Paq5000 Hotstart PCR Master Mix 货号:A-600872
Paq5000 Hotstart PCR Master Mix
背景资料:Hot start methods for PCR prevent mispriming events, improve PCR yields, and allow room-temperature reaction setup. Our novel hot start method utilizes a heat-sensitive blocking polymerase protein that has been mutated to inactivate catalytic activity while retaining DNA binding activity. At room temperature, this protein binds to primed templates in the PCR reaction and prevents extension by the Paq5000 DNA polymerase. The blocking protein is inactivated during the initial PCR denaturation step, allowing the Paq5000 DNA polymerase to access the templates properly primed during the annealing step and proceed with extension.
Unlike traditional chemical or antibody methods, our method achieves true hot start without any modification to the DNA polymerase. Since we utilize the concept of competitive binding to block the DNA polymerase from extending at room temperature, the DNA polymerase is not modified to prevent extension. This allows the full activity of the DNA polymerase once the blocking protein is inactivated, leading to higher PCR yields. In addition, our method does not require a lengthy heat inactivation step that can compromise the polymerase and template DNA, nor an expensive antibody that must be used in vast excess and can interfere with the PCR reaction.
产品描述:Paq5000 is capable of quickly and robustly amplifying up to 6kb genomic DNA targets. With a shortened extension rate of 30 sec/kb and robust yields, Paq5000 is a Taq alternative that can be substituted easily into many Taq-based procedures.
产品特点:
1· Equal to better yield with fast cycling conditions ;
2·Robust, cost-effective alternative to Taq ;
3·Pre-optimized reaction buffers included ;
4.Low cost hot start formulation。
保存建议:在接收到艾德寄出的试剂盒后请按照说明书建议,使用不同的保存条件或温度来保存试剂盒内组分
定购信息:
| 产品名称 |
规格 |
操作手册 |
货号 |
询价 |
| Paq5000 Hotstart PCR Master Mix |
400 次 |
PDF |
A-600872 |
 |
| Paq5000 Hotstart PCR Master Mix |
100 次 |
PDF |
A-600870 |
|
| 植物DNA小量提取试剂盒 |
50 次 |
PDF |
A-DH813-01 |
|
| 植物DNA小量提取试剂盒 |
200 次 |
PDF |
A-DH813-02 |
|
| 凝胶DNA纯化回收试剂盒 |
100 次 |
PDF |
A-D2110-01 |
|
| 凝胶DNA纯化回收试剂盒 |
200 次 |
PDF |
A-D2110-02 |
|
| 凝胶DNA纯化回收试剂盒 |
500 次 |
PDF |
A-D2110-03 |
|
| 凝胶DNA纯化回收试剂盒 |
1000次 |
PDF |
A-D2110-04 |
|
| 胶自动纯化回收试剂盒(磁珠法) |
150 次 |
PDF |
A-DM136-01 |
|
| 胶自动纯化回收试剂盒(磁珠法) |
500 次 |
PDF |
A-DM136-02 |
|
| 总RNA自动化富集纯化mRNA试剂盒(磁珠法) |
30 次 |
PDF |
A-RM911-01 |
|
| 植物自动化DNA大量提取试剂盒(磁珠法) |
50 次 |
PDF |
A-DM311-01 |
|
| 组织切片DNA极速提取试剂盒 |
100 次 |
PDF |
A-P-1003-100 |
|
表观遗传学产品全面解决方案列下:
| 产品名称 |
规格 |
操作手册 |
货号 |
询价 |
| DNA羟甲基化定量试剂盒(荧光法) |
48 次 |
PDF |
A-P-1037-48 |
|
| DNA羟甲基化定量试剂盒(荧光法) |
96 次 |
PDF |
A-P-1037-96 |
|
| DNA羟甲基化定量试剂盒(比色法) |
48 次 |
PDF |
A-P-1036-48 |
|
| DNA羟甲基化定量试剂盒(比色法) |
96 次 |
PDF |
A-P-1036-96 |
|
| DNA甲基化定量试剂盒(荧光法) |
48 次 |
PDF |
A-P-1035-48 |
|
| DNA甲基化定量试剂盒(荧光法) |
96 次 |
PDF |
A-P-1035-96 |
|
| DNA甲基化定量试剂盒(比色法) |
48 次 |
PDF |
A-P-1034-48 |
|
| DNA甲基化定量试剂盒(比色法) |
96 次 |
PDF |
A-P-1034-96 |
|
| 通用DNA甲基化定量试剂盒 |
48 次 |
PDF |
A-P-1011-48 |
|
| 通用DNA甲基化定量试剂盒 |
96 次 |
PDF |
A-P-1011-96 |
|
| 超敏DNA甲基化定量试剂盒 |
48 次 |
PDF |
A-P-1021-48 |
|
| 超敏DNA甲基化定量试剂盒 |
96 次 |
PDF |
A-P-1021-96 |
|
| 总DNA甲基化定量试剂盒 |
48 次 |
PDF |
A-P-1014-48 |
|
| 总DNA甲基化定量试剂盒 |
96 次 |
PDF |
A-P-1014-96 |
|
推荐阅读:
关于5-hmC
5-hmC是近年来在动物组织中发现的,由胞嘧啶修饰而来。5-hmC在表观遗传学上的功能可能与5-甲基化胞嘧啶(5-mC)不同。尽管到现在为止还不确知其功能,有研究者猜测它在调控基因的表达与关闭过程中起着重要的作用。5-mC的发现让我们不得不重新评估DNA甲基信息,也不得不监测人类的健康组织和病理组织之间5-mC相对分布的差异。在EPI公司的MethylFlash技术之前,我们还没有发现任何直接的常规方法来检测5- hmC,以及区分5-hmC和5-mC
5-hmC 和 5-mC的区别
时下常用的DNA甲基化分析方法包括限制内切酶酶切和亚硫酸氢盐或MeDIP介导的MS-PCR和测序,这些技术都不适合用来检测5-hmC,因为它与5-mC事实上很难用这类方法区分开来。为了解决这个问题,EPIk研制了MethylFlash羟甲基化DNA定量试剂盒(荧光法)。本试剂盒提供了一种很经济的方法来检测5-羟甲基化胞嘧啶,并且区分5-hmC, 5-mC, 和 C,使得研究者能够重新评估他们的DNA甲基化信息,也能够在新样品中寻找DNA羟甲基化。 |
