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引用和文献 (7)
Invitrogen™
Gateway™ LR Clonase™ 酶混合物
Gateway® LR Clonase® 酶混合物包含专有的 Int(整合酶)、IHF(整合宿主因子)和了解更多信息
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| 货号 | 数量 |
|---|---|
| 11791019 | 20 次反应 |
| 11791043 | 100 次反应 |
货号 11791019
价格(CNY)
7,145.00
飞享价
Ends: 31-Dec-2025
9,159.00共减 2,014.00 (22%)
Each
数量:
20 次反应
价格(CNY)
7,145.00
飞享价
Ends: 31-Dec-2025
9,159.00共减 2,014.00 (22%)
Each
Gateway® LR Clonase® 酶混合物包含专有的 Int(整合酶)、IHF(整合宿主因子)和 Xis(切除酶),可催化入门载体(含有侧翼是 attL 位点的目的基因)与目的载体(含有 attR 位点)进行体外重组,产生表达克隆。 根据具体的应用和所需的形式,我们提供不同规格的 LR Clonase 酶混合物。 LR Clonase II Plus 酶混合物是最新的产品型号,可提供最高的重组效率(表 1),并专门针对单片段和多片段克隆进行了优化(表 1)。 LR Clonase II Plus 为包含酶和反应缓冲液的优化型单一酶混合物,进行单片段和多片段克隆时所需的步骤更少,因此可以确保酶的稳定性和易用性。 我们的 LR Clonase II 酶混合物也有单一混合物形式,而最初的 LR Clonase® 酶提供单独管装的酶和缓冲液
仅供科研使用。不可用于诊断程序。
规格
兼容缓冲液反应缓冲液
产品类型LR Clonase 酶混合物
数量20 次反应
运输条件干冰
酶LR Clonase
产品线Clonase,Gateway
Unit SizeEach
内容与储存
所有 Gateway™ LR Clonase™ 酶试剂盒均包含蛋白酶 K 溶液 ( 2 µg/µL) 和阳性对照载体。在 -80°C 下储存 LR Clonase™ 酶;在 -20°C 下储存 LR Clonase™ II 或 II Plus 酶混合物。妥善储存时,可保证稳定储存 6 个月。
常见问题解答 (FAQ)
我进行了LR反应但是转化后背景很高,您可以提供一些解决这一问题的建议吗?
我进行了LR反应并在转化后得到了两种不同类型的克隆(大克隆和小克隆),可能原因有哪些?
我进行了LR反应但是转化后所得克隆很少或没有克隆,而转化对照也不成功。您能就此提供一些建议吗?
我进行了LR反应但是转化后所得克隆很少或没有克隆,而转化对照有克隆产生。您能就此提供一些建议吗?
我可以构建一个单独入门载体并和带有N-末端标记和C-末端标记的DEST载体一起使用吗?
引用和文献 (7)
引用和文献
Abstract
A suite of Gateway cloning vectors for high-throughput genetic analysis in Saccharomyces cerevisiae.
Journal:Yeast
PubMed ID:17583893
'In the post-genomic era, academic and biotechnological research is increasingly shifting its attention from single proteins to the analysis of complex protein networks. This change in experimental design requires the use of simple and experimentally tractable organisms, such as the unicellular eukaryote Saccharomyces cerevisiae, and a range of new high-throughput
Development of R4 gateway binary vectors (R4pGWB) enabling high-throughput promoter swapping for plant research.
Journal:Biosci Biotechnol Biochem
PubMed ID:18256458
We developed a new series of Gateway binary vectors, R4pGWBs, that are plant transformation vectors designed for one-step construction of chimeric genes between any promoter and any cDNA. The structure of R4pGWBs is almost the same as the promoterless type of improved pGWBs (ImpGWBs), except that the attR1 site is
Short hairpin RNAs (shRNAs) induce sequence-specific silencing in mammalian cells.
Journal:Genes Dev
PubMed ID:11959843
RNA interference (RNAi) was first recognized in Caenorhabditis elegans as a biological response to exogenous double-stranded RNA (dsRNA), which induces sequence-specific gene silencing. RNAi represents a conserved regulatory motif, which is present in a wide range of eukaryotic organisms. Recently, we and others have shown that endogenously encoded triggers of
Isolation of rat dihydrofolate reductase gene and characterization of recombinant enzyme.
Journal:Antimicrob Agents Chemother
PubMed ID:11502523
While assays of many antifolate inhibitors for dihydrofolate reductase (DHFR) have been performed using rat DHFR as a target, neither the sequence nor the structure of rat DHFR is known. Here, we report the isolation of the rat DHFR gene through screening of a rat liver cDNA library. The rat
High throughput immuno-screening of cDNA expression libraries produced by in vitro recombination; exploring the Plasmodium falciparum proteome.
Journal:Mol Biochem Parasitol
PubMed ID:14698438
Improved Plasmodium falciparum cDNA expression libraries were constructed by combining mRNA oligo-capping with in vitro recombination and directional cloning of cDNA inserts into a plasmid vector that expresses sequences as thioredoxin fusion proteins. A novel procedure has also been developed for the rapid identification of seropositive clones on high-density filters,