QIAquick Nucleotide Removal Kit

酵素反応液から最高10 µgまでのヌクレオチド（17～40 mer）およびDNA（40 bp～10 kb）をクリーンアップ

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QIAquick Nucleotide Removal Kit (250)

Cat. No. / ID: 28306

250 QIAquick Spin Columns, Buffers, Collection Tubes (2 ml)

￥66,000

KitColumn

QIAquick Nucleotide Removal Kit

QIAquick Spin Columns

QIAquick Nucleotide Removal Kitは分子生物学的アプリケーション用であり、疾病の診断、予防、あるいは治療に使用することはできません。

✓ オンライン注文による24時間年中無休の自動処理システム

✓ 知識豊富で専門的な製品&テクニカルサポート

✓ 迅速で信頼性の高い（再）注文

特徴

即使用可能なDNAの回収率が最高95％
迅速で簡便な操作
簡単な3ステップで最大10 kbまでのDNAをクリーンアップ
ゲル解析をより簡便化するGel Loading Dye付き

製品詳細

QIAquick Nucleotide Removal Kitは、スピンカラム、バッファー、コレクションチューブから構成され、シリカメンブレンによりオリゴヌクレオチドおよびDNAの精製を実現します。未反応のヌクレオチド、塩類、その他の夾雑物が除去され、迅速で簡便な結合・洗浄・溶出ステップと30～200 µlの溶出液により、オリゴヌクレオチド（17 nt以上）およびDNA（40 bp～10 kb）を精製できます。本キットは、QIAcubeで完全に自動化できます。

パフォーマンス

QIAquick Nucleotide Removal を用いて、DNAサンプルからヌクレオチド、酵素、塩類などの夾雑物を除去できます（図 ""）。マイクロ遠心機を使用することにより、17 mer～10 kbのDNAが精製されます。サンプル量が50 µl 以下の場合には、 DyeEx Spin Kitを使用可能です。

図参照

Complete removal of nucleotides from labeled oligos.

原理

QIAquick Kitでは、高塩濃度バッファーによりDNAを結合し、低塩濃度バッファーあるいは水によりDNAを溶出するシリカゲルメンブレンを利用しています。この精製法でDNAサンプルからプライマー、ヌクレオチド、酵素、ミネラルオイル、塩、アガロース、臭化エチジウム、およびその他の夾雑物が除去できます（図" 標識オリゴからのヌクレオチドの完全な除去"）。シリカメンブレンテクノロジーにより樹脂漏れ、および懸濁液関連の問題や不便さは解消されます。それぞれの用途に応じて至適化された結合バッファーにより、種々の大きさのDNAフラグメントを選択的に吸着します。

Gel Loading Dye

GelPilot Loading Dye は3 種類のマーカー色素（xylene cyanol、bromophenol blueおよびorange G）が入っており、短いDNAフラグメントのゲルからの流出を回避でき、アガロースゲルの泳動時間の至適化が簡単に行なえます（図 " GelPilot Loading Dye"）。

図参照

Complete removal of nucleotides from labeled oligos.

GelPilot Loading Dye.

操作手順

QIAquickシステムでは結合－洗浄－溶出という簡単な操作だけでDNAのクリーンアップが可能です（フローチャート" QIAquick Nucleotide Removal 操作手順"参照）。結合バッファーを直接サンプルに添加し、混合液を QIAquick Spin Column にアプライします。DNAは添付のバッファー中の高塩濃度の条件下でシリカゲルメンブレンに吸着します。不純物は洗い流され、純粋なDNAを添付の低塩濃度溶出バッファー、あるいは水で溶出します。得られたDNAは、幅広いアプリケーションに即使用可能です。

操作法

QIAquick Spin Column は2つの簡便な操作法オプションのためにデザインされました。スピンカラムは、簡便な卓上型マイクロ遠心機で使用することができます。QIAquick Nucleotide Removal Kitは、スピンカラム法を用いた他のQIAGEN Kit と同様にQIAcube上での完全自動化が可能で、生産性を高め、得られる結果を標準化することができます（図 "Spin Column操作オプション Aおよび B"）。

図参照

QIAquick Nucleotide Removal procedure.

