性猛交XXXX乱大交派对,四虎影视WWW在线观看免费 ,137最大但人文艺术摄影,联系附近成熟妇女

上海易匯生物科技有限公司

當前位置:上海易匯生物科技有限公司>>代理品牌>>qiagen>>qiagen REPLI-g Mini Kit Print 國內(nèi)現(xiàn)貨

qiagen REPLI-g Mini Kit Print 國內(nèi)現(xiàn)貨

參   考   價:面議
具體成交價以合同協(xié)議為準

產(chǎn)品型號:

品       牌:其他品牌

廠商性質(zhì):生產(chǎn)商

所  在  地:上海市

更新時間:2019-12-19 16:59:20瀏覽次數(shù):1953

聯(lián)系我時,請告知來自 化工儀器網(wǎng)
供貨周期 現(xiàn)貨 應(yīng)用領(lǐng)域 醫(yī)療衛(wèi)生,環(huán)保,食品,化工,生物產(chǎn)業(yè)
上海易匯生物科技有限公司 Qiagen凱杰銷售銷售338906Qiagen銷售銷售凱杰銷售銷售
QIAGEN是*的樣本制備和分析技術(shù)的供應(yīng)商。樣品制備技術(shù)用來分離和處理從血液或組織等樣品中提取的DNA 、RNA和蛋白,而分析技術(shù)使這些分離的分子可被檢測,便于生物學(xué)研究和疾病檢測。
qiagen REPLI-g Mini Kit Print 國內(nèi)現(xiàn)貨

qiagen REPLI-g Mini Kit Print 國內(nèi)現(xiàn)貨

qiagen REPLI-g Mini Kit Print 國內(nèi)現(xiàn)貨

qiagen REPLI-g Mini Kit Print 國內(nèi)現(xiàn)貨

For highly uniform whole genome amplification from small or precious samples

  • Easy amplification with consistent yields of up to 10 µg
  • Unbiased amplification of genomic loci
  • Reliable results due to Multiple Displacement Amplification (MDA)
  • Amplified DNA highly suitable for most downstream applications
  • No risk of DNA degradation during long-term storage

The REPLI-g Mini Kit provides optimized reagents for whole genome amplification (WGA) from small samples using innovative Multiple Displacement Amplification (MDA) technology. The typical DNA yield of a 50 μl reaction is  up to 10 μg, with an average product length greater than 10 kb (ranging between 2 kb and 100 kb). Unique REPLI-g technology delivers highly uniform WGA from a variety of small or precious sample types, including purified genomic DNA, or directly from fresh or dried blood, buccal swabs, fresh or frozen tissue, and cells. This simple and reliable method is capable of accurate and unbiased amplification of genomes and generates DNA that can be applied without further purification or quantification for downstream applications that do not require labeling. In contrast to PCR-based WGA technologies, high fidelity rates are increased up to 1000-fold, avoiding costly false positive or negative results.

The REPLI-g Mini Kit is intended for molecular biology applications. This product is not intended for the diagnosis, prevention, or treatment of a disease.

See trademarks.

 

  • Consistent DNA yields using any sample type.

  • <p>Effect of heat and alkaline denaturation on loci representation.</p>

  • <p>Consistent long-term stability.</p>

  • <p>Comparable NGS (next-generation sequencing) results obtained using purified gDNA or REPLI-g amplified DNA.</p>

  • <p>REPLI-g Mini and Midi procedure.</p>

  • Accurate genotyping.

  • Schematic representation of REPLI-g amplification.

  • <p>Unbiased amplification with Phi29 polymerase.</p>

  • Highly representative amplification.

  • Consistent and accurate whole genome amplification.

  • Uniform DNA yield from various amounts of template.

Unbiased amplification with Phi29 polymerase.

[A] Upon encountering secondary DNA structures, Taq polymerase may pause synthesis, slip, or dissociate from the template. This can result in inaccurate DNA amplification, incomplete loci coverage, and short fragment sizes. [B] REPLI-g Kits utilize Phi29 polymerase, which displaces secondary structures enabling accurate and highly uniform amplification of the entire genome.

Performance

High yields from a variety of samples, suitable for numerous applications

With the REPLI-g Mini Kit, various clinical and non-clinical research samples can be used, including genomic DNA, fresh or dried blood, fresh or frozen tissue, and cells. Typical DNA yields per 50 µl reaction consistently reach 10 µg (see figure "Consistent DNA yields using any sample type"), while a uniform yield of amplified DNA is usually achieved regardless of the quantity of template DNA (see figure "Uniform DNA yield from various amounts of template"). Obtaining uniform DNA yields from varying template concentrations is always important, but particularly essential for high-throughput applications, which require subsequent genetic analyses to be possible without additional measurement or adjustment of DNA concentration.

The average product length of REPLI-g amplified DNA is typically more than 10 kb, with a range between 2 kb and 100 kb, enabling downstream applications such as complex restriction enzyme analysis and long-range PCR to be carried out. REPLI-g amplified DNA is highly suited for genotyping applications, such as SNP genotyping with TaqMan® primer/probe sets (see figure "Reliable SNP genotyping "), sequencing, and STR/microsatellite analysis (see figure "Accurate genotyping").

