The Role of Deoxyribonuclease in RNA Purification

Modern molecular biology, transcriptomics, and clinical research require high-quality RNA. Even minor impurities can lead to flawed outcomes. Residual genomic DNA is the most common and problematic contaminant present in RNA.

Researchers incorporate Deoxyribonuclease (DNase) treatment in the RNA purification process to address these challenges. Highly purified forms of human deoxyribonuclease can degrade contaminating DNA while maintaining RNA integrity.

Deoxyribonuclease

These are nucleases that cleave phosphodiester bonds to hydrolyze DNA. Thereby, long DNA polymers are converted into shorter fragments or single nucleotides. The following are the two major categories of DNases:

1. DNase I
2. DNase II

Feature	DNase I	DNase II
Cofactor Requirement	Requires divalent cations	Not required
Optimal Conditions	Neutral pH	Acidic pH
Preferred Substrate	Double-stranded DNA	Double-stranded DNA
Cleavage Pattern	Produces 3′-OH and 5′-phosphate termini	Produces 3′-phosphate ends
Use in Research	RNA purification	Lysosomal DNA degradation

Human deoxyribonuclease, originating from human sources, offers:

• High catalytic efficiency
• Reduced immunogenicity 
• RNase-free purity

These deoxyribonucleases, ensuring consistent, specific DNA removal, are valuable for sensitive RNA purification.

Role of DNase Treatment in RNA Purification

Residual DNA in RNA samples can lead to:

• False-positive amplification
• Distorted gene expression measurements
• Reduced sequencing library quality
• Unreliable downstream analyses
• Ultimately leading to compromised conclusions

How DNase improves RNA integrity

Trace amounts of genomic DNA often co-purify with RNA. DNase eliminates the genomic DNA to preserve the true biological integrity of RNA. This helps prevent DNA-derived signals and ensures that true RNA levels are measured.

There is no false-positive amplification in qPCR/RT-PCR/dPCR. Maintaining RNA-seq quality prevents mapping errors, library prep issues, and skewed transcript counts. It also helps avoid background signals that mask rare RNA species.

Methods of DNase Treatment in RNA Purification

The choice of DNase treatment method depends on the following key factors:

• The workflow
• Sample type
• Desired RNA purity

On-column digestion and in-solution treatment are the most commonly used methods.

DNase activity must be terminated properly to prevent RNA degradation. This is achieved via heat inactivation or cleanup methods.

On-column DNase

In this method, DNase is applied directly to RNA bound on the purification column. This method is not only easy to perform but also integrates with standard kits. However, it may not remove heavy DNA contamination.

In-solution DNase

In this method, DNase is added to a solution containing RNA. This is done during or immediately after extraction, before final purification. It is flexible for different amounts, and the enzyme concentration can be optimized accordingly. However, this method requires additional cleanup to remove the enzyme and DNA fragments.

Heat inactivation

This method deactivates DNase by applying a brief heat treatment after digestion. It is fast and straightforward, but has the following disadvantages:

• It may not fully deactivate stable DNase.
• High heat can affect RNA.

DNase Cleanup

This method uses columns, magnetic beads, or precipitation to remove degraded DNA and DNase. While an extra step adds time, it ensures complete removal and preserves RNA quality.

Optimizing DNase Treatment

Optimization is done by carefully balancing enzyme activity, reaction conditions, and RNA stability.

Enzyme Concentration and Incubation Time

Using too little DNase often leaves residual DNA. On the other hand, excessive DNase use can degrade RNA. Researchers should use the manufacturer’s recommended concentrations. The concentration should be adjusted based on RNA amount, DNA contamination level, and sample type. Shorter incubation with sufficient enzymes can minimize RNA exposure to nucleases.

Buffer Composition and Required Cofactors

DNase activity greatly depends on optimal buffer conditions and cofactors. Improper buffers can reduce efficiency or increase nonspecific degradation.

Always use buffers recommended for the specific DNase. Also, ensure:

• Correct pH
• Ionic strength
• Cofactor concentration

Avoid buffers that contain RNases or chelating agents (like EDTA) that inhibit DNase activity.

Temperature Control

While high temperatures accelerate DNase activity and may destabilize RNA, low temperatures slow the reaction. Perform digestion at the recommended temperature and avoid prolonged exposure at elevated temperatures.

Avoiding RNA Degradation

RNA is highly susceptible to degradation by RNases present in reagents or on surfaces. Even optimized DNase treatment can fail if RNA integrity is compromised.

Always use RNase-free reagents, consumables, and gloves. RNase inhibitors should be included where appropriate. Keep handling time to a minimum and terminate DNase activity promptly.

Applications in Research

Gene Expression Studies (qPCR/RT-PCR)

Residual genomic DNA can lead to false-positive amplification in quantitative PCR (qPCR) and reverse transcription PCR (RT-PCR), skewing gene expression results. DNase treatment ensures that the detected signal originates solely from RNA transcripts.

RNA Sequencing (bulk and single-cell)

DNA contamination can lead to inaccurate mapping and distorted transcript counts. It can also compromise library preparation. DNase eliminates contaminating DNA, and the final data reflect the real transcriptome.

Clinical Diagnostics & Biomarker Research

Reliable RNA quantification underpins many clinical applications, including biomarker identification and RNA-based diagnostic panels. DNase treatment removes residual genomic DNA. The data reflects genuine outcomes instead of contamination-driven artifacts.