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HotStarTaq DNA Polymerase

高特异性扩增,所需优化次数少

S_1278_0_LS_OEM_HotStarTaq_DNA__Polymerase_250U
是否需要商用批量、定制或优化产品?我们还提供物流、合规等方面的支持。主动联系,与 QIAGEN 战略合作伙伴及 OEM 合作
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HotStarTaq DNA Polymerase (250 U)

目录编号 / ID.   203203

250 units HotStarTaq DNA Polymerase, 10x PCR Buffer, 5x Q-Solution, 25 mM MgCl2
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数量
250 U
1000 U
5000 U
25,000 U
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HotStarTaq DNA Polymerase 旨在用于分子生物学应用。该产品不能用于疾病诊断、预防和治疗。
是否需要商用批量、定制或优化产品?我们还提供物流、合规等方面的支持。主动联系,与 QIAGEN 战略合作伙伴及 OEM 合作
联系 OEM 专家

特点

  • 所需优化次数少
  • PCR特异性高
  • 操作方便,可在室温下构建反应体系

产品详情

不同于抗体介导的方法,HotStarTaq DNA Polymerase应用化学介导的热启动,可确保聚合酶在PCR初始加热阶段完全没有活性。HotStarTaq DNA Polymerase提供独特的QIAGEN PCR Buffer,将非特异性扩增产物、引物二聚体和其他污染降至最低。一种新型的添加剂Q-Solution,可实现难扩增的模板(如GC含量高的模板)高效扩增。

绩效

每一批HotStarTaq DNA Polymerase都经过全方位的质量控制测试,包括:严格的PCR特异性和具有可重复性的试剂,即使低拷贝的靶分子也可扩增。通过检测,HotStarTaq DNA Polymerase可确保高度特异性和在热启动PCR中的卓越表现(参见" Higher specificity with different primer–template systems"、" Superior performance"和表格)。该试剂盒提供的新型PCR缓冲液使得在多种PCR条件下都维持高特异性,无需优化(参见" Tolerance to variable magnesium concentration")。试剂盒中的Q-Solution可进一步优化PCR(参见" Amplification of difficult templates")。总之,这些组合确保了在多种应用中的特异性扩增(参见" Effect of hot start on RT-PCR performance"和" Highly sensitive single-cell PCR")。

热启动模式比较
HotStarTaq DNA Polymerase Supplier AII提供的热启动酶 抗体介导 手动 蜡屏障
特异性扩增 ++ + + +/– +/–
PCR优化需求 ++ +/– +/–
易用性 ++ ++ +
HotStarTaq DNA Polymerase特性

浓度:5 units/µl
重组酶:
底物类似物:dNTP、ddNTP、dUTP、biotin-11-dUTP、DIG-11-dUTP、fluorescent-dNTP/ddNTP
延伸速度:72°C条件下2–4 kb/min
酶半衰期:97°C条件下10 min,94°C条件下60 min
扩增效率:≥105
5'–>3'外切酶活性:
额外添加A:
3'–>5' 外切酶活性:
核酸酶污染:
蛋白酶污染:
RNases污染:
自启活性:否  

查看图表
Higher specificity with different primer–template systems.Higher specificity with different primer–template systems.Superior performance.Superior performance.Tolerance to variable temperature and magnesium concentrations.Tolerance to variable temperature and magnesium concentrations.Amplification of difficult templates.Amplification of difficult templates.Effect of hot start on RT-PCR performance.Effect of hot start on RT-PCR performance.Highly sensitive single-cell PCR.Highly sensitive single-cell PCR.

原理

HotStarTaq DNA Polymerase,一种经修饰的Taq DNA Polymerase,确保热启动PCR的高度特异性。该试剂盒包括新型的双阳离子PCR缓冲液、Q-Solution和MgCl2

HotStarTaq DNA Polymerase

HotStarTaq DNA Polymerase以非活性形式提供,常温下没有聚合酶活性。避免PCR构建和循环初始阶段低温条件下非特异性引物的延伸和引物二聚体的形成(参见" Superior performance in hot-start PCR"和" Higher specificity with different primer–template systems")。95°C条件下孵育15分钟即可激活HotStarTaq DNA Polymerase,这个步骤可整合入已有的热循环程序中。

QIAGEN PCR Buffer

QIAGEN PCR Buffer通过提高每个PCR扩增退火过程特异性引物的结合比例,确保PCR每个循环特异性扩增(参见" Increased specificity of primer annealing")。独特的KCl和(NH4)2SO4平衡组合,使得该缓冲液与传统的PCR缓冲液相比在很宽的温度和Mg2+浓度范围内都有严格的引物退火条件和高度的特异性,无需进行耗时的优化(参见" Tolerance to variable magnesium concentration")。

Q-Solution

该产品同时提供Q-Solution,一种新型的PCR添加剂,通过更改DNA熔解行为促进难扩增模板的扩增。这种独特的试剂可进一步优化由模板引起的表现不理想的PCR,如过多的二级结构和富含GC的模板(参见" Amplification of difficult templates")。不同于DMSO和其他PCR添加剂,Q-Solution的浓度是确定的,没有毒性,并且保证PCR的纯度。而且PCR中加入Q-Solution不会影响PCR的准确性。

查看图表
Superior performance.Superior performance.Higher specificity with different primer–template systems.Higher specificity with different primer–template systems.Increased specificity of primer annealing.Increased specificity of primer annealing.Tolerance to variable temperature and magnesium concentrations.Tolerance to variable temperature and magnesium concentrations.Amplification of difficult templates.Amplification of difficult templates.