Successfully used in next-generation sequencing

Numerous publications have demonstrated the successful utilization of REPLI-g amplified DNA for next-generation sequencing (NGS) applications that range from exome and whole genome sequencing of tumor cells, to metagenomics research, to single cell analysis (for a range of recent publications that successfully used REPLI-g in NGS, please see our WGA resource page). Since the use of whole genome amplified DNA for NGS and array applications has been debated, we detected potential factors that could influence the success of using amplified DNA for these downstream applications. We determined that the quality of input material strongly influences the success of downstream NGS experiments. If working with low quality DNA (e.g., degraded DNA) or aged tissue material, the resulting amplified DNA may not give reliable results (data not shown). However, WGA, using REPLI-g technology, on intact cells or non-degraded purified DNA shows that NGS results are comparable to those obtained with purified gDNA. Sequence coverage and alignment comparison of the genomic loci sequence indicates minimized levels of junk DNA after WGA, whereas error rates are in a similar percentage range for both amplified and genomic DNA(see figure “Comparable NGS (next-generation sequencing) results obtained using purified gDNA or REPLI-g amplified DNA”).

High fidelity whole genome amplification

REPLI-g technology provides highly uniform DNA amplification across the entire genome. Phi29 polymerase can replicate up to 70 kb without dissociating from the genomic DNA template (see figure "Schematic representation of REPLI-g amplification"). In contrast to PCR-based whole genome amplification (WGA) technologies, Phi29 polymerase has 3'→5' exonuclease proofreading activity and maintains up to 1000-fold higher fidelity compared to Taq DNA polymerase during replication. Exonuclease-resistant primers provided in the kit ensure high yields of DNA product, and the WGA buffer system is optimized for very long read length and unbiased locus representation.

REPLI-g outperforms PCR-based WGA methods

 

Traditional methods of genomic DNA amplification include the time-consuming process of creating EBV-transformed cell lines followed by whole genome amplification using random or degenerate oligonucleotide-primed PCR. Also, PCR-based methods (e.g., DOP-PCR and PEP), as generally used by other suppliers, can produce nonspecific amplification artifacts and give incomplete coverage of loci. In several cases, DNA less than 1 kb long may be generated that cannot be used in many downstream applications. In general, the resulting DNA is generated with a much higher mutation rate due to the use of the low-fidelity enzyme Taq DNA polymerase, which can lead to error-prone amplification that results in, for example, single base-pair mutations, STR contractions, and expansions. In contrast to these disadvantages, REPLI-g provides highly uniform amplification across the entire genome, with minimal locus bias and minimized mutation rates during amplification (see figures "Highly representative amplification using REPLI-g technology" and "Consistent and accurate whole genome amplification").

Principle

Unique REPLI-g technology uses the innovative, high-fidelity enzyme Phi 29 polymerase to amplify complex genomic DNA using Multiple Displacement Amplification (MDA) combined with a gentle alkaline denaturation step to amplify genomic loci uniformly. The typical yield of the REPLI-g Mini Kit is up to 10 µg, and can be easily scaled down according to your needs with the REPLI-g Midi Kit, since both kits are based on the same protocol and use the same reaction volumes. The easy reaction set-up and very low handling time of approximately 15 minutes makes REPLI-g an easy and reliable method to use when complete and unbiased locus representation is needed from limited or precious samples.

Amplification principle

REPLI-g uses isothermal genome amplification, termed Multiple Displacement Amplification (MDA), which involves the binding of random hexamers to denatured DNA followed by strand displacement synthesis at a constant temperature with the enzyme Phi29 polymerase. Additional priming events occur on each displaced strand that serve as a template, enabling generation of high yields of amplified DNA (see figure “Schematic representation of REPLI-g amplification”). Phi 29 polymerase, a phage derived enzyme, is a DNA polymerase with 3'→5' prime exonuclease activity (proofreading activity) that delivers up to 1000-fold higher fidelity compared to Taq DNA polymerase. Supported by the unique, optimized REPLI-g buffer system, Phi 29 polymerase easily solves secondary structures such as hairpin loops, thereby preventing slipping, stoppage, and dissociation of the polymerase during amplification. This enables the generation of DNA fragments up to 100 kb without sequence bias (see figure "Unbiased amplification with Phi 29 polymerase").

Alkaline denaturation of DNA

Genomic DNA must be denatured before use in enzymatic amplification procedures, which is often accomplished using harsh methods such as incubation at elevated temperatures (heat incubation) or increased pH (chemical alkaline incubation). The REPLI-g Midi Kit uses gentle alkaline incubation, allowing uniform DNA denaturation with very low DNA fragmentation or generation of abasic sites. This results in amplified DNA with very high integrity, and maximizes the length of amplified fragments so that genomic loci and sequences are uniformly represented. With the REPLI-g Mini Kit, reliable results without false positive or negative data are ensured in subsequent downstream applications, unlike with other WGA technologies that use heat-induced denaturation that can damage template DNA, leading to biased and underrepresented loci (see figure "Effect of heat and alkaline denaturation on loci representation").

