QIAexpress Type IV Kit

用于 N-末端 His 标签蛋白的高水平表达和一步法纯化

S_1126_8_QIAexpress_Type_IV_Kit

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QIAexpress Type IV Kit

Cat. No. / ID:   32149

各 5 µg:pQE-30、pQE-31、pQE-32(N-末端 6xHis);10 ml Ni-NTA 琼脂糖
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QIAexpress Type IV Kit 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。

✓ 全天候自动处理在线订单

✓ 博学专业的产品和技术支持

✓ 快速可靠的(再)订购

特点

  • 覆盖所有三个阅读框的载体
  • 用于 His 标签蛋白表达和纯化的完整试剂盒
  • N-末端 His 标签蛋白的高水平表达
  • 用于一步法纯化和灵敏性检测的通用型、完整系统

产品详情

QIAexpress System 提供了用于 His 标签蛋白表达、纯化和检测的材料。

绩效

QIAexpress Type IV Kit 提供高达总细胞蛋白 50% 的高效表达。

原理

QIAexpress pQE 载体将强效的噬菌体 T5 启动子(可被 E. coli RNA 聚合酶识别)与双 lac 操作子抑制模块相结合,以在 E. coli 中提供严格调控的高水平重组蛋白表达。在存在高水平 lac 阻遏物的情况下,蛋白质合成被有效阻断,并且细胞毒性构建体的稳定性得以增强。pQE 载体(参见图片  pQE 载体和表格)能够将 His 标签置入重组蛋白的 N-末端或 C-末端。

QIAexpress pQE 载体中存在的元件
元件 说明
1.优化的启动子/操作子元件 由噬菌体 T5 启动子和两个 lac 操作子序列组成,这增加了 lac 阻遏物结合的可能性,并确保强效 T5 启动子的有效抑制
2.合成核糖体结合位点 RBSII  用于高效翻译
3.His 标签编码序列 5' 或 3' 到多位点人工接头克隆区
4.翻译终止密码子 在所有阅读框架中,用于方便地制备表达构建体
5.两个强转录终止子 t0 来自噬菌体 λ,T1 来自 E. coli 的 rrnB 操纵子,以阻止连读转录并确保表达构建体的稳定性
6.ColE1 复制起点 来自 pBR322
7. β-内酰胺酶基因 (bla) 赋予氨苄青霉素耐药性
查看图表

程序

将编码目标蛋白质的插入片段克隆到合适的构建体中,并转化至合适的 E. coli 菌株中进行表达。通过添加 IPTG 来诱导表达。QIAexpress Type IV Kit 构建体可以转化至 E. coli 中,用作昆虫细胞中重组蛋白表达的穿梭载体,或转染至哺乳动物细胞中。

应用

QIAexpress Expression System 提供适用于许多应用的蛋白质高水平表达,包括:

  • 功能性构象活性蛋白质的纯化
  • 在变性条件下进行纯化用于抗体生产
  • 结晶用于三维结构测定
  • 涉及蛋白质-蛋白质和蛋白质-DNA 相互作用的检测

辅助数据和图表

Specifications

FeaturesSpecifications
Applications蛋白质组学
Yield总蛋白的 <50%
Special feature用于一步法纯化的通用型、完整系统
Tag6xHis 标签
Processing手动
Start material细胞裂解物
N- or C-terminal tagN-末端标签

资源

产品选择指南 (1)
安全数据表 (1)
Download Safety Data Sheets for QIAGEN product components.
试剂盒操作手册 (1)
A handbook for high-level expression and purification of 6xHis-tagged proteins
Safety Data Sheets (1)
Certificates of Analysis (1)

Publications

YtsJ has the major physiological role of the four paralogous malic enzyme isoforms in Bacillus subtilis.
Lerondel G; Doan T; Zamboni N; Sauer U; Aymerich S;
J Bacteriol; 2006; 188 (13):4727-36 2006 Jul PMID:16788182
Diurnal and seasonal variation of isoprene biosynthesis-related genes in grey poplar leaves.
Mayrhofer S; Teuber M; Zimmer I; Louis S; Fischbach RJ; Schnitzler JP;
Plant Physiol; 2005; 139 (1):474-84 2005 Aug 26 PMID:16126852
MtdC, a novel class of methylene tetrahydromethanopterin dehydrogenases.
Vorholt JA; Kalyuzhnaya MG; Hagemeier CH; Lidstrom ME; Chistoserdova L;
J Bacteriol; 2005; 187 (17):6069-74 2005 Sep PMID:16109948
Differential gene expression associated with euryhalinity in sea bream (Sparus sarba).
Deane EE; Woo NY;
Am J Physiol Regul Integr Comp Physiol; 2004; 287 (5):R1054-63 2004 Jul 8 PMID:15242828

FAQ

Are the buffers in the Ni-NTA Fast Start Kit the same as the ones for use with Ni-NTA purchased separately?

