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pHT01枯草胞内质粒

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基本信息

别名:

pHT-01

启动子:

Pgrac

复制子:

pUC

质粒分类:

广宿主系列,枯草杆菌载体

质粒大小:

7956bp

原核抗性:

Amp

真核抗性:

Chl

克隆菌株:

DH5a

培养条件:

37度

表达宿主:

枯草芽孢杆菌

诱导方式:

IPTG诱导

5'测序引物:

根据序列设计引物

3'测序引物:

根据序列设计引物

备注:

枯草杆菌IPTG诱导胞内表达空载体


质粒属性

质粒宿主:

枯草杆菌

质粒用途:

蛋白表达

片段类型:

ORF

片段物种:

空载体

原核抗性:

Amp

真核抗性:


荧光标记:



质粒简介

All vectors use the strong promoter preceding the groESL operon of Bacillus subtilis fused to the lac operator allowing their induction by addition of IPTG. While the background level of expression of these expression cassettes is very low in the absence of the inducer, an induction factor of about 1,300 was measured using the bgaB reporter gene. The amount of recombinant protein produced after addition of IPTG may represent 10 and 13%, respectively, of the total cellular protein. High level secretion of amyQ α-amylase and cellulase A and B of Clostridium thermocellum was demonstrated. An efficient Shine-Dalgarno sequence as well as a multiple cloning site (BamH I, Xba I, AatII, SmaI) were also inserted. To obtain secretion of recombinant proteins, the coding region for the signal peptide of the amyQ gene encoding an α-amylase was fused to the SD sequence of pHT01, thereby constructing pHT43.

大肠杆菌-枯草芽孢杆菌穿梭质粒的表达载体pHT01可以在枯草芽孢杆菌中高效表达重组外源蛋白。载体基于强σA-依赖性启动子的枯草杆菌groE操纵子,通过添加lac操纵子改造成为一种高效可控的(IPTG诱导的)启动子。


质粒图谱

image.png

质粒序列

质粒序列请下载:

pHT01枯草胞内质粒.txt


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