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  • Antibody engineering
  • Sample prep from FFPE tissue
  • Single-cell sequencing
Mini prep kits to isolate DNA from formalin-fixed, paraffin-embedded (FFPE) tissue specimens NucleoSpin DNA FFPE XS
Two-in-one mini prep kit for the isolation of small (e.g., miRNA) and large RNA from even very limited formalin-fixed, paraffin-embedded samples NucleoSpin totalRNA FFPE
Articles showing data related to our nucleic acid purification kits Nucleic acid purification learning center

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Home › Applications › Alzheimer's disease research › Sample prep from FFPE tissue

Alzheimer's disease research

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  • Sample prep from FFPE tissue
  • Single-cell sequencing
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Mini prep kits to isolate DNA from formalin-fixed, paraffin-embedded (FFPE) tissue specimens NucleoSpin DNA FFPE XS
Two-in-one mini prep kit for the isolation of small (e.g., miRNA) and large RNA from even very limited formalin-fixed, paraffin-embedded samples NucleoSpin totalRNA FFPE
Articles showing data related to our nucleic acid purification kits Nucleic acid purification learning center

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Sample prep for AD research: FFPE tissue

The fixation of brain tissue with formaldehyde (also known as formalin), followed by tissue dehydration and embedding into a paraffin block, is a common method of preservation that has been used for almost a century. This approach renders tissue remarkably stable, allowing the long-term storage (years to decades) of Alzheimer's and control tissue in ambient conditions. These FFPE blocks are highly compatible with immunohistochemical analyses of protein expression and cell morphology and, as a result, research and clinical institutions have accumulated enormous biobanks of human tissue that may consist of thousands of samples. These samples can span several decades and are linked with relevant genetic, clinical, and diagnostic data. Of particular utility for CNS researchers is that tissue blocks may be sorted by neuroanatomical region, a key consideration in understanding the progression and impact of Alzheimer's disease.

While FFPE tissue provides an incredibly valuable research tool, the fixation process causes extensive nucleic acid/protein crosslinking, DNA and RNA fragmentation, and the deamination and/or oxidation of bases, rendering FFPE samples a challenging source of DNA and RNA. Fortunately, specialized methods have been developed for nucleic acid extraction from FFPE samples that yield outputs suitable for applications such as PCR and next-generation sequencing.

Please note that Macherey-Nagel nucleic acid purification products are only available from Takara Bio in North America, India, and Japan.

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DNA purification

Takara Bio offers both silica membrane- and magnetic bead-based technologies for the purification of DNA from a wide array of FFPE tissue types with the NucleoSpin DNA FFPE XS and NucleoMag DNA FFPE kits. Both technologies incorporate the use of an odorless, non-toxic, xylene-free reagent for paraffin removal. Samples are then treated with proteinase to solubilize the fixed tissue and release DNA into solution, followed by heat incubation in a specially formulated buffer to eliminate crosslinks. Lysate DNA is then bound to a silica membrane or paramagnetic beads, subjected to sequential wash steps, and eluted. The NucleoSpin FFPE DNA kit is provided in both single- and multi-prep formats for varying throughput demands, whereas the NucleoMag FFPE DNA kit has been developed primarily for automated, high-throughput processing.

Demonstration of the outstanding yield and performance of our NucleoMag and NucleoSpin kits for DNA extraction from FFPE tissues.

Figure 1. Outstanding yield and PCR performance of de-crosslinked DNA with NucleoSpin DNA FFPE kits. Panel A. DNA was isolated with NucleoMag DNA FFPE from 1 slice of mouse FFPE tissue section/prep (4 preps for each tissue type). DNA yield (dark blue bars) was quantified via optical density, and qPCR analyses (orange squares) were performed using the Thermo Fisher Scientific Maxima SYBR Green qPCR Master Mix. Panel B. DNA was isolated from FFPE rat liver tissue with NucleoSpin DNA FFPE XS (2x blue graphs) and with an FFPE mini elution kit from Competitor Q (2x orange graphs), and a 100-bp target was amplified by PCR using a Roche LightCycler system. Yields were consistently higher with NucleoSpin DNA FFPE XS, and the DNA provided better PCR performance relative to the output from Competitor Q's kit. For this comparison, the starting sample was one section of FFPE tissue that was subjected to overnight lysis and eluted in a volume of 30 µl.

RNA purification

For purification of total RNA from FFPE samples, Takara Bio offers silica membrane-based technologies in single-prep formats designed for varying input amounts: NucleoSpin totalRNA FFPE and NucleoSpin totalRNA FFPE XS. Following deparaffinization, proteinase treatment, and heating, the lysate is applied to the membrane under conditions that enable binding of diverse RNA species, including small RNAs. Residual DNA is then digested via an on-column DNase treatment and, following successive washing steps, RNA is eluted in a small volume of RNase-free water, yielding highly concentrated RNA with superior yield and lower gDNA contamination than competitors' kits (Figure 2).

