Canine Pancreatic Microsomal Membranes

产品编号：Y4041 品牌：promega 原厂货号：Y4041
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
应用分类：

包装：

50μl

运保温度:

–70°C

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其它组分：

Signal Sequence Control mRNA【子货号：Y406B，包装：1 x 5μg，，运保温度：–70°C】

Glycosylation Control mRNA【子货号：Y407C，包装：1 x 1μg，，运保温度：–70°C】

Canine Microsomal Membranes【子货号：Y408A，包装：1 x 50μl，，运保温度：–70°C】

描述：

说明

微粒体囊泡被用于研究蛋白质的协同翻译和翻译后加工的初始过程。在微粒体膜存在的情况下，可通过合适的mRNA 在体外翻译来检验蛋白加工程序，这些程序包括信号肽剪切、膜插入、移位和核心糖基化。另外，也可以用Canine Pancreatic Microsomal Membranes ( 犬胰微粒体膜) 结合T_NT^®Lysate Systems(T_NT^® 裂解物系统) 对合适的DNA 模板进行转录/ 翻译反应，从而研究加工和糖基化过程。为了性能稳定、翻译反应中的抑制作用最小、本底最低，制备微粒体时去除了污染的膜片段以及内源性的、结合在膜上的核糖体和mRNA。使用两种不同的对照mRNA 模板，对膜制备物的信号肽酶和核心糖基化活性进行了检测。这两种对照mRNA 是E. coli的β- 内酰胺酶( 或氨苄青霉素抗性基因产物) 前体，以及啤酒酵母(S.cerevisiae ) 的α- 配合因子( 或α- 因子基因产物) 前体。

从含有编码大肠杆菌β- 内酰胺酶( 氨苄青霉素抗性基因产物)前体的基因序列的质粒上，使用SP6 RNA 聚合酶可转录得到对照信号序列mRNA( 大肠杆菌β- 内酰胺酶)。合成的RNA不含有帽类似物。该对照mRNA 用于检测信号肽酶活性，并与Canine Pancreatic Microsomal Membranes System 一起提供。

从含有啤酒酵母(S. cerevisiae )α- 配合因子(a-mating factor) 编码区的质粒上，使用SP6 RNA 聚合酶可转录得到Core Glycosylation Control mRNA (S. cerevisiae a-factor)( 对照核心糖基化mRNA( 啤酒酵母的α- 因子))。合成的RNA 不具有类似帽子结构，该对照mRNA 用于检测核心糖基化活性，并与Canine Pancreatic Microsomal Membranes System 一起提供。

特点

. 可靠：制备微粒体时去除了内源性的、结合在膜上的核糖体和mRNA，以确保微粒体膜的性能稳定，且对翻译反应的抑制作用最小、本底最低，并已使用兔网织红细胞裂解物系统检测过。

原厂资料：

Microsomal vesicles are used to study co-translational and initial post-translational processing of proteins. Processing events such as signal peptide cleavage, membrane insertion, translocation and core glycosylation can be examined by the translation of the appropriate mRNA in vitro in the presence of these microsomal membranes. In addition, processing and glycosylation events may be studied by the transcription/translation of the appropriate DNA in the TnT® Lysate Systems when used with Canine Pancreatic Microsomal Membranes. To assure consistent performance with minimal translational inhibition and background, microsomes have been isolated free from contaminating membrane fractions and stripped of endogenous membrane-bound ribosomes and mRNA. Membrane preparations are assayed for both signal peptidase and core glycosylation activities using two different control mRNAs. The two control mRNAs supplied with this system are the precursor for β-lactamase (or ampicillin resistance gene product) from E. coli and the precursor for α-mating factor (or α-factor gene product) from S. cerevisiae.
The Signal Sequence Control mRNA (E. coli β-lactamase) is transcribed by SP6 RNA polymerase from a plasmid bearing the coding region for the E. coli gene encoding the precursor to β-lactamase (the ampicillin resistance gene product). The RNA is synthesized without a cap analog. This control mRNA is used to assay for signal peptidase activity and is supplied with the Canine Pancreatic Microsomal Membranes System.
The Core Glycosylation Control mRNA (S. cerevisiae α-factor) is transcribed by SP6 RNA polymerase from a plasmid bearing the coding region for the S. cerevisiae α-mating factor. The RNA is synthesized without a cap analog. This control mRNA is used to assay for core glycosylation activity and is supplied with the Canine Pancreatic Microsomal Membranes System.

Features - Benefits

Reliable: Microsomes are stripped of endogenous membrane-bound ribosomes and mRNA to ensure consistent performance with minimal translational inhibition and background. Performance tested in rabbit reticulocyte lysate.

Applications

Examination of signal peptide cleavage, membrane insertion, translocation and core glycosylation.
Compatible with the TnT® Lysate Systems, Rabbit Reticulocyte Lysate, and Flexi® Lysate.
For more information, see the Protein Expression chapter of the Protocols & Applications Guide.

References

Walter, P. and Blobel, G. (1983) Meth. Enzymol. 96, 84–93.