土壌ゲノムDNA抽出キット
土壌ゲノムDNA抽出キット

Solarbio土壌ゲノムDNA抽出キット

から$121.00

送料USD 45 - 米ドル以上は無料 300

DTE は、分子検査のオンライン販売に特化した中国に拠点を置く電子商取引プラットフォームです, エリサ, および関連製品.

  • メーカー: 中国の一流ブランド
  • 配送: 工場から直接FedExで迅速に発送
  • 以内であれば返品または交換が可能です 30 日々
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説明

属性 詳細
カタログ番号. D2600
パッケージ 50T/100T
ストレージ At room temperature (15℃-25℃) のための乾燥した場所で 1 年

キット内容

成分 D2600-50T D2600-100T
Solution A 25 ミリリットル 50 ミリリットル
Solution B 3 ミリリットル 6 ミリリットル
Solution C 5 ミリリットル 10 ミリリットル
Solution D 10 ミリリットル 20 ミリリットル
Washing Buffer 15 ミリリットル 15 ml × 2
溶出バッファー 15 ミリリットル 15 ml × 2
Adsorption Column 50 Units 100 Units
Collection Tube 50 Units 100 Units
PCR Enhancer 500 ul 1 ミリリットル
命令 1 Piece 1 Piece

注記: Once opened, Solution A, B, C, D should be kept at 2-8℃. PCR Enhancer should be kept at -20℃.

製品説明

  • Suitability and Efficacy:
    • 土壌 ゲノムDNA抽出 Kit is ideal for extracting microbial DNA from extreme soil environments like cinnamon soil, mud, volcanic ash, 等.
    • It effectively lyses bacteria and fungi, preserving microbial DNA diversity.
  • Humus Removal:
    • Utilizes unique humus adsorption material to efficiently and specifically remove various humus components.
    • This process doesn’t compromise yield, and purity is significantly higher compared to the phenol-chloroform extraction method.
  • DNA Yield and Integrity:
    • Extracted DNA yields are substantial, and integrity is well maintained.
    • The extracted DNA is suitable for various routine operations, including enzyme digestion, PCR, library construction, Southern blot, 等.

プロトコル

Add fresh opened absolute ethanol in the Washing Buffer before use, volume is based on the label of the bottle as a reference. Put the cap back on the bottle and shake well. All centrifuge steps are performed at room temperature (15℃-25℃).

  1. Method A: Weigh soil sample 0.1-0.5g, add soil into the mortar, pour the proper amount of liquid nitrogen, grind immediately, and repeat three times. When the soil turns into powder, add 450ul Solution A, and keep shaking for 1-2min until the solute is completely suspended.

Method B: Weigh soil sample 0.1-0.5g in centrifuge tube (it is better to use 2ml round bottom), add 450ul Solution A, and keep shaking for 1-2min until solute is completely suspended. 注記: The effect of grinding with liquid nitrogen will be better.

  1. Add 50ul Solution B, and invert the tube several times to mix fully (don’t shake violently). Incubate at 65℃ water bath for 6 分, 反転, and mix each 2 分.
  2. Add 100ul Solution C, and invert the tube several times to mix fully (don’t shake violently). で遠心分離します。, 12000の回転数 10 分.
  3. Transfer supernatant to a new centrifuge tube, で遠心分離する, 12000の回転数 10 分.
  4. Add 200ul Solution D to the Adsorption Column, add supernatant centrifuged from step 4 to the Adsorption Column, mixed fully by pipette. Centrifuge at 12000rpm for 1 分.
  5. Mix filtrate in Collection Tube fully, add it into Adsorption Column, and centrifuge at 12000rpm for 1 分.
  6. Remove waste liquid in the Collection Tube, add 500ul Washing Buffer in the Adsorption Column, and centrifuge at 12000rpm for 10 分.
  7. ステップを繰り返します 7 twice (wash three times in total).
  8. Remove waste liquid in the Collection Tube, put the Adsorption Column back into the Collection Tube, and centrifuge at 12000rpm for 2 分.
  9. Dry the Adsorption Column at room temperature(15℃-25℃) for a few minutes or at 50℃ for 1 分.
  10. Put the Adsorption Column in a new centrifuge tube, add 50-100ul Washing Buffer (preheat at 65℃ before use), and centrifuge at 12000rpm for 1 分.
  11. Add filtrate in the centrifuge tube to the Adsorption Column, centrifuge at 12000rpm for 1 分. Liquid in the centrifuge tube is soil genomic DNA extraction solution.
  12. If the PCR effect of DNA is not good, properly dilute DNA concentration or add 1/10 volume of PCR enhancer.

ノート

  1. Fresh soil samples will get a higher yield. And it is better to refer to proper preservation conditions for different samples.
  2. If the solution shows precipitation, redissolve at 37℃ water bath for a moment, precipitation will disappear, and it does not affect DNA extraction.
  3. When taking supernatant, it should avoid taking precipitation, さもないと, it will block the absorption column and affect the purity of the product.
  4. Volume of the Elution buffer shouldn’t be less than 50ul, if the volume is too small, it will affect recovery It is suggested to use the Elution buffer provided with the kit, using water as an Elution buffer will lose a part of the DNA. Extracted DNA should be stored at -20℃ and avoid repeated freeze-thaw cycles to prevent DNA degradation.
  5. If the product contains residual humus, it will seriously affect DNA absorbance, so it should be identified by a combination of electrophoresis detection and spectrophotometer
  6. Avoid touching liquid reagents, in case of accidental contact, rinse immediately with plenty of water.

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  • D1010 6×DNA Loading Buffer
  • G8142 GoldView II Nuclear Staining Dyes (5000×)
  • D1500 Plant Genomic DNA Extraction Kit
  • D1600 Bacterial Genomic DNA Extraction Kit
  • D1700 Animal Tissues/Cells Genomic DNA Extraction Kit D1800 Blood Genomic DNA Extraction Kit (Spin column)

追加情報

サイズ

50T, 100T

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