원칙

1. 용해 및 소화: Begin by lysing and digesting the sample using a specialized lysate and protease combination. This step facilitates the release of DNA into the lysate, preparing it for the purification process.
2. Adsorption Column: Transfer the lysate mixture to an adsorption column. 여기, the nucleic acid selectively adheres to the silica membrane, while proteins and other contaminants remain unadsorbed. This selective binding ensures the efficient removal of impurities.
3. Filtration: Employ filtration to efficiently remove the unadsorbed proteins and other contaminants from the mixture. This step further enhances the purity of the nucleic acid sample.
4. Thorough Washing: Perform a thorough washing step to eliminate any remaining proteins and impurities, ensuring the purity of the nucleic acid sample.
5. 용출: 마지막으로, elute the purified nucleic acid from the adsorption column using a low-salt buffer solution (10mm 트리스, pH 9.0, 0.5mm EDTA). This gentle elution process preserves the integrity of the DNA, readying it for downstream applications.

• 다재: Suitable for a diverse range of downstream applications, PCR을 포함하여, qPCR, 효소 소화, 이종 교잡, 그리고 더. Whether you’re performing basic research or advanced molecular assays, our DNA meets your requirements.
• 능률: Accelerate your workflow with fast DNA extraction. Say goodbye to time-consuming processes like leukocyte separation, 유기 추출, 또는 에탄올 침전. Our method streamlines the extraction process for swift results.
• Simplicity: Enjoy a straightforward extraction process. No complex steps or specialized equipment are required. Obtain all nucleic acids directly through simple digestion, saving you time and effort in the lab.
• Broad Applicability: Our DNA extraction method is versatile and adaptable. It can handle various sample types, including liquid samples, animal tissues, 및 배양된 세포. Whether you’re working with blood, 조직, or cell cultures, our method delivers consistent results across different sample types.

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