The buffers of the Ni-NTA Fast Start Kit are based on recipes for the respective buffers for purification of 6xHis-tagged proteins under native or denaturing conditions listed in the QIAexpressionist handbook. Specific components have been added for optimized performance. The exact composition of the buffers in the Ni-NTA Fast Start Kit is confidential. However, the buffers listed in the Appendix Section of the QIAexpressionist are compatible with the Ni-NTA Fast Start Kit, and can also be used.

FAQ ID -791
What is the composition of PBS?

The composition of PBS is:

  • 50 mM potassium phosphate
  • 150 mM NaCl; pH 7.2

PBS solution is not a component of any QIAGEN kit, but is used in protocols for recombinant protein purification with the QIAexpress System, and in some protocols for DNA and RNA isolation with various QIAGEN Kits.

 

FAQ ID -361
How can I remove imidazole from a protein sample?
Imidazole does not interfere with most downstream applications and therefore does not need to be removed. If it is necessary to remove the imidazole (e.g., for some sensitive enzyme assays), it can be easily achieved by dialysis, precipitation (e.g., ammonium sulfate), or ultrafiltration.
FAQ ID -91
How can I increase expression of my 6xHis-tagged protein in E. coli?

Low-level expression can occur because the protein is toxic or unstable, or because the expression construct is not maintained in the cells during growth. In some cases, the 5' end of the inserted DNA sequence may encode elements that interfere with transcription or translation (e.g., masking of the Shine-Dalgarno sequence by stem-loop structures resulting from inverted repeats). In these instances, the sequence being expressed should be checked and modified if necessary. Modifications of growth media and different host strains may also have an effect on expression.

Please review the section "Specific considerations" in the Chapter 'Expression in E. coli' of the QIAexpressionist Handbook and refer to standard literature in protein science (e.g., Current Protocols in Protein Science, eds. John Wiley and Sons, New York) for additional information.

FAQ ID -63
What are the features and benefits of the QIAexpress 6xHis Tag System?

FEATURES BENEFITS
The interaction of the 6xHis tag with Ni-NTA matrices is conformation independent One-step purification can be carried out under native or denaturing conditions
Mild elution conditions can be used Binding, washing, and elution are highly reproducible, and have no effect on protein structure. Pure protein products are ready for direct use in downstream applications
The 6xHis tag is much smaller than other commonly used tags 6xHis tags can be used in any expression system. The Tag does not interfere with the structure and function of the recombinant protein
The 6xHis tag is uncharged at physiological pH The 6xHis tag does not interfere with secretion
The 6xHis tag is poorly immunogenic The recombinant protein can be used without prior removal of the tag as an antigen to generate antibodies against the protein of interest
Using Factor Xa Protease, 6xHis tag can be easily and efficiently removed The detagged protein can be used for crystallographical or NMR studies where removal of the 6xHis tag may be preferred
Some QIAexpress vectors feature a 6xHis-dihydrofolate reductase tag (6xHis-DHFR tag) Small peptides fused to the 6xHis DHFR tag are stabilized while being expressed. The 6xHis-DHFR tag is not highly immunogenic in mouse and rat, so that peptides fused to the tag can be used directly for immunizations or epitope mapping

 

FAQ ID -193
Can I use HEPES buffer instead of phosphate in my Ni-NTA column?
Although we do not strongly recommend it, up to 100 mM has been successfully used in some cases. Buffers that contain secondary or tertiary amines will reduce nickel ions and affect binding of 6xHis tagged proteins to the Ni-NTA resin.
FAQ ID -291
How does imidazole affect my quantitation of protein?

Since imidazole absorbs UV radiation at 280 nm, an elution profile measured at 280 nm while purifying a 6xHis tagged protein by FPLC will show an increase in absorbance above the background signal allowing quantitation of your protein. The absorbance of imidazole can vary depending on its source and purity, but elution buffer containing 250 mM imidazole usually has an A280 of 0.2–0.4.

To quantitate proteins in eluates containing imidazole, we recommend the Bradford protein assay, which is based on the ability of Coomassie Brilliant Blue R250 to form strong complexes with proteins. This assay is more tolerant of higher imidazole concentrations than the Lowry and the biuret assay, which are more sensitive to imidazole because they involve the reduction of copper. For accurate measurements, always use elution buffer without protein as the reagent blank.

