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pcDNA4/HisMax B

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  • 产品名称:pcDNA4/HisMax B
  • 产品型号:
  • 产品展商:HZbscience
  • 产品文档:无相关文档
  • 发布时间:2017-07-18
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简单介绍
pcDNA4/HisMax B的各批次质粒菌株发货前均经过严格的多重验证,如存在质量问题,请在收到产品的三个月内通知我司。收到pcDNA4/HisMax B后请短暂离心,取2μl转化至对应感受态中,挑取单克隆重新提取质粒后使用。
产品描述

pcDNA4/HisMax B载体基本信息

载体名称: pcDNA4/HisMax B
质粒类型: 哺乳动物表达载体;cDNA表达载体
高拷贝/低拷贝: 高拷贝
克隆方法: 多克隆位点,限制性内切酶
启动子: CMV
载体大小: 5259 bp
5' 测序引物及序列: T7 Forward: 5’-TAATACGACTCACTATAGGG-3’
3' 测序引物及序列: BGH Reverse: 5-TAGAAGGCACAGTCGAGG-3
载体标签: His Tag (N-端), Xpress Epitope Tag(N-端)
载体抗性: 氨苄青霉素
筛选标记: Zeocin
克隆菌株: TOP10F′, DH5a
宿主细胞(系): 常规细胞系,如293、Hela等
备注: pcDNA4/HisMax B 载体是哺乳动物表达载体,适用于cDNA的表达与克隆;
QBI SP163增强子,使得目的基因的高水平表达提高了3~5倍;
pcDNA4/HisMax A,B,C的区别仅在于多克隆位点处;
含EK (Enterokinase)切割位点
产品目录号: V864-20
稳定性: 瞬表达 或 稳表达
组成型/诱导型: 组成型
病毒/非病毒: 非病毒

pcDNA4/HisMax B载体质粒图谱和多克隆位点信息

pcDNA4-HisMax B载体图谱



pcDNA4-HisMax B 多克隆位点

pcDNA4-HisMax 载体特征1
pcDNA4-HisMax 载体特征2

pcDNA4/HisMax B载体简介

pcDNA4/HisMax A, B, and C载体介绍:

pcDNA4/HisMax is specifically designed to maximize protein expression in a variety of mammalian cells. The vector contains the QBI SP163 translational enhancer to increase expression levels two- to five-fold above those seen with the promoter alone . In addition to SP163-enhanced expression, pcDNA4/HisMax includes a cleavable N-terminal Xpress tag for rapid detection of recombinant protein with an Anti-Xpress Antibody. pcDNA4/HisMax is available TOPO Cloning-ready for five-minute cloning of Taqamplified PCR products.

pcDNA4/HisMax A, B, and C are 5.3 kb vectors derived from pcDNA4/His and designed for overproduction of recombinant proteins in mammalian cell lines. Features of the vectors allow purification and detection of expressed proteins. High-level stable and transient expression can be carried out in most mammalian cells. The vectors contain the following elements:
 Human cytomegalovirus immediate-early (CMV) promoter for high-level expression in a wide range of mammalian cells
 QBI SP163 translational enhancer for increased levels of recombinant protein expression (Stein et al., 1998) (see page 4 for more information)
 Three reading frames to facilitate in-frame cloning with an N-terminal peptide encoding the Xpress epitope and a polyhistidine metal-binding tag
 Zeocin resistance gene for selection of stable cell lines 
 Episomal replication in cell lines that are latently infected with SV40 or that express the SV40 large T antigen (e.g. COS-1, COS-7)
The control plasmid, pcDNA4/HisMax/lacZ, is included for use as a positive control for transfection, expression, and detection in the cell line of choice.

实验流程:

Use the following outline to clone and express your gene of interest in pcDNA4/HisMax.
 Consult the multiple cloning sites described on pages 5-7 to determine which vector (A, B, or C) should be used to clone your gene in frame with the N-terminal Xpress epitope and the polyhistidine tag.
 Ligate your insert into the appropriate vector and transform into E. coli. Select transformants on 50 to 100 μg/ml ampicillin or 25-50 μg/ml Zeocin.
 Analyze your transformants for the presence of insert by restriction digestion.
 Select a transformant with the correct restriction pattern and use sequencing to confirm that your gene is cloned in frame with the N-terminal peptide.
 Transfect your construct into the cell line of choice using your own method of transfection. Generate a stable cell line, if desired.
 Test for expression of your recombinant gene by western blot analysis or functional assay. .
 To purify your recombinant protein, you may use metal-chelating resin such as ProBond. ProBond resin is available separately.

表达目的基因:

We have a wide variety of mammalian expression vectors utilizing the CMV or EF-1α promoter. Vectors are available with the Xpress (N-terminal), c-myc (C-terminal), or V5 (C-terminal) epitope for detection and either the neomycin, blasticidin, or Zeocin resistance genes. All vectors utilize the polyhistidine tag for purification using ProBond resin. 

The pcDNA4/HisMax vectors are fusion vectors. To ensure proper expression of your recombinant protein, you must clone your gene in frame with the ATG at base pairs 1080-1082. This will create a fusion with the N-terminal polyhistidine tag, Xpress epitope, and the enterokinase cleavage site. The vector is supplied with the multiple cloning site in three reading frames relative to the N-terminal peptide to facilitate cloning.

If you wish to clone your gene as close as possible to the enterokinase cleavage site, follow the guidelines below:
 Digest pcDNA4/HisMax A, B, or C with Kpn I.
 Create blunt ends with T4 DNA polymerase and dNTPs.
 Clone your blunt-ended insert in frame with the lysine codon (AAG) of the enterokinase recognition site.

pcDNA4/HisMax B载体序列

hz-9316R NDE1  核分布基因E同源蛋白1抗体
hz-9317R NEK9  丝氨酸/苏氨酸蛋白激酶NEK9抗体
hz-9318R phospho-NEK9(Thr210)  磷酸化丝氨酸/苏氨酸蛋白激酶NEK9抗体
hz-9319R NNF1R/PMF1  多胺调控因子1抗体
hz-9320R NYS48  NYS48蛋白抗体
hz-1546R beta Adaptin/AP2  衔接蛋白β抗体
hz-9321R PRPF4  PRPF4蛋白抗体
hz-9322R RanBP1  RAN结合蛋白1抗体
hz-9323R RanBP2  RAN结合蛋白2/核孔蛋白抗体
hz-9325R ASZ1  锚定蛋白样蛋白1抗体
hz-9326R GDAP2  神经节苷脂诱导分化相关蛋白2抗体
hz-9327R LRCH1  富含亮氨酸重复家庭蛋白1抗体
hz-9328R LRCH2  富含亮氨酸重复家庭蛋白2抗体
hz-9329R LRCH3  富含亮氨酸重复家庭蛋白3抗体
hz-9330R LRCH4  富含亮氨酸重复家庭蛋白4抗体
hz-1600R Gamma-Adaptin/γ-Adaptin  衔接蛋白γ抗体
hz-9331R NHLRC1  肌痉挛性癫痫病相关EPM2蛋白抗体
hz-9332R NHLRC2  非霍奇金**瘤重复蛋白2抗体
hz-9333R NHLRC3  非霍奇金**瘤重复蛋白3抗体
hz-9334R RanBP3  RAN结合蛋白3抗体
hz-9335R MARCH1  膜相关环指蛋白1抗体
hz-9336R MARCH2  膜相关环指蛋白2抗体
hz-9337R MARCH3  膜相关环指蛋白3抗体

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