Spin column handling options — A.

Spin column handling options — B.

アプリケーション

QIAquickシステムを用いて精製したDNAは、シークエンシング、マイクロアレイ解析、ライゲーションおよびトランスフォーメーション、制限酵素分解、標識反応、マイクロインジェクションなどのほとんどのアプリケーションに直接使用できます。

裏付けデータと数値

QIAquick Nucleotide Removal procedure.

Specifications

Features	Specifications
Binding capacity	10 µg
Technology	Silica technology
Recovery: oligonucleotides dsDNA	Recovery: oligonucleotides, dsDNA
Format	Tube
Elution volume	30–50 µl
Processing	Manual
Sample type: applications	DNA, oligonucleotides: PCR reactions
Removal <10mers 17–40mers dye terminator proteins	Removal <10mers
Fragment size	40 bp – 10 kb

リソース

QIAquick® Spin Columns can now be used on any vacuum manifold with luer connectors, for example, the QIAvac 6S or QIAvac 24 with QIAvac Luer Adapters. This protocol is designed for removal of primers <10 bases, enzymes, salts, and unincorporated nucleotides from biotin-, or DIG-labeled DNA fragments and oligonucleotides >17 nucleotides.

Download Safety Data Sheets for QIAGEN product components.

FAQ

Larger DNA fragments bind more tightly to the QIAquick columns. It is difficult to predict whether a DNA fragment larger than 10 kb can be efficiently recovered, because this depends on base composition as well as fragment size. If the fragment is only a few kb larger than the 10 kb limit, it can be helpful to heat the elution buffer EB to 60°C and let it incubate on the column for a few minutes before centrifuging. However, please note that it will become less likely to recover your sample the larger the fragment size is. As we cannot guarantee recovery of fragments larger than the maximum cutoff size, we do not recommend to purify such fragments using QIAquick Kits.

The QIAEX II Kit can be used to extract DNA fragments up to 50 kb from agarose or polyacrylamide gels.

FAQ ID -756

Yes - all QIAquick Spin Kits contain identical columns, but different binding buffers optimized for each specific application.

FAQ ID -577

Buffer PE did not contain ethanol

Ethanol must be added to Buffer PE (concentrate) before use. Repeat procedure with correctly prepared Buffer PE.

Inappropriate elution buffer

DNA will only be eluted efficiently in the presence of low-salt buffer (e.g., Buffer EB: 10 mM Tris·Cl, pH 8.5) or water. Elution efficiency is strongly dependent on the salt concentration and pH of the elution buffer. Contrary to adsorption, elution is most efficient under basic conditions and low salt concentrations. DNA is eluted with 50 or 30 µl of the provided Buffer EB (10 mM Tris·Cl, pH 8.5), or water. The maximum elution efficiency is achieved between pH 7.0 and 8.5. When using water to elute, make sure that the pH is within this range. In addition, DNA must be stored at –20°C when eluted with water since DNA may degrade in the absence of a buffering agent. Elution with TE (10 mM Tris·Cl, 1 mM EDTA, pH 8.0) is possible, but not recommended because EDTA may inhibit subsequent enzymatic reactions.

Elution buffer incorrectly dispensed

Add elution buffer to the center of the QIAquick membrane to ensure that the buffer completely covers the membrane. This is particularly important when using small elution volumes (30 µl).

FAQ ID -180

Although it is possible to use the QIAquick Nucleotide Removal Kit and QIAquick PCR Purification Kit for RNA purification, the conditions are not optimized for RNA, nor are RNase-free conditions guaranteed. The RNeasy MinElute Cleanup Kit is recommended for clean-up, concentration and desalting of RNAs above 200 bases in length.

FAQ ID -490

Add 1/10 volume of 3 M Na-Acetate pH 5.2, and 2 to 2.5 volumes of ice-cold 100% ethanol to the DNA sample
Mix, and store at –20°C for at least 1 h to precipitate the DNA
Recover the precipitated DNA by centrifugation at full speed in a microcentrifuge for 15–20 min
Pour off the ethanol and wash the pellet twice with room-temperature 70% ethanol
Allow the DNA pellet to air-dry
resuspend the DNA in a suitable volume of sterile TE buffer or distilled water

FAQ ID -305

Yes, please follow the Supplementary Protocol 'Cleanup of nonradioactive samples using the QIAquick Nucleotide Removal Kit' (QQ04).

