PureLink™ HiPure 沉淀剂模块
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PureLink™ HiPure 沉淀剂模块
Invitrogen™

PureLink™ HiPure 沉淀剂模块

PureLink™ HiPure 沉淀剂能够使用阴离子交换色谱法快速、简单、高效地对分离的质粒 DNA 进行脱盐和浓缩。传统的阴离子交换分离的质粒 DNA 沉淀方法包括异丙醇沉淀,然后离心和干燥了解更多信息
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货号数量
K21002225 次制备
K21002110 次制备
货号 K210022
价格(CNY)
1,477.00
飞享价
Ends: 31-Dec-2025
1,883.00
共减 406.00 (22%)
Each
添加至购物车
数量:
25 次制备
价格(CNY)
1,477.00
飞享价
Ends: 31-Dec-2025
1,883.00
共减 406.00 (22%)
Each
添加至购物车
PureLink™ HiPure 沉淀剂能够使用阴离子交换色谱法快速、简单、高效地对分离的质粒 DNA 进行脱盐和浓缩。传统的阴离子交换分离的质粒 DNA 沉淀方法包括异丙醇沉淀,然后离心和干燥 DNA,这一过程耗时且费力。使用 PureLink™ HiPure 沉淀剂可在 5 分钟内进行质粒 DNA 浓缩,无需离心,并降低了在上清液去除过程中损失 DNA 沉淀的风险。回收率 >80%,得到的质粒 DNA 可直接用于具有挑战性的应用,如转染。
仅供科研使用。不可用于诊断程序。
规格
最终产品类型质粒 DNA
适用于(应用)下一代测序、转染、克隆、测序、转化、核酸标记、PCR、体外转录
高通量能力不兼容高通量应用(手动)
制备规模> 200 μg(大规模)质粒 DNA
产品线PureLink™
产品类型沉淀剂模块
数量25 次制备
样品类型细菌培养
运输条件室温
靶标质粒 DNA
测试时间5 min。
产品规格进样针
分离技术阴离子交换树脂
Unit SizeEach
内容与储存
PureLink™ HiPure 沉淀剂模块包括 HiPure 沉淀剂以及 5 ml 和 30 ml 注射器。将所有组分储存在室温下。

常见问题解答 (FAQ)

My plasmid yield was lower than expected. What could be the cause?

There are several reasons lower yields can occur:

-Make sure the binding of the plasmid is being done at RT. Temperature affects the pH of the binding solution.

-Make sure all other solutions are also warmed to RT for optimal yield.

-Verify that the centrifugation immediately following the neutralization step was not done at 4 degrees C. If it was, the supernatant MUST be warmed to RT before loading onto the column.

-The 1:1:1 ratio of buffers (Resuspension/Lysis/Precipitation) has not been kept precisely. A surplus of solution E3 will exceed the optimal salt concentration for DNA binding, thus leading to decreased DNA yield.

-Low-copy number plasmids give lower yields.

-If all of the medium was not removed at the cell harvesting step, the pH of the subsequent step can be affected and reduce yield.

-The cell pellet was not thoroughly resuspended before lysis.

-The purified DNA pellet was overdried after isopropanol precipitation and ethanol wash making it difficult to resuspend the pellet. Air dry only.

-Pellets can be easily lost during the alcohol precipitation and wash steps. It is best to pipette off the alcohol solutions rather than pouring them off, as the pellets tend to be slippery.

-After lysis and neutralization, the lysate is not homogeneous. After addition of solutions (Resuspension/Lysis/Precipitation buffers), cells must be mixed thoroughly by inverting the tubes until a homogeneous phase is obtained. Otherwise, cells will not be lysed completely and the plasmid DNA will stick to bacterial debris. In the case of bigger bacterial cell pellets, more vigorous shaking may be required to achieve homogeneity. However, do NOT vortex, as vortexing will release chromosomal DNA.

I did not recover any DNA after using one of your PureLink HiPure plasmid purification kits. Why?

The DNA pellet from precipitation with isopropanol is easily dislodged when washing with 70% ethanol. It is best to remove the isopropanol supernatant and the ethanol wash by pipetting. Be careful not to shoot the washing buffer directly onto the pellet. Instead, allow the washing buffer to run over the pellet. Regardless of which manufacturer's miniprep kit you use, washing the pellet can be challenging because it is so small.

What is the binding capacity of the PureLink HiPure Precipitator?

The binding capacity of the PureLink HiPure Precipitator is 2 mg.

Can I use the PureLink HiPure Precipitator with other anion exchange kits?

For best results, we recommend the use of the PureLink HiPure Precipitators with our PureLink HiPure Plasmid Filter Maxiprep/Midiprep Kit or PureLink HiPure Plasmid Maxiprep/Midiprep kit. However, PureLink HiPure Precipitator can be used with an equivalent anion exchange plasmid purification kit. We do offer the PureLink HiPure Precipitator as a stand-alone product (Cat. Nos. K210021 and K210022).

Can the PureLink HiPure Precipitator be re-used?

It is not recommended. We cannot guarantee the yield or the quality of the DNA from a re-used Precipitator.