載體名稱:	pFLAG-CMV-3
質(zhì)粒類型:	哺乳動(dòng)物表達(dá)載體；分泌表達(dá)載體
高拷貝/低拷貝:	低拷貝
克隆方法:	多克隆位點(diǎn)；限制性內(nèi)切酶
啟動(dòng)子:	CMV
載體大小:	6331 bp
5' 測(cè)序引物及序列:	CMV Forward：CGCAAATGGGCGGTAGGCGTG
3' 測(cè)序引物及序列:	hGH-pA-R：CCAGCTTGGTTCCCAATAGA
載體標(biāo)簽:	FLAG tag (N-末端）
載體抗性:	氨芐青霉素
篩選標(biāo)記:	Neomycin
克隆菌株:	--
宿主細(xì)胞（系）:	常用細(xì)胞系，如293、Hela等
備注:	pFLAG-CMV-3載體N端含有信號(hào)肽PPT ，輔助目的蛋白分泌表達(dá)； CMV啟動(dòng)子驅(qū)動(dòng)目的蛋白高水平表達(dá)；FLAG標(biāo)簽含8個(gè)氨基酸殘基（DYKDDDDK），一般位于融合蛋白的外表面，具有高度** 靈敏性，便于檢測(cè)和純化目的蛋白；
產(chǎn)品目錄號(hào):	E6783
穩(wěn)定性:	瞬表達(dá) 或穩(wěn)表達(dá)
組成型/誘導(dǎo)型:	組成型
病毒/非病毒:	非病毒

pFLAG-CMV-3載體質(zhì)粒圖譜和多克隆位點(diǎn)信息

pFLAG-CMV-3 載體圖譜

pFLAG-CMV-3 多克隆位點(diǎn)

pFLAG-CMV-3載體簡(jiǎn)介

FLAG 和 3xFLAG 標(biāo)簽：
A Proven System for Detection and Purification of Proteins The FLAG Expression System is an established way to express, purify and detect recombinant fusion proteins. FLAG and 3xFLAG have proven utility in numerous applications such as Western blotting, immunocytochemistry, immunoprecipitation, flow cytometry, protein purification, and in the study of protein-protein interactions, cell ultrastructure and protein localization. These small hydrophilic tags facilitate superior detection and purification of recombinant fusion proteins when using our highly specific and sensitive ANTI-FLAG antibodies. Ideal Epitope Tags: Small, Hydrophilic and Cleavable The FLAG expression system utilizes a short, hydrophilic 8-amino acid peptide that is fused to the recombinant protein of interest. Because of its hydrophilic nature, the FLAG peptide is likely to be located on the surface of the fusion protein. As a result, the FLAG peptide is easily accessible for cleavage by enterokinase (Ek) and for detection with antibodies. In addition, because of the small size of the FLAG peptide tag, it is not likely to obscure other epitopes, domains, or alter function, secretion, or transport of the fusion protein. The 3xFLAG system is an improvement upon the original system by fusing 3 tandem FLAG epitopes (22 amino acids). Detection of fusion proteins containing 3xFLAG is enhanced up to 200 times more than any other system. Like the original FLAG tag, 3xFLAG is hydrophilic, contains an Ek cleavage site, and is relatively small. Therefore, the risk of altering protein function, blocking other epitopes or decreasing solubility is minimized.

3xFLAG System Expression Vectors for Ultra-Sensitive

重組蛋白的檢測(cè)
The 3xFLAG system is an improvement upon the original system by fusing 3 tandem FLAG epitopes for a total of 22 amino acids. Detection of fusion proteins containing 3xFLAG is enhanced up to 200 times more than any other system. Like the original FLAG tag, 3xFLAG is hydrophilic, contains an Enterokinase cleavage site, and is relatively small. Therefore, the risk of altering protein function, blocking other epitopes or decreasing solubility is minimized. In cases of low-level expression, 3xFLAG is ideal. Our selection of CMV vectors provides options for transient or stable expression of 3xFLAG fusion proteins.

