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TNT? T7 Coupled Wheat Germ Extract System

TNT? T7 Coupled Wheat Germ Extract System

产品编号：L4140 品牌：promega 原厂货号：L4140
产品分类：蛋白质表达与纯化 > 蛋白质表达系统 > 无细胞表达系统
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包装：

40 reactions

运保温度:

到货周期：

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其它组分：

TnT® Wheat Germ Extract【子货号：L411A，包装：5 x 200μl，，运保温度：-70℃】

Amino Acid Mixture Minus Cysteine【子货号：L447C，包装：1 x 50μl，，运保温度：-70℃】

Luciferase Assay Wells【子货号：L457A，包装：1 x 3 each，，运保温度：室温】

TnT® Reaction Buffer【子货号：L462A，包装：1 x 90μl，，运保温度：-70℃】

T7 Linear Control DNA【子货号：P141A，包装：1 x 10μl，，运保温度：-70℃】

Luciferase Assay Reagent【子货号：L486A，包装：1 x 250μl，，运保温度：-70℃】

TnT® T7 Wheat Germ Polymerase【子货号：L516A，包装：1 x 60μl，，运保温度：–20°C】

Amino Acid Mixture Minus Leucine【子货号：L995A，包装：1 x 50μl，，运保温度：-70℃】

Amino Acid Mixture Minus Methionine【子货号：L996A，包装：1 x 50μl，，运保温度：-70℃】

描述：

说明

T_NT^® Coupled Wheat Germ Extract System (T_NT^® 麦胚提取物转录/ 翻译偶联系统) 为研究者提供了一个可应用于真核生物的无细胞蛋白表达方法，它是一个转录/ 翻译偶联的、在一个试管中即可完成实验的系统。T_NT^®提取物系统大大简化了体外翻译过程，缩短了获得翻译结果所需的时间。使用麦胚提取物进行体外翻译的常规方法一般采用由SP6、T3 或T7 RNA 聚合酶启动子在体外合成的RNA作模板，整个过程包括多个独立的反应，且每个反应之间有好几个步骤。T_NT^®提取物系统将转录反应的组分直接整合到翻译反应中，形成混合物，避开了常规方法的繁琐步骤。此外，与使用RNA 模板的常规麦胚提取物体外翻译系统相比，T_NT^® 提取物系统可在1.5 小时内生产出更多的蛋白 (2-6 倍)。

在T_NT^® T7 Quick Coupled Transcription/Translation System、Flexi^® Rabbit Reticulocyte Lysate System 和T_NT^® Coupled Wheat Germ Extract System 中，可以使用25mM 醋酸镁和2.5M 氯化钾对体外翻译反应进行优化。

特点

• 可靠：T_NT^®系统经过严格的质量控制，无论您的模板是线性的DNA( 仅限T3 或T7)，还是环状质粒，都能确保得到高水平的转录/ 翻译性能。

• 方便：单管操作避免了常规小麦胚芽翻译所需要制备RNA 的时间和精力，可在6-8 小时内看到由放射自显影得到的翻译结果。

• 通用性：T7 和T3 系统既可从线性DNA 也可以从环状DNA 生产蛋白质( 环状DNA 仅用于SP6 系统，如果模板是PCR 产物，则使用Cat.# L5540，T_NT^® T7Quick for PCR DNA)。

• 包含对照：系统中包括了萤光素酶对照DNA 和萤光素酶检测试剂，可用作功能对照。只有全长的萤光素酶基因才有活性。

原厂资料：

The TnT® Coupled Wheat Germ Extract Systems offer researchers an alternative for eukaryotic cell-free protein expression: a one-tube, coupled transcription/translation system. The TnT® Extract Systems greatly simplify the process and reduce the time required to obtain in vitro translation results. Standard wheat germ extract translations commonly use RNA synthesized in vitro from SP6 or T7 RNA polymerase promoters. This entire process requires separate reactions with several steps between each reaction. The TnT® Extracts bypass many of these steps by incorporating transcription directly in the translation mix. Additionally, the TnT® Extract reactions often produce significantly more protein (two- to sixfold) in a 1.5-hour reaction than do standard in vitro wheat germ extract translations using RNA templates.

Magnesium Acetate, 25mM, and Potassium Chloride, 2.5M, can be used to optimize in vitro translation reactions in the TnT® T7 Quick Coupled Transcription/Translation System, Flexi® Rabbit Reticulocyte Lysate System and TnT® Coupled Wheat Germ Extract System.

Features - Benefits

Reliable: The TnT® Systems are rigorously quality controlled to ensure the highest level of transcription/translation, whether your template is a linear (T7 only) or circular plasmid.
Convenient: Single-tube procedure eliminates the time and effort required to prepare RNA for a standard wheat germ translation. Translation results can be visualized by autoradiography in 6–8 hours.
Versatile: The T7 system will produce protein from linear DNA. The SP6 system will produce protein from circular DNA. For PCR templates use TnT® T7 Quick for PCR DNA (Cat.# L5540).
Controls Included: Luciferase Control DNA and Luciferase Assay Reagents are included with the system as functional controls. Only full-length luciferase is active.

Applications

Study protein:protein interactions.
Protein activity studies.
The Wheat Germ Extract System is particularly suited to translation of mammalian transcription factors, since it does not contain mammalian transcription factors.
Protein:nucleic acid interactions.
Simultaneously express multiple genes that are under the control of different phage polymerase promoters.
Rapid screening and analysis of mutants.
Protein Truncation Test (PTT).

For more information, see the Protein Expression chapter of the Protocols & Applications Guide.

References

Anderson, C.W. et al. (1983) Meth. Enzymol. 101, 635–44.
Krieg, P.A. and Melton, D.A. (1984) Nucl. Acids Res. 12, 7057–70.