Mouse Tail Genomic DNA Kit - 50 preps, high purity

Cat. No.: M665559
Disponible para pedir
GRADE & PURITY BioReagent ? BioReagent grade — tested suitable for life-science and molecular-biology use. Use for cell culture, assays, and biochemical work needing biological compatibility.
 ·  off list, applied to all prices below.
Size
Estado
Price
Qty
50T
M665559-50T
1-2 wks(?)
Item is derived from our semi-finished stock and is processed in 1-2 weeks.
139,90US$
Enter a quantity for the sizes you want to add.
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Why this grade

BioReagent BioReagent for sensitive chromatographic and analytical workflows requiring minimal baseline interference.

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Storage & shipping

Room temperature Ships Normal Check lot-specific COA for exact specifications.

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Quality documents

SDS, COA, datasheet, and spec sheet available for download. Lot-specific COA accessible via lot number lookup.

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Literature proof

Cited in 0 peer-reviewed publications across chromatography, organic synthesis, and cross-coupling reactions.

Descripción general

  This kit is suitable for rapid and simple extraction of genomic DNA from various blood/cell/tissue samples. The extracted genomic DNA features large fragment size, high purity, and good stability, and can be directly used in experiments such as PCR, enzyme digestion, and hybridization. The extraction process does not require phenol-chloroform extraction: blood, cells, or tissues are lysed with lysis buffer and digested with Proteinase K, then can bind to Spin Columns GH4 under the adjustment of absolute ethanol. Residual impurities such as proteins and salts are removed through rapid and thorough washing, and finally, DNA is eluted in Buffer EB.

Product Components and Storage Conditions:

M665559
Component
50T
Storage
M665559A
Buffer DA
15 ml
RT
M665559B
Buffer DLB
15 ml
RT
M665559C
Buffer DW1
13 ml
RT
M665559D
Buffer DW2Plus
12 ml
RT
M665559E
Buffer EB
15 ml
RT
M665559F
Proteinase K(20 mg/ml)
1.2 ml
RT
M665559G
Spin Columns GH4
50 pcs
RT
M665559H
2 ml Collection Tubes
50 pcs
RT

Storage Conditions:
All components of this kit can be stored at room temperature (15°C-25°C) under dry conditions for 12 months. Before use, check if Buffer DA and Buffer DLB have crystals or precipitates. If crystals or precipitates are present, place Buffer DA and Buffer DLB in a 37°C water bath to redissolve.
Precautions:
1. Samples should avoid repeated freezing and thawing, as this will result in smaller extracted DNA fragments and reduced extraction yield.
2. Before first use, 17mL of absolute ethanol must be added to Buffer DW1 (13mL), and 48mL of absolute ethanol must be added to Buffer DW2Plus (12mL).
3. If RNA removal is required, RNase A (100 mg/ml) (Catalog No.: R665518) must be prepared separately.
4. Absolute ethanol must be prepared separately.

Operating Steps:
Before use, add absolute ethanol to Buffer DW1 and Buffer DW2Plus. Please refer to the labels on the bottles for the volume to be added.
1. Sample Processing:
a. Mammalian blood: Take 200 μl of fresh or anticoagulated blood into a 1.5 ml centrifuge tube, and proceed directly to steps 2-10. If the blood volume is less than 200 μl, make up to 200 μl with Buffer DA.
b. Avian, poultry, and amphibian blood: Take 5-20 μl of fresh or anticoagulated blood into a 1.5 ml centrifuge tube, and make up to 200 μl with Buffer DA.
c. Tissue culture cells: Collect approximately 10⁵-10⁶ suspension cells (total cell count should not exceed 5×10⁶) into a 1.5 ml centrifuge tube; for adherent cells, first digest with trypsin and resuspend by pipetting. Centrifuge at 12,000 rpm (~13,400×g) for 1 min, discard the supernatant, add 200 μl Buffer DA to the cell pellet, and vortex until completely resuspended.
d. Animal tissue: Weigh < 25 mg of animal tissue (spleen should be less than 10 mg), grind into fine powder with liquid nitrogen or cut into small pieces with a scalpel, and transfer to a 1.5 ml centrifuge tube pre-filled with 180 μl Buffer DA.
In addition to efficiently extracting DNA from blood, cells, and tissues, this kit can also extract high-quality DNA from bacteria.
e. Bacteria: Take 1-5 ml of bacterial culture, centrifuge at 12,000 rpm (~13,400×g) for 1 min, and aspirate the supernatant as much as possible.
1)For gram-positive bacteria with difficult cell wall lysis, add lysozyme solution for cell wall disruption: Add 110 μl buffer (20 mM Tris, pH 8.0; 2 mM Na₂-EDTA; 1.2% Triton) and 70 μl lysozyme solution (50 mg/ml, provided by the user), and incubate at 37°C for at least 30 min.
2)For relatively easily lysed bacteria, directly add 200 μl Buffer DA to the bacterial pellet and vortex until the bacteria are completely resuspended.
2. Optional step: If RNA removal is required (for cells, tissues, and bacteria), add 4 μl RNase A (100 mg/ml) solution (Catalog No.: R665518). Vortex for 15 sec and incubate at room temperature for 5 min.
3. Add 20 μl Proteinase K and vortex to mix thoroughly.
a. For blood, cell, or bacterial samples, simply add Proteinase K, mix well, and proceed to the next step.
b. For animal tissue samples, add Proteinase K and vortex to mix. Incubate at 56°C until the tissue is completely dissolved, then briefly centrifuge to collect the solution on the inner wall of the tube cap before proceeding to the next step.
Note: Lysis time varies for different tissues, usually taking 1-3 hours (mouse tail requires 6-8 hours of digestion, and overnight digestion is necessary if needed), which will not affect subsequent operations.
4. Add 200 μl Buffer DLB, invert thoroughly to mix, incubate at 70°C for 10 min, and briefly centrifuge to collect the solution on the inner wall of the tube cap.
Note: White precipitate may form when adding Buffer DLB, but it usually disappears during incubation at 70°C and will not affect subsequent experiments.
5. Add 200 μl absolute ethanol and mix (precipitate may appear at this point). Transfer the resulting solution and precipitate to the adsorption column Spin Columns GH4 (place the column in the collection tube), centrifuge at 12,000 rpm (~13,400×g) for 30 sec, discard the filtrate, and return the adsorption column to the collection tube.
6. Add 500 μl Buffer DW1 (ensure absolute ethanol is added before use) to the adsorption column, centrifuge at 12,000 rpm (~13,400×g) for 30 sec, discard the waste liquid, and return the adsorption column to the collection tube.
7. Add 500 μl Buffer DW2Plus (ensure absolute ethanol is added before use) to the adsorption column, centrifuge at 12,000 rpm (~13,400×g) for 30 sec, discard the waste liquid, and return the adsorption column to the collection tube.
8. Repeat step 7 once.
9. Centrifuge at 12,000 rpm for 3 min, and discard the waste liquid in the collection tube.
10. Transfer the adsorption column to a new 1.5 ml centrifuge tube, 悬空滴加 60-200 μl Buffer EB to the center of the adsorption membrane, let stand at room temperature for 1 min, and centrifuge at 12,000 rpm (~13,400×g) for 1 min to obtain the DNA solution.
Note: The volume of Buffer EB should not be less than 60 μl, as a smaller volume will affect recovery efficiency. If water is used as the eluent, ensure its pH is within the range of 7.0-8.5 (NaOH can be used to adjust the pH of water to this range). Store the DNA solution at -20°C.

