The process of extracting DNA from mouse tails or ears can be very time-consuming and requires a lot of labor. Specific applications, such as genotyping transgenic mice using a tail section, demand a lengthy DNA extraction method. Traditional methods involve a long process of digesting the tissue with proteinase K for several hours, followed by using chemicals like phenol and chloroform to extract the DNA and then precipitating it with alcohol. Recently, new techniques have emerged that use silica-based kits to purify DNA. These kits use high concentrations of a salt called guanidine hydrochloride to bind the DNA to silica. After binding, the DNA is washed with a solution of salt and ethanol to remove other substances from the sample, and then eluted with a buffer or water to obtain pure DNA. However, these methods can also be time-consuming and require multiple washing and spinning steps, which can result in DNA loss and shearing. Additionally, impurities can easily pass through the eluted DNA, affecting its purity and quantification, and potentially affecting downstream processes like PCR.