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DNeasy PoweRSiofilm Kit

バイオフィルムサンプルから高純度なDNAを単離

Features

  • バイオフィルムサンプルから高収量にDNA単離
  • インヒビター除去技術(IRT)により、様々なアプリケーションに対応する高品質のDNAを精製
  • 歯垢および微生物マットを含むすべてのバイオフィルムからのDNA単離に最適
• • •

Useful Resources

DNeasy PowerBiofilm Quick Start Protocol DNeasy PowerBiofilm Kit Handbook
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DNeasy PowerBiofilm Sample (2)

Cat. No. / ID: 24000-S

Isolate high-quality, pure DNA from biofilm samples.
Size
DNeasy PowerBiofilm Sample (2)
DNeasy PowerBiofilm Kit (50)
DNeasy PoweRSiofilm Kit  は分子生物学実験用です。疾病の診断、治療または予防の目的に使用することはできません。

Product Details

DNeasy PowerBiofilm Kitは、化学的および機械的な溶解技術とインヒビター除去技術(IRT)を組み合わせることにより、最も困難なバイオフィルムにおける非効率的な細胞溶解という問題点を解決しました。 IRTは、フミン酸、金属、塩および農薬などバイオフィルムに存在する典型的な濃縮された阻害物質を除去し、微生物マットを含むあらゆるタイプのバイオフィルムから これらを含まないDNAを効率的に単離することを可能にしました。

DNeasy PowerBiofilm Kitは、MOBIO社よりPowerBiofilm DNA Isolation Kitとして販売されていた製品です。

Performance



Supporting data and figures

Figure 1: High-quality biofilm DNA isolated from a range of locations.

Biofilm DNA was isolated from a variety of locations. NanoDrop provided DNA yield. Agarose gel (1.2%) was used to assess quality. Each biofilm sample provided high-quality, high yield DNA when processed with the DNeasy PowerBiofilm Kit.
Figure 1: High-quality biofilm DNA isolated from a range of locations.
Figure 1: High-quality biofilm DNA isolated from a range of locations.
Figure 3: PCR-ready DNA from any biofilm.
Figure 2: Pure DNA from stream biofilm.

Specifications

FeaturesSpecifications
format
processing
samplesize
bindingcapacity
throughput
timeperrunorperprep
storagetemperature
sampletypes
beadsize

Resources

クイックスタートプロトコール (1)
DNeasy PowerBiofilm Quick Start Protocol
PDF (393KB)
キットハンドブック (1)
DNeasy PowerBiofilm Kit Handbook
PDF (513KB)

FAQ

Are there important considerations for plasma generation and urine handling?

It is strongly advised to follow the recommendations for preparing sample material provided in the corresponding Protocol Sheet to ensure reliable results.

Plasma: It is recommended to perform plasma separation immediately after blood collection when using EDTA or citrate as anticoagulant to prevent the release of genomic DNA into the plasma fraction.

Urine: Because circulating cell-free DNA in non-stabilized urine samples is rapidly degraded after sample collection due to high nuclease activity, eluates may contain no DNA or exhibit low DNA concentration. Therefore, it is recommended to stabilize urine samples. Even when using stabilized urine, it is recommended to perform a centrifugation step immediately after stabilization to prevent the release of genomic DNA from cells. Alternatively, non-stabilized urine samples can be processed immediately after collection and centrifugation using ATL-pretreatment and automated DNA extraction as described in the corresponding Protocol Sheet.

FAQ ID - 3699

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