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pGL4.33[luc2P/SRE/Hygro]

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  • 产品名称:pGL4.33[luc2P/SRE/Hygro]
  • 产品型号:
  • 产品展商:HZbscience
  • 产品文档:无相关文档
  • 发布时间:2017-07-17
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简单介绍
pGL4.33[luc2P/SRE/Hygro]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pGL4.33[luc2P/SRE/Hygro]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

pGL4.33[luc2P/SRE/Hygro]载体基本信息

载体名称: pGL4.33 ; pGL4.33[luc2P/SRE/Hygro]
质粒类型: 信号通路报告载体;哺乳动物载体;萤火虫荧光素酶报告载体
高拷贝/低拷贝: --
克隆方法: 限制性内切酶,多克隆位点
启动子: Minimal Promotor
载体大小: 6112 bp
5' 测序引物及序列: --
3' 测序引物及序列: --
载体标签: luc2P
载体抗性: 氨苄青霉素
筛选标记: 潮霉素(Hygromycin)
克隆菌株: TOP10等常规菌株
宿主细胞(系): HEK293等
备注: pGL4.33[luc2P]载体是信号通路报告载体;含SRE应答元件;含萤火 虫荧光素酶报告基因luc2P。
产品目录号: E134A
稳定性: 稳表达
组成型/诱导型: 组成型
病毒/非病毒: 非病毒

pGL4.33[luc2P/SRE/Hygro]载体质粒图谱和多克隆位点信息

pGL4.33载体图谱



pGL4.33 载体特征

pGL4.33[luc2P/SRE/Hygro]载体简介

The pGL4.33[luc2P/SRE/Hygro] Vector(a–c) contains a Serum Response Element (SRE) that drives transcription of the luciferase reporter gene luc2P in response to activation of MAPK/ERK signaling pathway. luc2P is a synthetically derived luciferase sequence with humanized codon optimization. The luc2P gene also contains hPEST, a protein destabilization sequence. The protein encoded by luc2P responds more quickly to induction than the protein encoded by the luc2 gene. The vector backbone contains an ampicillin resistance gene to allow selection in E. coli and the mammalian selectable marker for hygromycin resistance.


Sample Protocol to Determine Induction of Luciferase by FBS + PMA in HEK293 Cells Transfected with the pGL4.33[luc2P/SRE/Hygro] Vector

实验材料
 Dulbecco's PBS (DPBS)
 0.05% (w/v) trypsin in DPBS
 DMEM
 DMEM supplemented with 0.5%, 10% and 40% fetal bovine serum (DMEM/FBS)
 Phorbol 12-myristate 13-acetate (PMA, Promega Cat.# V1171 or Sigma Cat.# P8139),
1mg/ml solution in DMSO
 ONE-Glo Luciferase Assay System (Cat.# E6110)
 HEK293 cells
 transfection reagent

Day 1: Plate Cells
1. Grow HEK293 cells in DMEM/FBS to approximately 75% confluency.
2. Harvest cells via trypsinization: Remove the DMEM/FBS, wash the cells with DPBS
and add the trypsin/DPBS (1X volume). After 2 minutes, add a 4X volume of
DMEM/FBS, collect the cell suspension and pellet the cells by centrifugation.
Aspirate the supernatant, and resuspend in DMEM/FBS. We have routinely used a
concentration of 10,000–15,000 viable cells/100μl DMEM/FBS.
3. Dispense 100μl of the cell suspension into the wells of a 96-well plate. Plate enough
wells to perform each test condition in triplicate.
4. Cover the plate, and place it in a tissue culture incubator at 37°C overnight (or for 24 hours).

Day 2: Transfect Cells
1. Transfect the cells using a high-efficiency transfection reagent. Each well of cells in a 96-well plate requires 0.1μg pGL4.33[luc2P/SRE/Hygro] Vector DNA. Transfection conditions may require optimization.
2. Cover the plate, and place it in a tissue culture incubator at 37°C.
3. After 4–6 hours, change the medium to DMEM/0.5%FBS (100μl per well) to start
serum starvation.

Day 3: Induce Transfected Cells
1. Prepare 2X induction and 2X control solutions. Calculate the volume of 2X induction
and 2X control solution by multiplying the number of wells needed for each solution
by 50μl, and prepare 110% of this amount.
 2X induction solution: 40%FBS plus 20ng/ml PMA in DMEM
 2X control solution: DMEM
2. Remove 50μl of medium from wells that will be treated with either 2X induction solution or 2X control solution.
3. Add 50μl of 2X induction solution to the cells to be induced and 50μl of 2X control
solution to the control noninduced cells.
4. Return the plate to the tissue culture incubator, and induce for 6 hours.
5. Analyze luciferase activity using an appropriate luciferase detection assay. We have
observed comparable results for fold induction of the vector using a variety of
luciferase reagents, including: Bright-Glo Luciferase Assay System (Cat.# E2610,
Technical Manual #TM052); ONE-Glo Luciferase Assay System (Cat.# E6110,
Technical Manual #TM292); Dual-Luciferase Reporter Assay System (Cat.# E1910,
Technical Manual #TM040); and Dual-Glo Luciferase Assay System (Cat.# E2920,
Technical Manual #TM058).
6. Calculate the fold induction as follows:
fold induction = average relative light units of induced cells
average relative light units of control cells

pGL4.33[luc2P/SRE/Hygro]载体序列

hz-6348R PIWIL3  piwi样3蛋白抗体
hz-6349R VGF/Nerve growth factor inducible  神经生长因子诱导蛋白抗体
hz-6350R pan methyl Lysine  泛甲基赖氨酸抗体
hz-6351R DAP1  死亡相关蛋白1抗体
hz-6352R Adenylosuccinate Lyase  腺苷酸琥珀酸裂解酶抗体
hz-6353R HIPK2  Fas相互作用蛋白激酶2抗体
hz-6359R Glutamine PRPP amidotransferase  谷氨酰胺磷酸核糖基焦磷酸酰胺基转移酶
hz-6365R CROT/COT  过氧化物酶体肉碱酰基转移酶抗体
hz-6369R PAICS  磷酸核糖胺咪唑羧化酶抗体
hz-6370R p70 S6 kinase alpha  磷酸化核糖体p70 S6蛋白激酶抗体
hz-6371R Protamine 2  鱼精蛋白2抗体
hz-6372R Hepcidin-25  铁调节蛋白25抗体
hz-6373R CGR19  细胞生长调控蛋白19抗体(环指蛋白197)
hz-6374R FPR3/Lipoxin A4 receptor  甲酰肽受体3抗体(脂氧素A4受体)
hz-6375R CHMP1A  染色体修饰蛋白1抗体(金属蛋白酶1)
hz-6376R DDIT4L  DNA损伤诱导转录样蛋白4抗体
hz-6377R DEAF1/Deformed Epidermal Autoregulatory Factor 1  畸形表皮自调节因子1抗体
hz-6378R EID3  E1A样分化抑制因子3抗体
hz-6380R ERCC6L  发育相关蛋白ERCC6L抗体(乙醇致畸因子)
hz-6381R FAM107A  肾细胞癌下调蛋白1抗体
hz-6382R FRK/PTK5  胃肠道相关酪氨酸激酶抗体(蛋白酪氨酸激酶5)
hz-6383R GANP  **中心相关核蛋白MCM3抗体

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