产品信息

• 产品组分信息

  本产品提供以下试剂或组分：

  NEB #	名称	组分货号	储存温度	数量	浓度
  M0267V     -20       Taq DNA Polymerase with ThermoPol® Buffer M0267VVIAL -20 1 x 0.04 ml 5,000 units/ml   ThermoPol® Reaction Buffer B9004SVIAL -20 1 x 1.5 ml 10 X
  M0267S     -20       Taq DNA Polymerase with ThermoPol® Buffer M0267SVIAL -20 1 x 0.08 ml 5,000 units/ml   ThermoPol® Reaction Buffer B9004SVIAL -20 2 x 1.5 ml 10 X
  M0267L     -20       Taq DNA Polymerase with ThermoPol® Buffer M0267LVIAL -20 1 x 0.4 ml 5,000 units/ml   ThermoPol® Reaction Buffer B9004SVIAL -20 4 x 1.5 ml 10 X
  M0267X     -20       Taq DNA Polymerase with ThermoPol® Buffer M0267XVIAL -20 1 x 0.8 ml 5,000 units/ml   ThermoPol® Reaction Buffer B9004SVIAL -20 8 x 1.5 ml 10 X
  M0267E     -20       Taq DNA Polymerase with ThermoPol® Buffer M0267XVIAL -20 5 x 0.8 ml 5,000 units/ml   ThermoPol® Reaction Buffer B9004SVIAL -20 40 x 1.5 ml 10 X

• 特性和用法

  单位定义

  One unit is defined as the amount of enzyme that will incorporate 15 nmol of dNTP into acid-insoluble material in 30 minutes at 75°C.
  

  反应条件

  1X ThermoPol^® Reaction Buffer

  1X ThermoPol^® Reaction Buffer
  20 mM Tris-HCl
  10 mM (NH₄)₂SO₄
  10 mM KCl
  2 mM MgSO₄
  0.1% Triton® X-100
  (pH 8.8 @ 25°C)

  贮存溶液

  10 mM Tris-HCl
  100 mM KCl
  1 mM DTT
  0.1 mM EDTA
  0.5% Tween® 20
  0.5% IGEPAL® CA-630
  50% Glycerol
  pH 7.4 @ 25°C

  热失活

  否

  分子量

  理论上的: 94000 daltons

  5′ – 3′ 核酸外切酶

  Yes

  3′ – 5′ 核酸外切酶

  No

  链置换

  +

  产物末端

  • 3´ 单碱基突出末端

  单位活性检测条件

  1X ThermoPol Reaction Buffer, 200 µM dNTPs including [³H]-dTTP and 15 nM primed M13 DNA. 

  错配率

  ~ 285×10^-6bases

• 优势和特性

  应用特性

  • PCR
  • Primer extension
  • Colony PCR

• 相关产品

  相关产品

  • Taq 5X 预混液
  • Taq 2X 预混液
  • Taq PCR 试剂盒
  • dNTP 混合液
  • dNTP 套装
  • Quick-Load® Taq 2X 预混液
  • Magnesium Sulfate (MgSO₄) Solution

  单独销售的组分

  • ThermoPol® 反应缓冲液套装

• 注意事项

  1. 5´→3´ 结构特异性核酸内切酶活性会降解置换链。

• 参考文献

  1. Chien, A., Edgar, D.B. and Trela, J.M. (1976). J. Bact.. 127, 1550-1557.
  2. Kaledin, A.S., Sliusarenko, A.G. and Gorodetskii, S.I. (1980). Biokhimiya. 45, 644-651.
  3. Lawyer, F.C. et al. (1993). PCRMethods and Appl.. 2, 275-287.
  4. Longley, M.J., Bennett, S.E. and Mosbaugh D.W. (1990). NucleicAcids Res.. 18, 7317-7322.
  5. Lyamichev, V., Brow, M.A. and Dahlberg, J.E. (1993). Science. 260, 778-783.
  6. Saiki R.K. et al. (1985). Science. 230, 1350-1354.
  7. Powell, L.M. et al. (1987). Cell. 50, 831-840.
  8. Sun, Y., Hegamyer, G. and Colburn, N. (1993). Biotechniques. 15, 372-374.
  9. Sarkar, G., Kapelner, S. and Sommer, S.S. (1990). Nucleic Acids Res.. 18, 7465.

操作说明、说明书 & 用法

• 操作说明

  1. PCR Protocol for Taq DNA Polymerase with ThermoPol^® Buffer (M0267)
  2. A-Tailing with Taq Polymerase

• 使用指南

  • Activity of Restriction Enzymes in PCR Buffers
  • Guidelines for PCR Optimization with Taq DNA Polymerase
  • Guidelines for PCR Optimization with Thermophilic DNA Polymerases

工具 & 资源

• 选择指南

  • DNA Polymerase Selection Chart
  • NEB Diluent and Buffer Table
  • Taq Buffer Selection Chart
  • Thermophilic DNA Polymerases

• Web 工具

  • Tm Calculator

FAQs & 问题解决指南

• FAQs

  1. What ends will my PCR products have?
  2. How should I determine the appropriate annealing temperature for my reaction?
  3. What should the final primer concentration be in my PCR?
  4. What are the properties of this polymerase (fidelity, product ends, max amplicon, modified base incorporation, etc.)?
  5. What are the stability and storage requirements for NEB’s Taq and OneTaq DNA Polymerases?
  6. Is this Taq DNA Polymerase product compatible with other NEB Buffers?
  7. Can Taq/OneTaq^® DNA Polymerases be used for nick translation?
  8. How can I optimize my PCR when using Taq DNA Polymerase?

• 问题解决指南

  • PCR Troubleshooting Guide
  • Taq PCR Kit Troubleshooting Guide

• 实验技巧

  Did you know most Taq reactions amplify more efficiently and robustly when you use a 68°C extension temperature?