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- 文献和实验
- 技术资料
- 英文名:
FastDigest XbaI
- 规格:
300 reactions
描述
| 5' | T ↓ | C | T | A | G | A | 3' | ||||
| 3' | A | G | A | T | C ↑ | T | 5' |
Thermo Scientific FastDigest XbaI restriction enzyme recognizes T^CTAGA site and cuts best at 37°C in 5–15 minutes using universal FastDigest Buffer.
Thermo Scientific FastDigest XbaI is one of an advanced line of fast restriction enzymes that are all 100% active in the universal FastDigest and FastDigest Green reaction buffers.
The universal buffer allows rapid single-, double-, or multiple DNA digestion within 5–15 minutes eliminating any need for buffer change or subsequent DNA clean-up steps. See Reaction Conditions for FastDigest Enzymes for a table of enzyme activity, heat inactivation and incubation times for this and other FastDigest restriction enzymes. DNA modifying enzymes, such as Klenow Fragment, T4 DNA Ligase, alkaline phosphatases and T4 DNA Polymerase all have 100% activity in FastDigest Buffer. Therefore, enzymes for downstream applications can be directly added to the FastDigest reaction mix.
For additional convenience FastDigest Green Buffer includes a density reagent and two tracking dyes for direct loading of digestion reaction products on gels.
Short incubation times and optimal composition of the universal FastDigest Buffer eliminate star activity effects.
Features
• 100% activity of all FastDigest enzymes in the universal buffer
• 100% buffer compatibility with downstream applications
• Complete digestion in 5–15 minutes
规格
| Compatible Buffer: | 10x FastDigest Buffer/FastDigest Green Buffer |
|---|---|
| Enzyme: | Xba I |
| Methylation Sensitivity: | Not CpG methylation-sensitive, Not dcm methylation-sensitive, dam methylation-sensitive |
| Optimal Reaction Temperature: | 37° C |
| Product Line: | FastDigest |
| Product Size: | 300 reactions |
| Sensitive to Heat Inactivation: | Yes |
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文献和实验【求助】请教关于xbaI酶切位点甲基化的问题(看了这么多帖子,都好象没分析到位啊)
2012hunanjob 在xbaI酶切位点上:T^CTAGA碱基对应的是AGATC^T,因为质粒是双链,所以在质粒的xbaI酶切位点上中间肯定有GATC,所以说:我觉得理论上只要是dam+细菌提出来的质粒,xbaI酶切位点都受甲基化影响而切不开.但是我见过别人也是用dam+菌扩增过质粒,用xbaI也可以切开它的酶切位点~~~所以我就迷糊了,请各位大侠们多多指点,小弟在此感激不尽了~~~ 2012hunanjob 顶,有没有
wj1989113 最近在构建一个质粒。 根据我的目的基因序列,筛了两个酶切位点,而且只有这两个酶切位点能用,XbaI和EcoRI, 设计引物时XbaI 加了两个保护碱基,EcoRI 加了三个保护碱基。根据takara公司的说明,选择了共用Buffer1xM,酶切,连接,转化之后挑克隆,抽质粒酶切鉴定,发现都是空载体。网上说XbaI对甲基化敏感,有什么对策?因为我别无他选,只能用这两个酶。 不胜
Determining the Direction of Replication Fork Movement
without interference from nicked or broken DNA. As an example of the procedure, consider an XbaI restriction fragment that is replicated by a single replication fork and has an AvaI site near one end. The XbaI cleaved replication intermediates are separated by mass
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