Sanshibio Agarose

$58.00

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.

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説明

製品導入

  • Support Material: Agarose serves as a common support material in gel electrophoresis.
  • Purity Impact: The purity of agarose directly influences the resolution of DNA bands and the clarity of electrophoresis results.
  • 準備: Agarose, a high-purity form of agar, is typically prepared as a gel with concentrations ranging from 0.5% に 2%.
  • アプリケーション: Agarose gel electrophoresis is utilized for the separation and identification of nucleic acids, including DNA profiling and DNA restriction enzyme mapping.
  • Visualization: Nucleic acid fluorescent dyes are added to the gel, and DNA bands are visualized using a gel imaging scanner post-electrophoresis.

商品内容:

コンポーネントDA003-02(100g)
Agarose100g

品質管理:

Parameter仕様
Gel Strength (1% gel)> 1200g/cm²
Electroendosmosis (EEO)< 0.15
Sulfate 0.15%
Gel Temperature (1.5% gel)35-37℃
Melting Temperature (1.5% gel)87-89℃
水分 10%

Absence of Nucleases.

Usage Instructions:

  • Depending on the size of the target nucleic acid fragments and the type of electrophoresis buffer, determine the required agarose concentration:
Agarose concentrationIdeal linear resolution range(bp)
1× TAE1× TBE
0.6%1200-150001200-12000
0.8%1000-100001000-12000
1.0%200-10000100-10000
1.2%100-8000100-5000
1.5%100-500050-3000
2.0%50-300050-3000
2.5%50-300050-2000
  • Agarose Gel Preparation (Horizontal Gel Electrophoresis Example):
  • Based on the amount of gel needed and the desired agarose concentration, 適切な量​​の電気泳動バッファーを測定します。 (TAE または TBE) そして三角フラスコに注ぎます.

注記: The buffer used for gel preparation should be the same as the electrophoresis buffer.

  • Accurately weigh the agarose and carefully add it to the triangular flask. Cover the flask opening with parchment paper and heat it in a microwave oven to dissolve the agarose. Heat the solution until it boils, then wearing heat-resistant gloves, gently swirl the flask. Repeat this process several times until the agarose is completely dissolved.

注記: Use multiple short boiling steps during the agarose dissolution to avoid overheating and boiling over. Ensure the agarose is fully dissolved to avoid blurry electrophoresis results.

  • Add nucleic acid dye to the fully dissolved agarose solution.
  • Pour the agarose solution into the gel mold, then insert the comb at the appropriate position. The gel thickness is usually between 3-5mm.
  • Let the gel solidify at room temperature (approximately 30 分まで 1 時間) and then place it in the electrophoresis apparatus for electrophoresis.

予防:

  1. Beware of boiling during the agarose dissolution process to prevent scalding.
  2. DA003-01 is a domestic proprietary brand, and DA003-02 is an imported reagent.
  3. Please wear gloves, especially when using fluorescent dyes with carcinogenic properties (such as ethidium bromide) for gel nucleic acid staining.
  4. If the prepared gel is not used immediately, store it submerged in electrophoresis buffer (TAE または TBE) に avoid gel drying out.

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