FAQ ID -132
What are the most commonly used protease inhibitors?

The most commonly used protease inhibitors and their working concentrations are included in the table below:

Protease inhibitor Inhibits Suggested working concentration Stock solution (200x)
PMSF* Serine proteases and cysteine proteases such as papain 85 µg/ml (0.5 mM) 17 mg/ml (200 mM) in ethanol or isopropanol
Leupeptin Serine and thiol proteases 0.5 µg/ml (1 µM) 0.1 mg/ml (200 µM) in water
Pepstatin Aspartic proteases 0.7 µg/ml (1 µM) 0.14 mg/ml (200 µM) in ethanol
Aprotinin Serine proteases 1 µg/ml (0.15 µM) 0.2 mg/ml (30 µM) in water
Pefabloc® Serine proteases 0.5 mg/ml (2 mM) 100 mg/ml (400 mM) in water
Na2-EDTA Metalloproteases 0.35 mg/ml (0.75 mM) 70 mg/ml (150 mM) in water, pH 8.0

* PMSF is inactivated in aqueous solutions and should be added to buffers immediately before use. The half-life of an aqueous solution of PMSF is around 30 minutes at pH 8.

All these protease inhibitors are normally prepared as stock solutions and stored in aliquots at –20°C. Stock solutions are usually stable for up to six months. In addition, ready-to-use mixtures of protease inhibitors are available. Complete Protease Inhibitor Cocktail Tablets (Roche Molecular Biochemicals) are available in an EDTA-free formulation and are recommended for use during the purification of 6xHis-tagged proteins under native conditions.

FAQ ID -53
Which primers can I use for sequencing pQE-expression vector constructs?
All pQE vectors (except pQE-TriSystem) can be sequenced using any of the primers described on page 118 of the QIAexpressionist.
FAQ ID -343
What is the difference between Ni-NTA Agarose and Ni-NTA Superflow?

The binding capacity of both resins is the same: up to 50mg/ ml mg 6xHis-tagged protein per ml of resin (2500 nmol @ ~20 kDa). The difference between them is the bead support, which determines pressure resistance and flow rate:

Ni-NTA Agarose:

  • Sepharose CL-6B (bead size 45–165 µm)
  • max. volumetric: 0.5–1.0 ml/min
  • max. pressure: 2.8 psi/(0.2bar)
  • for use with gravity flow only

Ni-NTA Superflow:

  • Superflow (bead size 60–160 µm)
  • max. volumetric: 20 ml/min
  • max. pressure: 140 psi/(10bar)
  • for use with gravity flow or FPLC

You can find a detailed comparison table in the Appendix at the back of the QIAexpressionist Handbook under the title 'Ni-NTA Matrices'.

FAQ ID -764
How can I increase the amount of soluble recombinant protein in E. coli expression?

The QIAexpress Protein Purification System allows easy solubilization of 6xHis-tagged proteins sequestered into insoluble inclusion bodies by using denaturants such as 6 M Guanidine-HCl or 8 M Urea, or a variety of detergents. Proteins purified under denaturing conditions can then be refolded if necessary before use (please see: Wingfield, P. T., Palmer, I., and Liang, S.-M. (1995). Folding and purification of insoluble (inclusion-body) proteins from Escherichia coli. In: Current Protocols in Protein Science, vol. 1, Coligan, J. E., Dunn, B. M., Ploegh, H. L., Speicher, D. W., and Wingfield, P.T. eds. Wiley and Sons, Inc. New York, pp. 6.5.1–6.5.27.). The QIAexpressionist also contains recommendations for refolding proteins prior to the Appendix section of the handbook.

To increase levels of soluble protein, here are a few recommendations:

  • a reduction in growth temperature following induction may be helpful. Growth temperature often directly affects both expression levels and protein solubility, and lower temperatures will reduce expression levels leading to a higher amount of soluble protein.
  • the culture can be grown to a higher cell density before induction and the expression period can be kept to a minimum.
  • The IPTG concentration can be reduced from 1 mM to 0.005 mM, which would reduce the expression level by 90–95%.
  • it may be sufficient to change the host strain used, since certain strains tolerate some proteins better than others and allow higher levels of expression before forming inclusion bodies.
  • many proteins require metal cofactors in order to remain soluble, and the addition of metal salts to the culture media may be helpful. If the metal requirements of the protein are not known, a number of different supplements should be tested. Note that some divalent cations may interfere with protein binding to Ni-NTA.