NucleoSpin total RNA FFPE provides high RNA yields and lower DNA contamination from brain tissue relative to competitor's kits.

Figure 2. NucleoSpin totalRNA FFPE provides higher RNA yields and lower DNA contamination from brain tissue relative to competitor's kits. Total RNA was isolated from four 10-µm thick FFPE sections of mouse brain tissue with NucleoSpin totalRNA FFPE (MN) and three competitor kits (Q, A, and P). Panel A. mRNA and miRNA targets were amplified by qPCR (the mRNA target consisted of a 230-nt portion of the β2-microglobulin gene, while the miRNA target was analyzed using the miR-16 TaqMan MicroRNA Assay. (Note: miRNA samples were reverse transcribed separately using the TaqMan MicroRNA Reverse Transcription Kit from Thermo Fisher Scientific.) Panel B. Residual DNA was assayed by amplifying a 191-bp fragment of the mGAPDH gene. For both assays, the lower CT values observed for samples processed with the NucleoSpin totalRNA FFPE kit provided higher RNA yields and lower DNA contamination relative to competitor's kits.


Featured products

Cat. # Product Size Price License Quantity Details
740980.10 NucleoSpin® DNA FFPE XS 10 Preps USD $54.00

NucleoSpin DNA FFPE XS 10 preps for the purification of DNA from FFPE samples - NucleoSpin DNA FFPE XS Columns, Collection Tubes, Paraffin Dissolver, buffers, Proteinase K

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

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740980.10: NucleoSpin DNA FFPE XS

740980.10: NucleoSpin DNA FFPE XS

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Outstanding PCR performance due to efficient recovery of de-crosslinked DNA

Outstanding PCR performance due to efficient recovery of de-crosslinked DNA

Outstanding PCR performance due to efficient recovery of de-crosslinked DNA. DNA was isolated from formalin-fixed and paraffin-embedded rat liver tissue with NucleoSpin DNA FFPE XS (2X, blue graphs) and with a FFPE mini elution kit from Competitor Q (2X, orange graphs). DNA isolated with NucleoSpin DNA FFPE XS is consistently high in yields and shows better performance in the PCR reaction than the competitor kit. Roche LightCycler real-time PCR, target length: 100 bp. Starting material: 1 section FFPE rat liver with overnight lysis and 30 μl elution volume.

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NucleoSpin DNA FFPE XS procedure

NucleoSpin DNA FFPE XS procedure

NucleoSpin DNA FFPE XS procedure.

744320.1 NucleoMag® DNA FFPE 1 x 96 Preps USD $520.00

NucleoMag DNA FFPE kits employ superparamagnetic beads to enable high-throughput DNA purification from formalin-fixed, paraffin-embedded (FFPE) samples using manual or automated processing. The kits can be used to process fresh or archived samples and are compatible with inputs of ≤5 mg of tissue and ≤15 mg of paraffin. Purified DNA fragments typically range in size from 50 bp–5 kbp and are eluted in volumes >25 µl. The kits include blue-colored Paraffin Dissolver for convenient paraffin removal and enable processing of 96 samples in ~2 hours.

Cat. # 744320.1 includes sufficient reagents and materials for processing of 96 samples.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

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744320.1: NucleoMag DNA FFPE

744320.1: NucleoMag DNA FFPE

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Competitor A (A) and competitor I (B) show higher CT values, indicating a lower yield compared to samples purified with NucleoMag DNA FFPE.

Competitor A (A) and competitor I (B) show higher CT values, indicating a lower yield compared to samples purified with NucleoMag DNA FFPE.

NucleoMag DNA FFPE provides better PCR performance than competitor kits. Genomic DNA was purified from FFPE samples using NucleoMag DNA FFPE in comparison with kits from Competitor A and Competitor I and analyzed using a LightCycler PCR system and the DyNAmo Capillary SYBR Green qPCR Kit (amplicon size: 191 bp). qPCR of DNA purified with kits from Competitor A (Panel A) and Competitor I (Panel B) resulted in higher Ct values, indicating lower DNA yields compared to samples purified with NucleoMag DNA FFPE.

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The NucleoMag DNA FFPE kit leverages the reversible adsorption of nucleic acids on paramagnetic beads to allow a quick, simple workflow for high-purity genomic DNA from FFPE tissue.

The NucleoMag DNA FFPE kit leverages the reversible adsorption of nucleic acids on paramagnetic beads to allow a quick, simple workflow for high-purity genomic DNA from FFPE tissue.

The NucleoMag DNA FFPE procedure.

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The NucleoMag DNA FFPE kit provides higher DNA yields from embedded mouse lung, liver, and kidney sections compared to competitor kits (A, I).

