K1232 Thermo PCR 克隆 ,CloneJET PCR Cloning Kit /CloneJET PCR 克隆试剂盒

2024-10-24

CloneJET PCR Cloning Kit /CloneJET PCR 克隆试剂盒

货号:K1232,K1231

规格:40 reactions,20 reactions

价格:3296,1762

产品类型:PCR 及DNA聚合酶

品牌:Thermo Fisher

Thermo Scientific CloneJET PCR Cloning Kit, also available with DH10B cells (K123120), is an advanced positive selection system for high-efficiency cloning of PCR products generated with any thermostable DNA polymerase. Any other blunt or sticky-end DNA fragment can be cloned. It is ideal for phosphorylated or non-phosphorylated DNA fragments. Ligation into the included positive selection vector takes only 5 minutes, yielding more than 99% recombinant clones. Blunt-ended PCR products generated with a proofreading enzyme are ligated directly into the cloning vector.PCR products generated either with non-proofreading DNA polymerases or mixtures of DNA polymerases are blunted prior to ligation in 5 minutes with the thermostable DNA Blunting Enzyme provided with the kit. All common laboratoryE. colistrains can be directly transformed with the ligation product.FeaturesThe CloneJET PCR Cloning Kit contains a novel, ready-to-use positive selection cloning vector pJET1.2/blunt. The vector contains a lethal restriction enzyme gene that is disrupted by ligation of a DNA insert into the cloning site. As a result, only bacterial cells with recombinant plasmids are able to form colonies. Recircularized pJET1.2/blunt vector molecules lacking an insert express a lethal restriction enzyme, which kills the hostE. colicell after transformation. This positive selection drastically accelerates the process of colony screening and eliminates additional costs required for blue/white selection.For convenience in mapping and manipulation of the insert, the pJET1.2/blunt cloning vector multiple cloning site contains two BglII recognition sequences that flank the insertion site. In addition, the vector contains a T7 promoter forin vitroandin vivotranscription as well as sequencing of the insert.Prior to electroporation, always column-purify the ligation mixture using e.g.GeneJET PCR Purification Kit #K0701or chloroform to extract it. Electroporation is inhibited by the presence of proteins and salts in the mixture.

优点:

-Fast—PCR cloning in only 5 minutes-Highest efficiency– > 99% of positive clones-No cloning background—positive selection vector-Versatile—ideal for blunt-end or sticky-end cloning-Economical—no expensive blue/white screening

数据:

图1.pJET1.2/blunt 载体携带一个致死性限制性酶基因,此基因在 DNA 片段插入克隆位点后即被破坏。因此,只有含重组质粒的细菌细胞才能生长形成菌落。如果 pJET1.2/blunt 载体在没有片段插入的情况下重新环化,会表达致死性限制性酶,其在转化后杀死宿主E. coli细胞。这种阳性筛选大大加快了菌落筛选的进程,节省了蓝白斑筛选所需的额外成本。为了便于对插入片段进行鉴定和后续处理,pJET 1.2/blunt 载体的多克隆位点包含两个 BgIII 识别序列,横跨插入位点两端。此外,载体含有用于in vitro和in vivo转录以及插入片段测序的 T7 启动子。

图2. 粘性末端和平末端 PCR 产物克隆效率。根据供货商推荐的方案,将由TaqDNA 聚合酶或 Phusion DNA 聚合酶生成的976 bp PCR 产物连接到不同的克隆载体中。使用供货商指定片段作为阳性对照。各取2 μl 连接混合物转化E. coliDH10B 细胞。供货商提供的感受态细胞用于相应基于拓扑异构酶的反应。根据对照物的阳性重组百分比,计算克隆效率。图3.CloneJET Cloning Procedure

图4. Transformation efficiency of sticky- and blunt- end PCR productsA 976-bp PCR product generated with either Taq DNA Polymerase or Phusion DNA Polymerase was ligated into different cloning vectors according to the vendor’s recommended protocols. As a control, the vendor-specific fragment was used. Ligation mixtures of 2 µl each were used to transform E.coli DH10B cells. Transformation efficiency of competent cells was 1.2x10E7 transformants per µg supercoiled DNA.

组成成分:

▪pJET1.2/blunt Cloning Vector▪T4 DNA Ligase▪ 2X Reaction Buffer▪ DNA Blunting Enzyme▪ pJET1.2Forward Sequencing Primer(5'-CGACTCACTATAGGGAGAGCGGC-3')▪ pJET1.2Reverse Sequencing Primer(5'-AAGAACATCGATTTTCCATGGCAG-3')▪ Control PCR Product▪Water, nuclease-free▪ Detailed Protocol

相关产品:

▪DNA 片段标准品▪DNA ladder▪DNA 聚合酶▪PCR▪DNA纯化▪RNA纯化

技术参数

产品应用 • Cloning of blunt-end or 3'-dA tailed PCR products up to 10 kb • Cloning of DNA fragments generated by restriction enzymes • Sequencing of cloned DNA • in vitro and in vivo transcription of cloned inserts from the T7 promoter

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