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HomeMagPrep® Magnetic for Nucleic Acid Technology

MagPrep® Magnetic for Nucleic Acid Technology

Micrograph showing microspheres and silica.

When it comes to nucleic acid purification, the need for a more convenient, automatable approach is paramount. Traditional methods may be time-consuming and labor-intensive, making the demand for a scalable and environmentally friendly solution all the more critical. Additionally, concerns about the safety and environmental impact of purification methods drive the need for a process that avoids wasteful and dangerous chemicals and byproducts.

Section Overview

Silica Magnetic Microspheres 

MagPrep® Silica magnetic particles were designed to meet the most important requirements for solid supports being used in nucleic acid purification protocols. MagPrep® Silica binds RNA as well as DNA with very high efficiency and under generic conditions, such as in the presence of chaotropic reagents/salts and under mild acidic buffer conditions). More importantly, nucleic acids bound to the particles tolerate the use of slightly acidic aqueous wash buffers without being released. Based on the binding buffer formulation design, the use of alcohol containing buffer or non-alcohol containing buffer can be utilized during nucleic acid binding and the wash steps. Elution of bound nucleic acids is accomplished by aqueous buffer pHed higher than 8.0. MagPrep® Silica have a particle size of 100nm. Homogenized suspensions of the particles are stable for up to five minutes without further agitation. Magnetic clearance of the suspension takes less than 15 seconds. These properties are particularly useful for high-throughput screening (HTS) applications. Our flagship MagPrep® Silica Particles (1.01193) have been widely used in large-scale high-throughput settings and are prized for their easy handling and reliable performance with robust yield at an affordable price point.

  • Convenience and Automation: Traditional nucleic acid purification methods may be time-consuming and labor-intensive. MagPrep® Magnetic Silica Particles offer a more convenient and automatable approach, potentially reducing the manual effort required for purification processes.
  • Scalability: Some purification methods may not scale well to high-throughput settings or may require significant adjustments when dealing with larger sample sizes. The use of magnetic particles allows for easily scalable purification processes.
  • Safety and Environmental Concerns: Column or solvent-based purification approaches might involve the use of hazardous chemicals and generate wasteful byproducts, presenting safety and environmental challenges. Magnetic particle purifications offer a safer and more environmentally friendly alternative.

Frequently Asked Questions about DNA and RNA Purification with Silica Magnetic Particles 

With significant scientific expertise and continuous product innovations, we are happy to help troubleshoot your particle-based nucleic acid purification needs.

What Is The Principle Behind Silica Particle Nucleic Acid Purification?

The principle behind silica particle nucleic acid purification revolves around the selective binding of nucleic acids to the silica surface under specific buffer conditions. Silica particles have a high affinity for nucleic acids, allowing them to efficiently capture DNA and RNA from complex biological samples. This binding occurs in the presence of chaotropic reagents or under mild acidic buffer conditions, ensuring that the nucleic acids are effectively immobilized on the particles.

Once bound to the silica particles, the nucleic acids can withstand wash steps using slightly acidic aqueous buffers without being released, eliminating the need for the use of ethanol during the wash process. Elution of the bound nucleic acids is achieved by using any type of aqueous buffer at a higher pH, typically above 8.0.

This method provides a highly efficient and reliable means of purifying nucleic acids from a variety of sample types, making it a preferred choice for applications such as pathogen detection, cancer screening, genetic testing, and high-throughput screening (HTS) due to its robust yield, ease of handling, and scalability.

 

This illustration depicts the initial step of DNA/RNA purification, starting with a biological sample containing the nucleic acids to be extracted.

1. Sample

Begin with the biological sample containing the nucleic acids to be extracted.

    An illustration showing the addition of lysis buffer and proteinase K to a sample, highlighting the breakdown of cellular components to release nucleic acids.

    Add lysis buffer and proteinase K to break down cellular components and release nucleic acids.

      This image illustrates the addition of MagPrep® Silica Particles, which bind to the released nucleic acids during the purification process.

      Introduce MagPrep® Silica Particles to bind the released nucleic acids.

        An illustration depicting the optional step of adding DNase or RNase to degrade unwanted nucleic acids, depending on the desired outcome.

        Optionally, add DNase or RNase to degrade unwanted nucleic acids, depending on the desired outcome.

          This image shows the magnetic separation process used to isolate silica particles bound with nucleic acids from the solution.

          Use magnetic separation to isolate the silica particles bound with nucleic acids from the solution.

            An illustration highlighting the washing step to remove impurities and contaminants from the bound nucleic acids

            Wash the bound nucleic acids to remove impurities and contaminants.

              A second magnetic separation to ensure that only the purified nucleic acids remain for further analysis.

              Perform another magnetic separation to ensure only the purified nucleic acids remain.