The NucleoMag DNA FFPE kit provides higher DNA yields from embedded mouse lung, liver, and kidney sections compared to competitor kits (A, I).

NucleoMag DNA FFPE provides higher yields than competitor kits. Genomic DNA was purified in triplicate from embedded mouse lung, liver, and kidney tissue sections using NucleoMag DNA FFPE and two competitor kits. The NucleoMag DNA FFPE kit provided higher DNA yields than the competitor kits (A, I).

740982.10 NucleoSpin® totalRNA FFPE 10 Preps USD $92.00

The NucleoSpin totalRNA FFPE kit (50 preps) allows for the purification of small and large RNA species from standard FFPE samples (<50 mg tissue) into a 30–50 µl elution volume. The kit includes NucleoSpin RNA Columns, Collection Tubes, Paraffin Dissolver, buffers, Proteinase K, and RNase-free rDNase.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

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740982.10: NucleoSpin totalRNA FFPE

740982.10: NucleoSpin totalRNA FFPE

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NucleoSpin totalRNA FFPE provides better RT-PCR performance (lower CT values) than competitor kits, indicating higher RNA yields

NucleoSpin totalRNA FFPE provides better RT-PCR performance (lower CT values) than competitor kits, indicating higher RNA yields

NucleoSpin totalRNA FFPE provides better RT-PCR performance (lower CT values) than competitor kits, indicating higher RNA yields. Large (e.g., mRNA) and small (e.g., miRNA) RNA were isolated from 4 x 10 μm FFPE sections of mouse brain tissue with NucleoSpin totalRNA FFPE and three competitor kits (Q, A, P). Quantification of mRNA* and miRNA** was performed using qRT-PCR. Low CT values indicate high RNA yields.

*The amplification target consists of a 230-base fragment of the β2-microglobulin gene.
**miRNA was quantified using the miR-16 MicroRNA Assay in the TaqMan MicroRNA Reverse Transcription Kit from Applied Biosystems.

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NucleoSpin totalRNA FFPE provides more efficient gDNA removal than competitor kits

NucleoSpin totalRNA FFPE provides more efficient gDNA removal than competitor kits

NucleoSpin totalRNA FFPE provides more efficient gDNA removal than competitor kits. Large (e.g., mRNA) and small (e.g., miRNA) RNA were isolated from 4 x 10 μm FFPE sections of mouse brain tissue with NucleoSpin totalRNA FFPE and three competitor kits (Q, A, P). Residual DNA was assayed by amplifying a 191-bp fragment of the mGAPDH gene. Higher CT values correspond to lower amounts of residual DNA.

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The higher concentration of total RNA obtained from XS columns allows efficient, sensitive qRT-PCR from very small FFPE samples

The higher concentration of total RNA obtained from XS columns allows efficient, sensitive qRT-PCR from very small FFPE samples

The higher concentration of total RNA obtained from XS columns allows efficient, sensitive qRT-PCR from very small FFPE samples. Trace amounts of FFPE samples (1 x 15 μm mouse spleen and 1 x 10 μm mouse heart) were used to isolate mRNA and miRNA with NucleoSpin totalRNA FFPE and NucleoSpin totalRNA FFPE XS. The RNA was eluted in 50 μl (using a NucleoSpin totalRNA FFPE mini spin column) and 20 μl (using a NucleoSpin totalRNA FFPE XS column). The mRNA* and miRNA** eluted from the XS column at higher concentrations, reducing the CT value by at least one cycle. When using standard FFPE sample amounts, NucleoSpin totalRNA FFPE (which uses mini spin columns) is recommended in order to avoid possible column overloading.

*The amplification target consists of a 230-base fragment of the β2-microglobulin gene.
**miRNA was quantified using the miR-16 MicroRNA Assay in the TaqMan MicroRNA Reverse Transcription Kit from Applied Biosystems

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The NucleoSpin totalRNA FFPE and NucleoSpin totalRNA FFPE XS procedures are the same for both kits

The NucleoSpin totalRNA FFPE and NucleoSpin totalRNA FFPE XS procedures are the same for both kits
The NucleoSpin totalRNA FFPE and NucleoSpin totalRNA FFPE XS procedures are the same for both kits. They only differ in that NucleoSpin totalRNA FFPE uses mini spin columns which elute in 30–50 µl to purify standard FFPE samples (<50 mg tissue), while NucleoSpin totalRNA FFPE XS uses XS columns which elute in 5–30 µl to purify very small FFPE samples (< 5 mg tissue).
740969.10 NucleoSpin® totalRNA FFPE XS 10 Preps USD $101.00

The NucleoSpin totalRNA FFPE kit (50 preps) allows for the purification of small and large RNA species from very small FFPE samples (<5 mg tissue) into a 5–30 µl elution volume. The kit includes NucleoSpin RNA FFPE XS Columns, Collection Tubes, Paraffin Dissolver, buffers, Proteinase K, and RNase-free rDNase.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

