His-Strep pQE-TriSystem Vector Set

用于在 E. coli、昆虫和哺乳动物细胞中平行表达 His-Strep 标签蛋白

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His-Strep pQE-TriSystem Vector Set

Cat. No. / ID: 32942

pQE-TriSystem His-Strep 1 和 pQE-TriSystem His-Strep 2 载体，各 25 µg

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His-Strep pQE-TriSystem Vector Set 旨在用于分子生物学应用。该产品不能用于疾病诊断、预防和治疗。

✓ 24/7 automatic processing of online orders

✓ Knowledgeable and professional Product & Technical Support

✓ Fast and reliable (re)-ordering

Features

使用单一构建体在三个系统中平行表达
无需耗时的亚克隆
高水平表达
严格调控的表达
增强细胞毒性构建体的稳定性

Product Details

His-Strep pQE-TriSystem Vector Set 中的载体含有适用于 E. coli、昆虫和哺乳动物细胞表达系统的启动子。利用 His-Strep pQE-TriSystem 载体表达的蛋白质携带 6xHis 和 Strep 标签，能够在 Ni-NTA 和 Strep-Tactin 基质中进行序贯纯化，从而得到超纯（纯度 >98%）蛋白质。两种载体都编码 C-末端标签，确保只有全长蛋白质被纯化。

Performance

使用 His-Strep pQE-TriSystem Vector Set 表达的双标签蛋白可以通过两步法亲和纯化进行分离，从而得到超纯（纯度 >98%）蛋白质（参见图片“”）。

See figures

两步法纯化得到的超纯蛋白质。

Principle

His-Strep pQE-TriSystem Vector Set 允许同时具有 6xHis 标签和 Strep 标签 II 的蛋白质的表达。双标签允许通过两步法亲和纯化系统进行纯化，从而能够在标准化程序中简单高效地纯化得到超纯蛋白质。该系统还通过消除蛋白质特异性方案开发和优化的需要来提高通量。携带两种标签的重组蛋白在 Ni-NTA 和 Strep-Tactin 基质中依次纯化（参见图片“ 两步法亲和纯化程序”）。这两步简单的亲和纯化提供了适用于任何下游应用的完整活性、全长和超纯蛋白质。

See figures

两步法亲和纯化程序。

Procedure

携带两个小亲和标签（6xHis 标签和 Strep 标签 II）的重组蛋白可以使用 pQE-TriSystem His-Strep 载体在 E. coli、昆虫或哺乳动物细胞中高效表达。在细胞裂解和裂解物澄清后，使用基于已证实的 6xHis 标签-Ni-NTA 相互作用的固定化金属亲和层析 (immobilized-metal affinity chromatography, IMAC) 程序对蛋白质进行初步纯化。使用咪唑从 Ni-NTA 基质中洗脱后，将重组蛋白（也携带 Strep 标签 II 表位）直接装载至 Strep-Tactin 基质（参见图片“两步法亲和纯化程序”）。不需要更换缓冲液。使用生物素或脱硫生物素从 Strep-Tactin 基质中洗脱蛋白质。使用小鼠单克隆 Strep 标签或抗 His 抗体能够以高度特异性和灵敏度进行蛋白质检测（参见图片“ 携带 Strep 标签的蛋白质的高度灵敏性检测”）。

See figures

Highly sensitive detection of proteins carrying a Strep-tag.

Applications

Two-Step Affinity Purification System 非常适合必需使用高纯度并且难以单独使用 His 标签实现的应用，例如在真核细胞中表达的蛋白质。Two-Step Affinity Purification System 提供的超高纯度和便利性使其成为以下应用的首选方法：

高纯度蛋白质纯化
结构和功能分析
真核细胞系统中的表达

Supporting data and figures

Highly sensitive detection of proteins carrying a Strep-tag.

Specifications

Features	Specifications
Expression species	E. coli，哺乳动物细胞，昆虫细胞
Tag removal sequence	否
N- or C-terminal tag	N-末端和 C-末端标签
In-frame cloning necessary	是
Tag	6xHis 标签
Expression	体内
All three reading frames provided	否

Resources

For the pQE-TriSystem His-Strep 2 vector

For the pQE-TriSystem His-Strep 1 vector

Download Safety Data Sheets for QIAGEN product components.

For the pQE-TriSystem His-Strep 1 vector

For the pQE-TriSystem His-Strep 2 vector

FAQ

The basic technology behind the Strep-tag System is a Two-Step Affinity Protein Purification using sequential purification of recombinant proteins carrying two affinity tags. Proteins that carry these two small tags (the 6xHis tag and the 8 amino acid containing Strep-tag) are efficiently expressed in E. coli, insect, or mammalian cells using pQE-TriSystem His·Strep vectors. After cell lysis and clearing of the lysate, proteins are initially purified by a procedure based on the proven 6xHis-tag-Ni-NTA interaction. After elution from the Ni-NTA matrix using imidazole, recombinant proteins (which also carry the Strep-tag epitope) are loaded directly onto a Strep-Tactin matrix (Strep-Tactin SuperFlow or Strep-Tactin Magnetic Beads). Protein is eluted from the Strep-Tactin matrix using either biotin or desthiobiotin. This two-step affinity purification delivers ultrapure (>98% pure) protein. The order of purifications can also be reversed (i.e., Strep-Tactin followed by Ni-NTA purification). Since purification is done under native conditions, the Two-Step Affinity Purification System can be beneficial for highly demanding applications (i.e., crystallization studies).

FAQ ID -740