TGuide Blood Genomic DNA Kit

For extracting genomic DNA from human or mammalian whole blood.

TGuide Blood Genomic DNA kit is specially designed for extracting DNA (including genomic DNA, mitochondrial DNA and viral DNA) from whole blood, serum, plasma and leukocytes using TGuide Series Automated Nucleic Acid Extractor. Reagents required for cell lysis and protein degradation, the magnetic beads specifically adsorbing DNA, washing buffer, etc. are pre-packed in reagent cartridges. The purified DNA will be eluted in a low-salt buffer. The length of genomic DNA purified by the kit is 20- 30 kb, which is suitable for PCR or other enzymatic reactions.

Cat. No Packing Size
OSR-M102 48 preps
OSR-M102-T1 48 preps
OSR-M104 48 preps
OSR-M104-T1 48 preps

Product Detail

Product Tags

Applications

The purified genome can be directly used in PCR, RT-PCR, enzyme digestion reaction, Southern hybridization and other experiments.

Features

■ Simple and fast extraction: TGuide accessory products are based on the principle of nucleic acid purification by magnetic beads, and the genomic DNA extraction can be completed in 44 min.
■ Reliable results: The genomic DNA extracted by the kit has no impurities such as RNA and protein, and can be directly used for PCR or fluorescence quantitative PCR.
■ No phenol and chloroform extraction: No organic solvents harmful to human body such as phenol and chloroform are needed.
■ Flexible initial sample size: 200 μl, 400 μl, 1.2 ml of whole blood or 1-3 ml of pre-separated leukocyte can be directly extracted by selecting the corresponding kit.

All the products can be customized for ODM/OEM. For details, please click Customized Service(ODM/OEM)

Experimental Example 1

Experimental Example 2

Experimental Example 3

Experimental Example 1 Results of genomic DNA extracted from 200 μl whole blood treated with different anticoagulants
Experimental Example 1 DNA was dissolved in 200 μl elution buffer.
M: 1 kb ladder
1-5 Detection of inhibitors of different anticoagulants.
Target gene: Cbl-b gene, 1.7 kb
P: Positive control
Experimental Example 2 Results of genomic DNA extracted from 400 μl or 600 μl whole blood
Experimental Example 2 DNA was dissolved in 100 μl elution buffer
Genomic DNA extracted from 400 μl or 600 μl whole blood
M: DL15000 Marker
Loading volume: 2 μl
Experimental Example 3 Results of genomic DNA extracted from 1.2 ml whole blood
Experimental Example 4 DNA was dissolved in 300 μl elution buffer
Genomic DNA extracted from 1.2 ml whole blood
M: DL15000 Marker;
Loading volume: 2 μl

FAQ

Q: Little or no DNA in the eluent.

A-1 Low concentration of cells or virus in the starting sample —Enrich the concentration of cells or viruses.

A-2 Insufficient lysis of the samples —The samples has not been mixed thoroughly with the lysis buffer. It is suggested to thoroughly mix by pulse-vortexing for 1-2 times. —Insufficient cell lysis caused by the activity decrease of proteinase K. —Insufficient cell lysis or protein degradation due to insufficient warm bath time. It is suggested to cut the tissue into small pieces and extend the bath time to remove all the residue in the lysate.

A-3 Insufficient DNA adsorption. —No ethanol or low-percentage instead of 100% ethanol was added before the lysate was transfer to the spin column.

A-4 The pH value of elution buffer is too low. —Adjust the pH to between 8.0-8.3.

Q: DNA does not perform well in downstream enzymatic reaction experiments.

Residual ethanol in the eluent.

—There is residual washing buffer PW in the eluent. The ethanol can be removed by centrifuging the spin column for 3-5 min, and then placing at room temperature or 50℃ incubator for 1-2 min.

Q: DNA degradation

A-1 The sample is not fresh. —Extract a positive sample DNA as control to determine whether the DNA in the sample has degraded.

A-2 Improper pre-treatment. —Caused by excessive liquid nitrogen grinding, moisture regaining, or too large amount of the sample.

Q: How to perform the pretreatment for gDNA extraction?

The pretreatments should vary for different samples. For plant samples, make sure to thoroughly grind in liquid nitrogen. For animal samples, homogenate or thoroughly grind in liquid nitrogen. For samples with cell walls that are hard to break, such as G+ bacteria and yeast, it is suggested to use lysozyme, lyticase or mechanical methods to break the cell walls.

Q: What is the difference between the three plant gDNA extraction kits 4992201/4992202, 4992724/4992725, 4992709/4992710?

4992201/4992202 Plant Genomic DNA Kit adopts a column-based method that requires chloroform for the extraction. It is especially suitable for various plant samples, as well as plant dry powder. Hi-DNAsecure Plant Kit is also column-based, but with no need of phenol/chloroform extraction, making it safe and non-toxic. It is suitable for plants with high polysaccharides and polyphenol content. 4992709/4992710 DNAquick Plant System adopts a liquid-based method. Phenol/chloroform extraction is not needed as well. The purification procedure is simple and fast with no limit for the sample start amounts, so users can adjust the amount flexibly according to the experimental requirements. Large size of gDNA fragments can be obtained with high yield.

What's the estimated yield of gDNA from 1 ml blood sample by TIANamp Blood DNA Kit?

The genomic DNA was extracted from different volumes of human whole blood samples by TIANamp Blood DNA Kit. The results are as follow. The results are listed as reference only, the actual extraction results depends on the conditions of samples.

faq

Q: Can 4992207/4992208 and 4992722/4992723 be used to extract blood clots DNA?

The blood clot DNA extraction can be performed using the reagents provided in these two kits by simply changing the protocol to the specific instruction for the blood clot DNA extraction. The soft copy of the blood clot DNA extraction protocol can be issued upon requesting.

Q: When applying TIANamp Genomic DNA Kit, how to break the fresh tissues into cell suspension?

Suspend the fresh sample with 1 ml PBS, normal saline or TE buffer. Completely homogenize the sample by a homogenizer and collect the precipitate to the bottom of a tube by centrifuging. Dispose the supernatant, and resuspend the precipitate with 200 μl buffer GA. The following DNA purification can be performed according to the instruction.

Q: How to choose the product for the DNA extraction from plasma, serum and body fluid samples?

For the purification of gDNA in plasma, serum and body fluid samples, TIANamp Micro DNA Kit is recommended. For the purification of virus gDNA from serum/plasma samples, TIANamp Virus DNA/RNA Kit is recommended. For the purification of bacterial gDNA from serum and plasma samples, TIANamp Bacteria DNA Kit is recommended (lysozyme should be included for positive bacterial). For saliva samples, Hi-Swab DNA Kit and TIANamp Bacteria DNA Kit are recommended.

Q: How to choose the kits for the gDNA extraction from fungi samples?

DNAsecure Plant Kit or DNAquick Plant System are recommended for fungal genome extraction. For yeast genome extraction, TIANamp Yeast DNA Kit is recommended (lyticase should be self-prepared).


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