 

 

FAQ ID -64
What is the origin of replication and the plasmid copy number of the pQE vectors?
The QIAexpress pQE vectors contain a pBR322 derived ColE1 origin of replication and are classified as low-copy plasmids (by our estimate, approximately 20-30 copies per cell; exact numbers have not been determined). The pQE-TriSystem Vector has a pUC origin of replication and is classified as a high-copy vector. Please see also FAQ 350 for general information on replication origins and copy numbers of various commonly used plasmids.
FAQ ID -338
How do I prepare an insert for pQE vectors?

In general, it is only necessary to prepare the insert by restriction digestion and gel purification. The fragment can be ligated into the vector directly. If there is no appropriate restriction site, if it is desirable to minimize the number of extra codons, or if the construct must be optimized in some other way, more complicated manipulations may be necessary. The ends of coding fragments can be modified by PCR, by in vitro mutagenesis, or by the addition of linkers. Please refer to standard laboratory manuals for details on such procedures.

If the 6xHis tag needs to be integrated into other vectors, please follow the recommendations in the 'Cloning' chapter of the QIAexpressionist handbook, section "Integration of 6xHis tags in other vectors".

FAQ ID -185
How can I improve the expression of proteins containing hydrophobic regions?
The addition of either 1% Octylglycoside or 1% Dodecylmaltoside to the lysate might help to solubilize proteins containing large hydrophobic regions. The detergents should be added directly to the reaction mix.
FAQ ID -339
How can I eliminate contaminating protein in my Ni-NTA 6xHis-tag protein purification?
  • Use 10-20 mM imidazole in the lysis and wash buffers (both for native and denaturing conditions). Optimal imidazole concentrations have to be determined empirically.
  • Increase the NaCl concentration (up to 2 M) in the purification buffers to reduce the binding of contaminants as a result of nonspecific ionic interactions.
  • Add ß-mercaptoethanol (up to 20 mM) to the lysis buffer to prevent copurification of host proteins that may have formed disulfide bonds with the protein of interest during cell lysis.
  • Add detergents such as Triton X-100 and Tween 20 (up to 2%), or additives such as glycerol (up to 50%) or ethanol (up to 20%) to reduce nonspecific binding to the matrix due to nonspecific hydrophobic interactions.
  • Reduce the amount of Ni-NTA matrix. Low-affinity binding of background proteins will be reduced by matching the total binding capacity of Ni-NTA matrix with the expected amount of 6xHis-tagged protein.
FAQ ID -102
Why do you recommend using Triton X for the purification of 6xHis-tagged protein?

Nonionic detergents such as Triton X-100 (0.1 - 1%) and Tween 20 (up to 2%) can be used to reduce non-specific binding of contaminating proteins due to non-specific hydrophobic or ionic interactions. They will have no effect on the binding of 6xHis-tagged protein to the Ni-NTA resin when used within the recommended concentration range.

Optimal concentrations for these additives to binding and wash buffers should be determined empirically for each purification protocol and protein.

-100
How can I be sure that I am harvesting my induced bacterial culture at the best time point for protein expression?

To optimize the expression of a given recombinant protein, a time-course analysis of the level of protein expression in the induced culture is recommended. Intracellular protein content is often a balance between the amount of soluble protein in the cells, the formation of inclusion bodies, and protein degradation. By checking the 6xHis-tagged protein present at various times after induction in the soluble and insoluble fractions, the optimal induction period can be established, and the bacterial culture can be harvested at this time. It may be useful to perform plasmid Mini preparations on culture samples during the time-course to enable monitoring of plasmid (expression construct) maintenance.

Below, you can see an example of a time course of recombinant protein expression using the QIAexpress System. You can find this information also in the Section 'Expression in E. coli' in the QIAexpressionist Handbook. The handbook is an important resource for useful background information and protocols. For instructions on how to isolate protein from the soluble and insoluble fractions of induced cultures please see Protocol 14. "Protein minipreps of 6x His-tagged proteins from E. coli under native conditions" and Protocol 19. "6xHis-tagged protein minipreps under denaturing conditions."

 

 

 

Time course of expression using the QIAexpress System. Expression of 6xHis-tagged DHFR was induced with 1 mM IPTG. Aliquots were removed at the times indicated and purified on Ni-NTA Agarose under denaturing conditions. Proteins were visualized by Coomassie staining. Yields per liter culture were 2.8, 5.5,12.3, 33.8, and 53.9 mg, respectively. ■A Crude cell lysate; ■B purification with Ni-NTA. 1: flow-through, 2 & 3: first and second eluates; M: markers; C: noninduced control.

 

 

FAQ ID -788