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6DZ6472
- 206145
- QIAGEN Multiplex PCR Kit (1000),206145,Qiagen,凯杰
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- 45个工作日
- ¥ 38910.00
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6DZ6472
For 100 x 50 µl multiplex PCR reactions: 2x QIAGEN Multiplex PCR Master Mix (providing a final concentration of 3 mM MgCl2, 3 x 0.85 ml), 5x Q-Solution (1 x 2.0 ml), RNase-Free Water (2 x 1.7 ml)
用于高特异性和灵敏度的多重PCR,无需优化
无需优化步骤
高特异性和高灵敏度,热启动
高度适合用于各种类型的多重PCR应用
使用简单,经济实惠
QIAGEN Multiplex PCR Kit提供方便的即用型预混液。QIAGEN Multiplex PCR Master Mix包含HotStarTaq DNA Polymerase和含有新型合成因子MP的独特PCR缓冲液。配合优化的盐浓度,MP因子可以促进引物与模板的特异性结合,使反应体系中所有的引物都能有效延伸,无需额外优化。该试剂盒还包含新型的辅助剂Q-Solution,有助于实现“困难”模板(比如,GC含量高的模板)的高效扩增。
QIAGEN Multiplex PCR Kit可确保高特异性和灵敏度的多重PCR扩增。该试剂盒能成功应用于各种多重应用,如转基因生物分型和微卫星分析。该混合物包含HotStarTaq DNA Polymerase,用于高效的平行扩增多个靶。扩增效率经新型的PCR缓冲液进一步优化,该缓冲液也包含在混合物中。独特的缓冲液确保了在广泛的PCR条件下PCR的特异性,无需优化步骤。试剂盒还包含辅助剂Q-Solution,用于扩增高GC含量的模板,优化PCR反应。
HotStarTaq DNA Polymerase规格
浓度:5单位/µl
重组酶:有
底物类似物:dNTP、ddNTP、dUTP、biotin-11-dUTP、DIG-11-dUTP、荧光-dNTP/ddNTP
延伸率:72°C下2–4 kb/分钟
半衰期:97°C下10分钟;94°C下60分钟
扩增效率:≥105倍
5'–>3'外切酶活性:有
Extra A辅助剂: 有
3'–>5'外切酶活性:无
污染核酸:无
污染RNA酶:无
污染蛋白酶:无
自吸泵活性:无
Features | Specifications |
| 应用 | PCR, RT-PCR, multiplex PCR, typing, detection |
| 酶活 | 5' -> 3' exonuclease activity |
| 预混液 | Yes |
| 反应类型 | PCR amplification |
| real-time或终点法PCR | Endpoint |
| 样本/目标类型 | Genomic DNA and cDNA |
| 单一或多重 | Multiplex |
| 有/无热启动酶 | With hotstart |
Successful microsatellite analysis.
Analysis of microsatellite loci D3S1358, TH01, D21S11, D18S51, and Penta E was carried out using 1 ng of K562 human genomic DNA and fluorescein-labeled primers. Reactions were analyzed on the ABI PRISM 377 Sequencer. Top: The QIAGEN Multiplex PCR Kit ensured high sensitivity and uniform signal intensity. Bottom: Results using a hot-start DNA polymerase from Supplier AII.
Stable and efficient primer annealing.
Genotyping transgenic mice.
Transgenic mice were screened using the QIAGEN Multiplex PCR Kit and sets of 3 primers to distinguish wild-type (wt), heterozygous mutant (ht), and homozygous mutant (hm) mice. [A] Using a primer set for the recombination activating gene 2 locus. [B] Using a primer set for the interferon-γ gene locus. M: markers. (Data kindly provided by S. zur Lage and S. Weiss, National Research Center for Biotechnology, Braunschweig, Germany.)
Successful 16-plex PCR.
Multiplex PCR of 16 targets (99–955 bp) was carried out for 35 cycles using standard conditions for the QIAGEN Multiplex PCR Kit, without further optimization or using a variety of conditions with a hot-start DNA polymerase from Supplier AII. [A] Comparison using 2.5 units per 50 µl reaction of the hot-start DNA polymerase from Supplier AII and with the indicated Mg2+ concentrations. [B] Comparison using the optimized Mg2+ concentration (3.5 mM) for the hot-start DNA polymerase from Supplier AII (part A) and the indicated amounts of enzyme per 50 µl reaction. Successful results were ensured with the QIAGEN Multiplex PCR Kit. M: markers.
QIAGEN Multiplex PCR Kit高度适用于各种多重应用,包括:
转基因生物的分型和分析
微卫星的扩增和分析
细菌和病毒的分型和检测
用于SNP分析的多个DNA扩增
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