程序

HotStarTaq DNA Polymerase提供高效、经优化的实验方案,用于快速、方便的构建PCR反应体系。95°C条件下孵育15分钟激活HotStarTaq DNA Polymerase,可以整合入已有的热循环程序。反应可在室温下建立,更加方便和易于使用(参见" HotStarTaq procedure")。
查看图表
HotStarTaq procedure.HotStarTaq procedure.

应用

HotStarTaq DNA Polymerase适合多种应用,包括各种富有挑战性的研究,如各种扩增应用:

  • 复杂的基因模板
  • 复杂的cDNA模板(如RT-PCR)
  • 低拷贝的靶序列(如单细胞PCR)
  • 多重引物对反应

辅助数据和图表

HotStarTaq procedure.

HotStarTaq procedure.
HotStarTaq procedure.
HotStarTaq procedure.
Increased specificity of primer annealing.
Effect of hot start on RT-PCR performance.
Higher specificity with different primer–template systems.
Superior performance.
Tolerance to variable temperature and magnesium concentrations.
Amplification of difficult templates.
Highly sensitive single-cell PCR.

规格

特点规格
applicationsPCR, RT-PCR, Complex genomic templates, very low-copy targets
withwithouthotstartWith hotstart
reactiontypePCR amplification
sampletargettypeGenomic DNA and cDNA
realtimeorendpointEndpoint
enzymeactivity5' -> 3' exonuclease activity
mastermixNo
singleormultiplexSingle

资源

快速启动实验方案 (1)
HotStarTaq DNA Polymerase (EN)
PDF (59KB)
试剂盒操作手册 (1)
HotStarTaq PCR Handbook - (EN)
PDF (178KB)
HotStarTaq DNA Polymerase; HotStarTaq Master Mix Kit - For highly specific hot-start PCR without optimization  
补充实验方案 (1)
Polyacrylamide gel analysis of oligonucleotides
PDF (36KB)
产品介绍与指南 (2)
HotStarTaq DNA Polymerase
PDF (537KB)
(EN) - Maximizing PCR and RT-PCR success — Third Edition
PDF (2MB)
Addressing critical factors and new solutions
安全数据表 (2)
Safety Data Sheets
Download Safety Data Sheets for QIAGEN product components.
Safety Data Sheets
Download Safety Data Sheets for QIAGEN product components.
技术资讯 (1)
(EN) - Maximizing end-point PCR success with QIAGEN's automatable PCR solutions
PDF (1MB)
Certificates of Analysis (1)
Certificates of Analysis

文献

MALDI-TOF mass spectrometry for multiplex genotyping of CYP2B6 single-nucleotide polymorphisms.
Blievernicht JK; Schaeffeler E; Klein K; Eichelbaum M; Schwab M; Zanger UM;
Clin Chem; 2006; 53 (1):24-33 2006 Nov 2 PMID:17082249
Age-related urinary excretion of BK polyomavirus by nonimmunocompromised individuals.
Zhong S; Zheng HY; Suzuki M; Chen Q; Ikegaya H; Aoki N; Usuku S; Kobayashi N; Nukuzuma S; Yasuda Y; Kuniyoshi N; Yogo Y; Kitamura T;
J Clin Microbiol; 2006; 45 (1):193-8 2006 Nov 8 PMID:17093017
Transcriptional regulation of human CYP2A13 expression in the respiratory tract by CCAAT/enhancer binding protein and epigenetic modulation.
Ling G; Wei Y; Ding X;
Mol Pharmacol; 2006; 71 (3):807-16 2006 Dec 5 PMID:17148654
Seizures and enhanced cortical GABAergic inhibition in two mouse models of human autosomal dominant nocturnal frontal lobe epilepsy.
Klaassen A; Glykys J; Maguire J; Labarca C; Mody I; Boulter J;
Proc Natl Acad Sci U S A; 2006; 103 (50):19152-7 2006 Dec 4 PMID:17146052
Assessing combined methylation-sensitive high resolution melting and pyrosequencing for the analysis of heterogeneous DNA methylation.
Candiloro IL; Mikeska T; Dobrovic A;
Epigenetics; 2011; 6 (4):500-7 2011 Apr 1 PMID:21364322
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