T-REx™ 核心试剂盒,含 pcDNA™4/TO 载体
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T-REx™ 核心试剂盒,含 pcDNA™4/TO 载体

A Tetracycline-Regulated Expression System without Viral TransactivatorsThe T-REx™ System yields higher levels of induced expression than any other regulated mammalian了解更多信息
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货号数量
K102002
又称 K1020-02
1 kit
货号 K102002
又称 K1020-02
价格(CNY)
19,543.34
飞享价
Ends: 31-Dec-2025
23,338.00
共减 3,794.66 (16%)
Each
添加至购物车
数量:
1 kit
价格(CNY)
19,543.34
飞享价
Ends: 31-Dec-2025
23,338.00
共减 3,794.66 (16%)
Each
添加至购物车
A Tetracycline-Regulated Expression System without Viral Transactivators
The T-REx™ System yields higher levels of induced expression than any other regulated mammalian expression system. It utilizes the complete CMV promoter and adds control elements from the bacterial tetracycline resistance operon to effectively repress and derepress transcription from one of the strongest mammalian promoter sequences known (1,2).

Specific Activation
The T-REx™ System uses a repressor mechanism that blocks transcription from the powerful CMV promoter in the absence of tetracycline. Because the T-REx™ System elements do not use viral transactivators, you can achieve high-level expression from the complete CMV promoter without secondary, non-specific activation of host genes.

The T-REx™ Mechanism
The T-REx™ transcriptional control elements are illustrated in Figure 1. Two tetracycline operator sequences (TetO2) have been inserted between the TATA box of the CMV promoter and the transcriptional start site. The TetO2 sequence itself has no effect on expression. When the tetracycline repressor protein (TR) is present, it effectively binds the TetO2 sites and blocks transcription initiation. Tetracycline added to the culture medium binds to, and changes the conformation of, the TR protein. This change causes the TR protein to release the TetO2 sites, derepressing transcription from the CMV promoter. The result is high-level expression of the gene of interest (Figure 2). Expression levels can be modulated based on the tetracycline concentration and can be induced to levels that are achieved with constitutive CMV expression vectors.

T-REx™ is a powerful inducible mammalian expression system that allows you to regulate expression from the complete human cytomegalovirus (CMV) enhancer-promoter. T-REx™inducible expression vectors offer the following features:

• Complete CMV enhancer-promoter sequence containing two copies of the tetracycline operator TetO2 sequence for high-level regulated expression
• Zeocin™ or hygromycin resistance gene for effective selection of stable mammalian cell lines
• Large multiple cloning site to simplify cloning

In addition, pcDNA™4/TO/myc-His offers a c-myc epitope for rapid detection of the recombinant protein with an Anti-myc Antibody and a polyhistidine (6xHis) sequence for simple purification of the recombinant protein with nickel-chelating resin and detection with Anti- His(C-term) Antibody.

The regulatory vector, pcDNA™6/TR, is provided for high-level expression of the tetracycline repressor (TR) protein. This vector expresses the Blasticidin resistance gene for rapid selection of mammalian cell lines that stably express the TR protein.
仅供科研使用。不可用于诊断程序。
规格
构成或诱导系统诱导
输送类型转染
适用于(应用)调节表达
诱导剂四环素
产品类型T-Rex 核心克隆试剂盒,带载体
数量1 kit
选择试剂(真核生物)Zeocin™、杀稻瘟菌素
载体pcDNA
克隆方法限制性内切酶/MCS
产品线Gateway、T-REx、pcDNA, T-REx, pcDNA
促进剂CMV/TO
蛋白标记未标记
Unit SizeEach
内容与储存
T-REx™ 核心试剂盒包括 20 µg pcDNA™4/TO 或 pcDNA™4/TO/myc-His A、B 和 C 各 20 µg;阳性对照载体、pcDNA™6/TR 以及正向和反向测序引物。

所有载体均超螺旋化并提供冻干形式。

所有组分均储存在 -20°C 下。妥善储存时,所有组分可保证稳定储存 6 个月。

常见问题解答 (FAQ)

为何在T-REx和GeneSwitch系统中推荐使用连续转染而非共转染?

当执行共转染时,用户无法在稳转细胞系中同时完成功能性TetR或GeneSwitch蛋白的双重测试。另一方面,如果执行连续转染,用户就可对所生成的T-REx或GeneSwitch细胞系进行功能性测试,他们可将LacZ对照表达质粒瞬转进入细胞,并挑取那些在诱导剂缺乏条件下表达LacZ的本底水平最低,而在含诱导剂条件下LacZ表达水平最高的克隆。之后可对这一克隆进行扩增,并按需用于T-REx或GeneSwitch表达载体的转染实验。

GeneSwitch系统超越T-REx系统的主要优势有哪些?其主要劣势有哪些?