                An illustration showing the final step of eluting the bound nucleic acids to recover RNA, DNA, or both for subsequent analysis.

                Finally, elute the bound nucleic acids to recover either RNA, DNA, or both for further analysis.

                  What Downstream Assays Can Be Performed on Purified Sample?

                  The purified nucleic acid samples obtained through silica particle nucleic acid purification can be utilized in a wide range of downstream assays and applications. These include but are not limited to:

                  • Pathogen Detection: Purified nucleic acids can be used for the detection of viral, bacterial, or fungal pathogens, allowing for the identification and diagnosis of infectious diseases.
                  • Genetic Testing: The purified samples are suitable for genetic testing, including genotyping, gene expression analysis, and mutation detection.
                  • Cancer Screening: Nucleic acid purification enables the extraction of genetic material for cancer-related assays, such as the detection of oncogenes, tumor suppressor genes, and cancer biomarkers.
                  • Sequencing: Purified DNA can be used for various sequencing applications, including whole-genome sequencing, targeted gene sequencing, and metagenomic sequencing.
                  • PCR and qPCR: The purified nucleic acids are suitable for PCR (Polymerase Chain Reaction) and qPCR (quantitative Polymerase Chain Reaction), enabling the amplification and quantification of specific DNA or RNA sequences.
                  • Transcriptional Analysis: Purified RNA can be used for transcriptional analysis, including gene expression profiling, mRNA quantification, and non-coding RNA analysis.
                  • Cloning and Genomic Library Construction: The purified DNA samples can be utilized for cloning and the construction of genomic libraries for downstream functional studies.

                  These applications demonstrate the versatility and utility of purified nucleic acid samples obtained through silica particle nucleic acid purification, making them valuable for a broad spectrum of research, diagnostic, and investigative purposes.

                  What Conditions Are Most Critical To Ensuring High Yield and Sensitive Detection?

                  Several conditions are critical to ensuring high yield and sensitive detection in silica particle nucleic acid purification:

                  • Buffer Conditions: The buffer conditions during binding and wash steps play a crucial role. The use of specific chaotropic reagents or mild acidic buffer conditions facilitates the efficient binding of nucleic acids to the silica surface and subsequent removal of impurities.
                  • Drying: If alcohol containing wash buffers were utilized, ensure particles are dry as alcohols inhibit PCR. 
                  • Elution Buffer pH: The pH of the elution buffer is essential for releasing the bound nucleic acids from the silica particles. Using an aqueous buffer with a pH higher than 8.0 is typically recommended for efficient elution. Typically 10mM Tris pH 8.2 buffer or water. 
                  • Wash Steps: Ensuring that the wash steps are performed using slightly acidic aqueous buffers.
                  • Homogenization and Magnetic Clearance: Proper homogenization of the silica particle suspension and efficient magnetic clearance of the suspension are critical for maintaining stability and ensuring rapid and effective nucleic acid capture and release.

                  By optimizing these conditions, it is possible to achieve high yield and sensitive detection in nucleic acid purification, enabling the successful isolation and subsequent analysis of DNA and RNA from complex biological samples.

                   What Is the Purpose of Silica Resin in DNA Extraction?

                  Salt conditions allow for silica surface groups to capture DNA molecules from complex biological samples, allowing for their subsequent isolation and purification. Silica resin, due to its high affinity for nucleic acids, provides an efficient and reliable means of extracting DNA from various sources, including blood, tissue, and cultured cells.

                  During the extraction process, the DNA in the sample is selectively bound to the silica resin under specific buffer conditions. Impurities and contaminants are effectively removed through subsequent washing steps, leaving the purified DNA bound to the silica resin. Elution of the DNA is then achieved by using an appropriate elution buffer, releasing the purified DNA from the resin for downstream applications.

                  The use of silica resin in DNA extraction facilitates the isolation of high-quality DNA, free from contaminants, and is a critical step in various research, diagnostic, and forensic applications, including PCR, sequencing, genotyping, and genetic testing.

                  What Is the Function of Magnetic Beads in RNA Extraction?

                  In RNA extraction  MagPrep® magnetic beads facilitate binding and purification of RNA molecules from complex biological samples. 

                  During the extraction process, the RNA in the sample is efficiently captured by the magnetic beads. Subsequent washing steps remove impurities and contaminants, leaving the purified RNA bound to the magnetic beads. The use of magnetic beads streamlines the extraction process by enabling the rapid and efficient capture of RNA without the need for labor-intensive centrifugation or filtration steps.

                  Once the RNA is bound to the magnetic beads, it can be eluted using an appropriate buffer, releasing the purified RNA from the beads. The function of magnetic beads in RNA extraction is pivotal for obtaining high-quality RNA samples, free from contaminants, and is an essential step in various research, diagnostic, and therapeutic applications.

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