FAQ ID -945

DNA fragments purified with the QIAGEN DNA Cleanup Systems, i.e., the QIAquick PCR Purification Kit, the MinElute Reaction Cleanup Kit, the QIAEX II Gel Extraction Kit etc. may float out of the loading wells of agarose gels due to residual ethanol carried over from the wash step with Buffer PE (despite the addtition of glycerol-containing loading buffer).

Use either of the following options to remove residual ethanol from the eluate:

re-purify the sample using a QIAquick-, or MinElute column, or QIAEX II resin
incubate the eluate at 56°C for 10 min to evaporate the ethanol
dry down the sample in a vacuum centrifuge, and resuspend the pellet in a small volume of sterile water

FAQ ID -205

Yes, bisulfite containing methylation reactions can be cleaned up with our silica-based cleanup products, such as QIAquick and QIAEX II. Please see Goyon et al. (1994), 'Perpetuation of cytosine methylation in Ascobolus immersus implies a novel type of maintenance methylase', published in J Mol Biol. 1994 Jul 1;240(1):42-51, for a reference.

FAQ ID -519

As a rule of thumb, single-stranded DNA binds to silica with approximately half the affinity of a double-stranded DNA fragment of the same length under the buffer conditions used in the QIAquick and MinElute Kits. Even though no systematic experimental data exists, we expect that recovery of ssDNA fragments of approximately 200 nucleotides and below will not be very efficient after cleanup using the QIAquick PCR Purification Kit or MinElute PCR Purification Kit. By comparison, it should be possible to purify fragments longer than 140 nucleotides using the QIAquick Gel Extraction Kit.

Note that recovery of single strand DNA is influenced to some degree also by factors such as base composition and secondary structure. It has to be determined empirically by the researcher if cleanup of single-stranded DNA with QIAquick columns yields satisfactory results.

FAQ ID -759

The composition of Buffer EB is:

10 mM Tris-Cl, pH 8.5

Buffer EB is the elution buffer used in the QIAquick PCR, Gel Extraction, Nucleotide Removal Kits, and MinElute Kits for DNA cleanup, and the QIAprep Miniprep Kits for small-scale plasmid purification. The purified DNA can also be eluted in TE (10 mM Tris-Cl, 1 mM EDTA, pH 8.0), but the EDTA may inhibit subsequent enzymatic reactions.

FAQ ID -199

Occasionally, DNA fragments eluted from the silica matrix of QIAquick, MinElute or QIAEX II Kits will contain denatured single-stranded DNA (ssDNA), appearing as a smaller band on an analytical gel. Under certain conditions, chaotropic agents (present in all silica-based DNA purification methods) can denature DNA fragments. This is a rare event that may be influenced by sequence characteristics such as the presence of inverted repeats or A–T-rich stretches.

Because salt and buffering agents promote renaturation of DNA strands, the following tips are recommended:

use the eluted DNA to prepare your downstream enzymatic reaction, but omit the enzyme. Incubate the reaction mix at 95°C for 2 minutes to reanneal the ssDNA, and allow the tube to cool slowly to room temperature before adding the enzyme and proceeding
alternatively, the DNA can be eluted from the silica-gel membrane or resin in 10 mM Tris buffer containing 10 mM NaCl. However, the salt concentration of the eluate must then be taken into consideration in downstream applications.

FAQ ID -148

The QIAquick Spin Columns (100) (cat. no. 28115) in the QIAquick PCR Purification, Gel Extraction, Nucleotide Removal and PCR & Gel Cleanup kits are also sold separately from the kits.

The MinElute columns in the MinElute PCR Purification, Gel Extraction and Reaction Cleanup kits are not sold separately.

We always provide extra buffers in our kits so you can scale up reactions, add extra washes or allow for spillage.

FAQ ID -2460