使用GeneSwitch系统能够确保目的基因处于极低的基础表达水平,而T-REx系统可能会有少量渗漏表达,因为FBS中不可避免的存在着一些四环素。GeneSwitch系统的诱导表达水平可能甚至高于CMV启动子。GeneSwitch系统的劣势在于,尽管该系统能够在转基因条件下以优异的性能工作,但在培养系统中关闭表达的操作不是很容易实现。而另一方面,T-REx系统可通过加入和去除诱导剂来切换开关状态。

Flp-In T-REx系统超越T-REx系统的优势有哪些?

Flp-In T-REx系统将Flp-In系统的靶向整合与T-REx系统的强大诱导表达能力整合在一起。该系统能够生成同基因,可诱导的稳定表达细胞系,并能够针对这些细胞系实行多克隆筛选。一旦建立了包含整合FRT位点的Flp-In T-REx宿主细胞系,后续建立表达目的基因的Flp-In T-REx细胞系就变得迅速高效了。

我能否使用强力霉素代替四环素,来作为T-REx系统中的诱导剂?

强力霉素可作为T-REx系统中诱导剂的代替品。它的作用机理与四环素相近,并在T-REx系统中表现出与四环素相似的剂量效应和诱导性质。强力霉素显示出比四环素更长的半衰期(分别为48小时和24小时)。我们未提供强力霉素,但用户可从Sigma(货号D9891)进行购买。

我计划使用pcDNA6/TR构建一株T-REx细胞系。我能否使用TetR的抗体和免疫印迹实验来评估细胞中是否表达了足量的TetR?你们是否提供TetR的抗体?

我们未提供anti-TetR的抗体。即使使用anti-TetR抗体的免疫印迹技术能够筛选出不表达TetR蛋白的克隆,这也不能作为筛选功能性克隆的理想方法。通过瞬转表达LacZ的对照质粒来进行功能测试可以满足这一需求,用户可挑选那些在无四环素条件下β-半乳糖苷酶表达水平极低,而加入四环素后β-半乳糖苷酶表达水平极高的那些克隆。

View all T-REx™ 核心试剂盒,含 pcDNA™4/TO 载体 FAQs

引用和文献 (4)

引用和文献
Abstract
Comparison of seven different heterologous protein expression systems for the production of the serotonin transporter.
Authors:Tate CG, Haase J, Baker C, Boorsma M, Magnani F, Vallis Y, Williams DC,
Journal:Biochim Biophys Acta
PubMed ID:12586388
'The rat serotonin transporter (rSERT) is an N-glycosylated integral membrane protein with 12 transmembrane regions; the N-glycans improve the ability of the SERT polypeptide chain to fold into a functional transporter, but they are not required for the transmembrane transport of serotonin per se. In order to define the best ... More
Effect of some aldoses on growth of Saccharomyces cerevisiae inhibited with molybdenum.
Authors:Zemek J, Bílik V, Zákutná L,
Journal:Folia Microbiol (Praha)
PubMed ID:285
The inhibitory effect of molybdenum ions on growth of yeasts at pH 5.5 was found to be decreased by aldoses in the following order: D-talose greater than L-mannose greater than L-ribose greater than D-lyxose greater than L-galactose greater than L-arabinose greater than L-glucose greater than L-xylose. Increased concentrations of molybdenum ... More
Human TRPC5 channel activated by a multiplicity of signals in a single cell.
Authors:Zeng F, Xu SZ, Jackson PK, McHugh D, Kumar B, Fountain SJ, Beech DJ,
Journal:J Physiol
PubMed ID:15254149
Here we explore the activation mechanisms of human TRPC5, a putative cationic channel that was cloned from a region of the X chromosome associated with mental retardation. No basal activity was evident but activity was induced by carbachol stimulation of muscarinic receptors independently of Ca2+ release. This is 'receptor activation', ... More
The gamma -secretase-cleaved C-terminal fragment of amyloid precursor protein mediates signaling to the nucleus.
Authors: Gao Y; Pimplikar S W;
Journal:Proc Natl Acad Sci U S A
PubMed ID:11742091
Sequential processing of the amyloid precursor protein (APP) by beta- and gamma-secretases generates the Abeta peptide, a major constituent of the senile plaques observed in Alzheimer's disease. The cleavage by gamma-secretase also results in the cytoplasmic release of a 59- or 57-residue-long C-terminal fragment (Cgamma). This processing resembles regulated intramembrane ... More