencingPurify product, proceed to sequencing/

Workflow Overview

A typical CUT&Tag workflow includes:

  • 2400.Cell immobilization using ConA beads
  • 2401.Cell permeabilization and antibody incubation
  • 2402.Binding of Protein A/G–Tn5 transposase
  • 2403.Activation of tagmentation reaction
  • 2404.DNA purification
  • 2405.PCR amplification and sequencing

The streamlined workflow enables efficient transition from sample to sequencing-ready libraries.

Applications in Research and Drug Development

CUT&Tag is widely applicable in:

  • Epigenetic profiling
  • Transcription factor binding analysis
  • Chromatin accessibility studies
  • Mechanistic studies in disease models
  • Biomarker discovery

Toprion’s Role

As MDL’s international partner, Toprion provides overseas clients with direct access to CNASaccredited laboratory services. We ensure efficient communication, project coordination, and reliable delivery for global collaborations.

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