QIAquick Nucleotide Removal Kit

효소 반응에서 최대 10µg 올리고뉴클레오타이드(17~40mers) 및 DNA(40bp~10kb) 클린업에 사용합니다

✓ 연중무휴 하루 24시간 자동 온라인 주문 처리

✓ 풍부한 지식과 전문성을 갖춘 제품 및 기술 지원

✓ 신속하고 안정적인 (재)주문

QIAquick Nucleotide Removal Kit (250)

Cat. No. / ID: 28306

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

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QIAquick Nucleotide Removal Kit

QIAquick Spin Columns

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QIAquick Nucleotide Removal Kit은/는 분자생물학 분야에 사용하기 위한 것입니다. 이 제품은 질병의 진단, 예방, 또는 치료용이 아닙니다.

✓ 연중무휴 하루 24시간 자동 온라인 주문 처리

✓ 풍부한 지식과 전문성을 갖춘 제품 및 기술 지원

✓ 신속하고 안정적인 (재)주문

특징

바로 사용 가능한 DNA 최대 95% 회수
빠르고 편리한 절차
간단한 3단계로 최대 10kb의 DNA 클린업
편리한 샘플 분석을 위한 겔 로딩 염료

제품 세부 정보

QIAquick Nucleotide Removal Kit는 올리고뉴클레오타이드와 DNA의 실리카 막 기반 정제를 위한 스핀 컬럼, 완충액, collection 튜브를 제공합니다. 간단하고 빠른 결합-세척-용출 절차와 30~200µl의 용출량으로 미삽입 뉴클레오타이드, 염 및 기타 오염 물질을 제거하고 40bp~10kb 범위의 올리고뉴클레오타이드(>17nt)와 DNA 절편을 정제합니다. 해당 절차는 QIAcube Connect에서 완전히 자동화됩니다.

성능

QIAquick Nucleotide Removal 절차는 DNA 샘플에서 뉴클레오타이드, 효소, 염 및 기타 불순물을 제거합니다(그림 " 라벨링된 올리고에서 뉴클레오타이드 완전 제거" 참조). 마이크로 원심분리기를 사용하여 17mer – 10kb DNA를 정제합니다. 샘플 부피가 50µl 미만인 경우 DyeEx Spin kit도 사용할 수 있습니다.

그림 참조

라벨링된 올리고에서 뉴클레오타이드를 완전히 제거합니다.

원리

QIAquick Kit에는 염도가 높은 완충액에서 DNA를 결합하고 저염 완충액 또는 물로 용출하기 위한 실리카 막 어셈블리가 포함되어 있습니다. 정제 절차는 DNA 샘플에서 프라이머, 뉴클레오타이드, 효소, 미네랄 오일, 염, 아가로스, 브로민화 에티듐(ethidium bromide) 및 기타 불순물을 제거합니다(그림 " 라벨링된 올리고에서 뉴클레오타이드 완전 제거" 참조). 실리카 막 기술은 분산 수지 및 슬러리(slurry)와 관련된 문제와 불편을 해소합니다. 특수 결합 완충액은 각 응용 분야에 최적화되어 있으며 특정 크기 범위 내에서 DNA 분자를 선택적으로 흡착하도록 합니다.

겔 로딩 염료

더 빠르고 편리한 샘플 처리 및 분석을 위해 겔 로딩 염료가 제공됩니다. GelPilot 로딩 염료는 아가로스 겔 실행 시간을 최적화하고 작은 DNA 절편이 너무 멀리 이동하는 것을 방지하기 위해 세 가지 추적 염료(크실렌 시아놀, 브로모페놀 블루, 오렌지 G)를 함유하고 있습니다(그림 " GelPilot 로딩 염료" 참조).

그림 참조

라벨링된 올리고에서 뉴클레오타이드를 완전히 제거합니다.

GelPilot 로딩 염료.

절차

QIAquick system은 간단한 결합–세척–용출 절차를 사용합니다(순서도 " QIAquick Nucleotide Removal 절차" 참조). 결합 완충액을 샘플에 직접 첨가하고 혼합물을 QIAquick 스핀 컬럼에 적용합니다. 핵산은 완충액의 높은 염도 조건에서 실리카 막에 흡착됩니다. 불순물을 씻어내고 제공된 소량의 저염 완충액 또는 물로 순수한 DNA를 용출하여 모든 후속 응용 분야에 바로 사용할 수 있습니다.

취급

QIAquick 스핀 컬럼은 두 가지 편리한 취급 옵션을 제공하도록 고안되었습니다. 스핀 컬럼은 기존 탁상용 마이크로 원심분리기에 장착할 수 있습니다. QIAquick Nucleotide Removal Kit는 다른 QIAGEN 스핀 컬럼 기반 키트와 더불어 QIAcube Connect에서 완전히 자동화할 수 있어 생산성을 높이고 결과를 표준화할 수 있습니다(그림 "스핀 컬럼 취급 옵션 A" 및 " QIAcube Connect" 참조).

그림 참조

QIAquick Nucleotide Removal 절차.

스핀 컬럼 취급 옵션 — A.

QIAcube Connect.

응용 분야

QIAquick system으로 정제된 DNA 절편은 염기서열 분석, 마이크로어레이 분석, 결찰(ligation) 및 형질전환, 제한효소 처리(restriction digestion), 라벨링, 미세 주입을 포함한 모든 응용 분야에서 바로 사용할 수 있습니다.

지원되는 데이터 및 수치

QIAquick Nucleotide Removal 절차.

Specifications

Features	Specifications
Binding capacity	10µg
Technology	실리카 기술
Recovery: oligonucleotides dsDNA	회수: 올리고뉴클레오타이드, dsDNA
Format	튜브
Elution volume	30~50µl
Processing	수동
Sample type: applications	DNA, 올리고뉴클레오타이드: PCR 반응
Removal <10mers 17–40mers dye terminator proteins	<10mers 제거
Fragment size	40bp~10kb

리소스

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.

Publications

Effects of the chemotherapeutic agent doxorubicin on the protein C anticoagulant pathway.

Woodley-Cook J; Shin LY; Swystun L; Caruso S; Beaudin S; Liaw PC;

Mol Cancer Ther; 2006; 5 (12):3303-11 2006 Dec PMID:17172434

Differential effects of NF-kappaB on apoptosis induced by DNA-damaging agents: the type of DNA damage determines the final outcome.

Strozyk E; Pöppelmann B; Schwarz T; Kulms D;

Oncogene; 2006; 25 (47):6239-51 2006 May 15 PMID:16702954

Human enhancer of rudimentary is a molecular partner of PDIP46/SKAR, a protein interacting with DNA polymerase delta and S6K1 and regulating cell growth.

Smyk A; Szuminska M; Uniewicz KA; Graves LM; Kozlowski P;

FEBS J; 2006; 273 (20):4728-41 2006 Sep 19 PMID:16984396

Dual effects of plant steroidal alkaloids on Saccharomyces cerevisiae.

Simons V; Morrissey JP; Latijnhouwers M; Csukai M; Cleaver A; Yarrow C; Osbourn A;

Antimicrob Agents Chemother; 2006; 50 (8):2732-40 2006 Aug PMID:16870766

Autoregulation of the MisR/MisS two-component signal transduction system in Neisseria meningitidis.

Tzeng YL; Zhou X; Bao S; Zhao S; Noble C; Stephens DS;

J Bacteriol; 2006; 188 (14):5055-65 2006 Jul PMID:16816178

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