Ultrasensitive System - Detect < 10 femtomoles using ANTI-FLAG Antibodies; Ideal for cases of low-level expression in mammalian cells.
Superior Detection - 20-200x more sensitive than any other system.
Versatile - Enhanced detection for immunoprecipitation, Western blots and immunocytochemistry.
Wide Selection of Detection and Purification Products - ANTI-FLAG antibodies, resins, and affinity capture plates.

Figure 1. 3xFLAG Sequence. Removal of N-terminal 3xFLAG tags is possible using enterokinase, which cleaves following the Asp-Asp-Asp-Asp-Lys amino acid sequence at the c-terminal end of the tag.
Figure 2. Western Blot of Original FLAG Versus 3xFLAG. Western blot of purified 3xFLAG-BAP (bacterial alkaline phosphatase) and FLAG-BAP transferred onto a nitrocellulose membrane. Detection was performed with ANTI-FLAG M2 monoclonal primary antibody, anti-mouse-HRP secondary antibody, and ECL chemiluminescent substrate.
Figure 3. Comparative Sensitivity of 3xFLAG. Each protein fusion tag was cloned separately on the C terminal of GST. The purified proteins were diluted from 1 ug to 0.01 ng and analyzed. The limit of detection of each tag was determined by Western blot analysis using the recommended dilutions of each respective primary antibody and secondary anti-mouse IgG-HRP conjugate. The blot was developed using ECL.

CMV啟動(dòng)子：
Our mammalian expression vectors contain the strong CMV promoter for high-level constitutive expression in mammalian cells. The strong human cytomegalovirus (CMV) promoter regulatory region drives constitutive protein expression levels as high as 1 mg/L in COS cells. For less potent cell lines, protein levels are typically ~0.1 mg/L. The presence of the SV40 replication origin will result in high levels of DNA replication in SV40 replication permissive COS cells. Vectors containing the preprotrypsin leader (PPT) sequence direct secretion of FLAG fusion proteins into the culture medium for purification using ANTI-FLAG antibodies, resins, and plates.

pFLAG-CMV-3載體序列

hz-4171R Angiomotin 血管抑素結(jié)合蛋白抗體
hz-4193R HIP4/CBS 絲氨酸羧甲半胱氨酸合成酶抗體
hz-1004R ACE2 血管緊張素轉(zhuǎn)換酶2抗體
hz-0203R ACEI 血管緊張素1轉(zhuǎn)換酶抑制劑抗體
hz-2745R Acetyl CoA Carboxylase 乙酰輔酶A羧化酶抗體
hz-3036R Phospho-Acetyl CoA Carboxylase(Ser79) 磷酸化乙酰輔酶A羧化酶抗體
hz-1962R ACD 腎上腺皮質(zhì)發(fā)育異常蛋白抗體
hz-2511R ACHE/Acetylcholinesterase 乙酰膽堿酶抗體
hz-0120R Acinus Acinus抗體
hz-3001R phospho-Acinus(Ser1180) 磷酸化腺泡Acinus蛋白抗體
hz-1227R Ack1 醋酸激酶1抗體
hz-3038R Phospho-Ack1(Tyr859/860) 磷酸化Ack1抗體
hz-3045R Phospho-Ack1(Tyr284) 磷酸化Ack1抗體
hz-3046R Phospho-Ack1(Tyr326) 磷酸化Ack1抗體
hz-5022R ACSL1 長(zhǎng)鏈脂肪酸輔酶A連接酶1/2抗體
hz-0443R ACTH (1-39) 促腎上腺皮質(zhì)**(1-39)抗體
hz-3678R Phospho-MKP1 (Ser318) 磷酸化絲裂原活化蛋白激酶磷酸酶1抗體
hz-0442R ACTH (18-39) 促腎上腺皮質(zhì)**ACTH(18-39)抗體
hz-0004R ACTH (7-23) 促腎上腺皮質(zhì)**ACTH (7-23)抗體
hz-0189R Actin α/alpha-SMA 肌動(dòng)蛋白α(α-SMA)抗體
hz-4178R Sarcomeric Alpha Actinin/ACTN2 α橫紋肌輔肌動(dòng)蛋白/α-SCA抗體

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