Documents Image Data

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740969.10: NucleoSpin totalRNA FFPE XS

740969.10: NucleoSpin totalRNA FFPE XS

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NucleoSpin XS columns are designed for efficient elution of DNA/RNA in small volumes

NucleoSpin XS columns are designed for efficient elution of DNA/RNA in small volumes

NucleoSpin XS columns are designed for efficient elution of DNA/RNA in small volumes. Panel A. The columns are optimized to hold a very small silica membrane, yet fit inside a standard 1.5 ml microfuge tube. Panel B. The exceptionally small (2.0 mm) diameter of the NucleoSpinXS membrane (Column MN) allows efficient elution in only 5–30 μl. It provides a significant advantage over the small-sample column offered by Competitor Q (Column Q; 4.8 mm diameter), which requires an elution volume of at least 10–30 μl.

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NucleoSpin totalRNA FFPE provides better RT-PCR performance (lower CT values) than competitor kits, indicating higher RNA yields

NucleoSpin totalRNA FFPE provides better RT-PCR performance (lower CT values) than competitor kits, indicating higher RNA yields

NucleoSpin totalRNA FFPE provides better RT-PCR performance (lower CT values) than competitor kits, indicating higher RNA yields. Large (e.g., mRNA) and small (e.g., miRNA) RNA were isolated from 4 x 10 μm FFPE sections of mouse brain tissue with NucleoSpin totalRNA FFPE and three competitor kits (Q, A, P). Quantification of mRNA* and miRNA** was performed using qRT-PCR. Low CT values indicate high RNA yields.

*The amplification target consists of a 230-base fragment of the β2-microglobulin gene.
**miRNA was quantified using the miR-16 MicroRNA Assay in the TaqMan MicroRNA Reverse Transcription Kit from Applied Biosystems.

Back

NucleoSpin totalRNA FFPE provides more efficient gDNA removal than competitor kits

NucleoSpin totalRNA FFPE provides more efficient gDNA removal than competitor kits

NucleoSpin totalRNA FFPE provides more efficient gDNA removal than competitor kits. Large (e.g., mRNA) and small (e.g., miRNA) RNA were isolated from 4 x 10 μm FFPE sections of mouse brain tissue with NucleoSpin totalRNA FFPE and three competitor kits (Q, A, P). Residual DNA was assayed by amplifying a 191-bp fragment of the mGAPDH gene. Higher CT values correspond to lower amounts of residual DNA.

Back

The higher concentration of total RNA obtained from XS columns allows efficient, sensitive qRT-PCR from very small FFPE samples

The higher concentration of total RNA obtained from XS columns allows efficient, sensitive qRT-PCR from very small FFPE samples

The higher concentration of total RNA obtained from XS columns allows efficient, sensitive qRT-PCR from very small FFPE samples. Trace amounts of FFPE samples (1 x 15 μm mouse spleen and 1 x 10 μm mouse heart) were used to isolate mRNA and miRNA with NucleoSpin totalRNA FFPE and NucleoSpin totalRNA FFPE XS. The RNA was eluted in 50 μl (using a NucleoSpin totalRNA FFPE mini spin column) and 20 μl (using a NucleoSpin totalRNA FFPE XS column). The mRNA* and miRNA** eluted from the XS column at higher concentrations, reducing the CT value by at least one cycle. When using standard FFPE sample amounts, NucleoSpin totalRNA FFPE (which uses mini spin columns) is recommended in order to avoid possible column overloading.

*The amplification target consists of a 230-base fragment of the β2-microglobulin gene.
**miRNA was quantified using the miR-16 MicroRNA Assay in the TaqMan MicroRNA Reverse Transcription Kit from Applied Biosystems

Back

The NucleoSpin totalRNA FFPE and NucleoSpin totalRNA FFPE XS procedures are the same for both kits

The NucleoSpin totalRNA FFPE and NucleoSpin totalRNA FFPE XS procedures are the same for both kits
The NucleoSpin totalRNA FFPE and NucleoSpin totalRNA FFPE XS procedures are the same for both kits. They only differ in that NucleoSpin totalRNA FFPE uses mini spin columns which elute in 30–50 µl to purify standard FFPE samples (<50 mg tissue), while NucleoSpin totalRNA FFPE XS uses XS columns which elute in 5–30 µl to purify very small FFPE samples (< 5 mg tissue).

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Takara Bio USA, Inc. provides kits, reagents, instruments, and services that help researchers explore questions about gene discovery, regulation, and function. As a member of the Takara Bio Group, Takara Bio USA is part of a company that holds a leadership position in the global market and is committed to improving the human condition through biotechnology. Our mission is to develop high-quality innovative tools and services to accelerate discovery.

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