Frequently Asked Questions and Solutions:

Frequently Asked Questions
Cause
Solution
Column blockage
1. Too much sample input
Please use samples within the compatible range.

2. Inadequate Sample Lysis
Extend the 56°C water bath time and increase the number of inversion and mixing times.
Low DNA Yield
1. The sample has been repeatedly frozen and thawed
Avoid repeated freezing and thawing of samples. It is recommended to use fresh samples or samples that have been frozen frozen and thawed only once.

2. Inadequate lysis of animal tissue
Cut tissue blocks into small pieces as much as possible or grind them with liquid nitrogen. During extraction, ensure that the samples are fully mixed with Buffer DA and Proteinase K in a timely manner, and the 56°C water bath lysis time can be appropriately extended.

3. Incomplete transfer of the lysis mixture into the adsorption column
After cell lysis, add absolute ethanol, flocculent precipitates will appear in the solution, which need to be transferred to the adsorption column together with the solution.

4. Issues with the eluent
Please use the Buffer EB provided with the kit for elution. If using ddH₂O or other eluents, ensure that the pH value of the eluent is between 7.0 - 8.0. Buffer EB can be preheated to 55°C in advance before elution, which is beneficial to improve the DNA yield.

5. Low elution efficiency
The eluent should be dropped in the center of the membrane; increase the elution volume or the number of elutions.

6. Failure to add absolute ethanol to Buffer DW1/DW2Plus
Add the specified volume of absolute ethanol to Buffer DW1 and Buffer DW2Plus as indicated on the bottle labels.
Low DNA Purity
1. Contamination with foreign proteins
Buffer DW1 was not used for rinsing, or the correct volume of absolute ethanol was not added to Buffer DW1. Please add the specified volume of absolute ethanol according to the bottle label before operation.

2. Contamination with impurity ions
Buffer DW2Plus was not used for rinsing, or rinsed only once. Please rinse twice with Buffer DW2Plus according to the instruction manual.
Almacenamiento y envío
Condiciones de almacenamiento de almacenamiento
Room temperature
Enviado en
Normal
Estabilidad y almacenamiento
Store at room temperature long term (12 months).

Documentation

📋 Safety Data Sheet (SDS)

Comprehensive hazard, handling, storage, and regulatory compliance document.

Download SDS →

✅ Certificate of Analysis (COA)

Lot-specific quality data. Enter your lot number to retrieve the exact COA.

Look up COA →

📊 Datasheet

Quick-reference summary of product specifications and applications.

View datasheet →

🔬 Specification Sheet

Full quality attributes and acceptance criteria for this grade.

View spec sheet →

Advanced Data

Certificados (CoA, COO, BSE/TSE y tabla de análisis)
C of A & Other Certificates(BSE/TSE, COO):
Analytical Chart:

Find and download the COA for your product by matching the lot number on the packaging.

1 results found

Lot NumberCertificate TypeFechaArticulo
ZJ26F0333292Certificate of AnalysisMar 23, 2026 M665559
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