Procedure

Simple, one tube procedure

The REPLI-g Mini Kit uses a simple and reliable method to achieve accurate genome amplification from small quantities of isolated target genomic DNA, or directly from whole blood, dried blood cards, buffy coat, and tissue culture cells (see figure "REPLI-g Mini and Midi procedure"). The addition of lysis buffer, which both lysis the sample material and denatures the DNA, is followed by a short minute incubation (see figure "REPLI-g Mini and Midi procedure"). After neutralization, master mix (including REPLI-g Mini DNA Polymerase) is added and the isothermal amplification reaction proceeds overnight at 30°C. REPLI-g amplified DNA can be stored long-term at –20°C with no negative effects (see figure "Consistent long-term stability").

Select the REPLI-g Kit most suited to your specific requirements from our complete range of dedicated REPLI-g products (see table).

Specifications for the wide range of REPLI-g Kits
 REPLI-g Single CellREPLI-g MiniREPLI-g UltraFast MiniREPLI-g MidiREPLI-g ScreeningREPLI-g FFPEREPLI-g Mitochondrial DNA
Starting materialSingle cells, gDNAPurifed gDNA, blood, cellsPurifed gDNA, blood, cellsFFPE tissue, purified gDNA from FFPE tissuePurified gDNA
(Protocols for other starting materials available from )
Input amountSingle cells, 2–1000 cells, tissue, purified gDNA (1–10 ng)>10 ng gDNA, 0.5 µl blood or cells (>600 cells/µl)>10 ng gDNA, 0.5 µl blood or cells (>600 cells/µl)Section (1 cm diamter, 10–40 µm thick); >100 ng gDNA>1 ng purified gDNA
Yield (µg/reaction)40107–10408Standard yield: ≤10; High yield: ≤403–5
Reaction time8–16 h10–16 h1.5 h8–16 h12–16 hStandard yield: 4 h; High yield: 10 h8 h
Hands-on time15 min15 min15 min15 min15 min40 min15 min
FormatTubeTubeTubeTubePlateTubeTube
 

Applications

REPLI-g amplified genomic can be used in a variety of downstream applications, including:

  • SNP genotyping with TaqMan® primer/probe sets
  • qPCR- and PCR-based mutation detection
  • Next-generation sequencing
  • STR/microsatellite analysis
  • Sanger sequencing
  • RFLP and Southern blot analysis
  • Array technologies, such as comparative genomic hybridization 

Features

Specifications

AmplificationWhole genomic DNA
ApplicationsGenotyping, hybridization, RFLP
Denaturation stepAlkaline
Maximum input volume>10 ng DNA, 0.1– 0.5 µl whole blood, >600 cells/µl
Minimal pipetting volume needed0.5 µl
Quality assessmentNo
Reaction time8–16 hours (overnight)
Reaction volume50 µl
Samples per run (throughput)Mid
Starting amount of DNA>10 ng purified genomic DNA
Starting materialGenomic DNA, blood, cells, tissue
TechnologyMultiple Displacement Amplification (MDA)
Yield10–40 µg

QIAGEN 19133蛋白酶

QIAGEN 19133蛋白酶K(10ml)$r$

Qiagen 51304基因組

Qiagen 51304基因組DNA小提試劑盒$r

Qiagen試劑盒 QIAam

qiagen 57731 QIAamp 96 Vi

會員登錄

X

請輸入賬號

請輸入密碼

=

請輸驗證碼

收藏該商鋪

X
該信息已收藏!
標簽:
保存成功

(空格分隔,最多3個,單個標簽最多10個字符)

常用:

提示

X
您的留言已提交成功!我們將在第一時間回復(fù)您~

以上信息由企業(yè)自行提供,信息內(nèi)容的真實性、準確性和合法性由相關(guān)企業(yè)負責(zé),化工儀器網(wǎng)對此不承擔(dān)任何保證責(zé)任。

溫馨提示:為規(guī)避購買風(fēng)險,建議您在購買產(chǎn)品前務(wù)必確認供應(yīng)商資質(zhì)及產(chǎn)品質(zhì)量。

撥打電話
在線留言
庄浪县| 涞源县| 工布江达县| 凤山县| 玉溪市| 彭山县| 改则县| 汶川县| 巫山县| 通山县| 永定县| 石楼县| 博客| 资阳市| 青冈县| 石泉县| 阿拉善盟| 肥乡县| 乐昌市| 家居| 同江市| 衡山县| 额敏县| 石狮市| 涟源市| 略阳县| 南郑县| 平利县| 凤庆县| 台北县| 静宁县| 玛多县| 绥德县| 新丰县| 乐陵市| 靖宇县| 峡江县| 牙克石市| 托克托县| 自治县| 正蓝旗|