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產(chǎn)品資料

pcDNA5/FRT/V5-His-TOPO

如果您對該產(chǎn)品感興趣的話,可以
產(chǎn)品名稱: pcDNA5/FRT/V5-His-TOPO
產(chǎn)品型號:
產(chǎn)品展商: HZbscience
產(chǎn)品文檔: 無相關(guān)文檔

簡單介紹

pcDNA5/FRT/V5-His-TOPO的各批次質(zhì)粒菌株發(fā)貨前均經(jīng)過嚴格的多重驗證,如存在質(zhì)量問題,請在收到產(chǎn)品的三個月內(nèi)通知我司。收到pcDNA5/FRT/V5-His-TOPO后請短暫離心,取2μl轉(zhuǎn)化至對應感受態(tài)中,挑取單克隆重新提取質(zhì)粒后使用。


pcDNA5/FRT/V5-His-TOPO  的詳細介紹

pcDNA5/FRT/V5-His-TOPO載體基本信息

載體名稱: pcDNA5/FRT/V5-His-TOPO
質(zhì)粒類型: 哺乳動物細胞表達載體;cDNA表達載體;定向重組載體
高拷貝/低拷貝: 高拷貝
克隆方法: TOPO-TA
啟動子: CMV
載體大小: 5094 bp
5' 測序引物及序列: T7 Forward: 5’-TAATACGACTCACTATAGGG-3’
3' 測序引物及序列: BGH Reverse: 5’-TAGAAGGCACAGTCGAGG-3’
載體標簽: V5 Epitope(C-端);His tag(C-端)
載體抗性: 氨芐青霉素
篩選標記: 潮霉素(Hygromycin)
克隆菌株: TOP10, DH5α, JM109
宿主細胞(系): Invitrogen公司出品的Flp-In細胞系,293、CV-1、CHO、BHK等
備注: pcDNA5/FRT/V5-His-TOPO載體是cDNA的表達與克隆載體;
CMV啟動子驅(qū)動目的基因的過表達;
含有FRT位點(重組酶識別位點),與pOG44載體共轉(zhuǎn)染,利用重組酶進行定向重組;
采用TOPO-TA技術(shù),只用5分鐘即可將PCR片段連接到載體上去;
產(chǎn)品目錄號: K6020-01
穩(wěn)定性: 瞬表達 或 穩(wěn)表達
組成型/誘導型: 組成型
病毒/非病毒: 非病毒

pcDNA5/FRT/V5-His-TOPO載體質(zhì)粒圖譜和多克隆位點信息

pcDNA5-FRT-V5-His-TOPO載體圖譜



pcDNA5-FRT-V5-His-TOPO特征位點



pcDNA5-FRT-V5-His-TOPO 多克隆位點

pcDNA5-FRT-V5-His-TOPO 載體特征1
pcDNA5-FRT-V5-His-TOPO 載體特征2

pcDNA5/FRT/V5-His-TOPO載體簡介

pcDNA5/FRT/V5-His-TOPO 載體 pcDNA5/FRT/V5-His-TOPOis a 5.1 kb expression vector designed to facilitate rapid cloning and expression of PCR products using the Flp-InSystem (Catalog nos. K6010- 01 and K6010-02) available from Invitrogen. When cotransfected with the pOG44 Flp recombinase expression plasmid into a Flp-Inmammalian host cell line, the pcDNA5/FRT/V5-His-TOPOvector containing the PCR product of interest is integrated in a Flp recombinase-dependent manner into the genome. 

The pcDNA5/FRT/V5-His TOPOTA Expression Kit combines the Flp-InSystem with TOPOCloning technology to provide a highly efficient, rapid cloning strategy for the direct insertion of Taq polymerase-amplified PCR products into a plasmid vector for targeted expression of the gene of interest in mammalian cell lines. TOPO Cloning
requires no ligase, post-PCR procedures, or PCR primers containing special, additional sequences. pcDNA5/FRT/V5-His-TOPO載體含有以下元件: The human cytomegalovirus (CMV) immediate-early enhancer/promoter for highlevel constitutive expression of the gene of interest in a wide range of mammalian cells (Andersson et al., 1989; Boshart et al., 1985; Nelson et al., 1987)
TOPOCloning site for rapid and efficient cloning of Taq-amplified PCR products
C-terminal peptide containing the V5 epitope and a polyhistidine (6xHis) tag for detection and purification of recombinant protein
FLP Recombination Target (FRT) site for Flp recombinase-mediated integration of the vector into the Flp-Inhost cell line 
Hygromycin resistance gene for selection of stable cell lines (Gritz and Davies, 1983)

The control plasmid, pcDNA5/FRT/V5-His/CAT, is included for use as a positive control for transfection and expression in the Flp-In host cell line of choice.
For more information about the Flp-In System, the pOG44 plasmid, and generation of the Flp-In host cell line, refer to the Flp-In System manual. The Flp-In System manual is supplied with the Flp-In Complete or Core Systems, but is also available for downloading from our World Wide Web site or by contacting Technical Service Flp 重組酶介導的DNA重組 In the Flp-In System, integration of your pcDNA5/FRT/V5-His-TOPO expression construct into the genome occurs via Flp recombinase-mediated intermolecular DNA recombination. The hallmarks of Flp-mediated recombination are listed below.
 Recombination occurs between specific FRT sites on the interacting DNA molecules
 Recombination is conservative and requires no DNA synthesis; the FRT sites are preserved following recombination and there is minimal opportunity for introduction of mutations at the recombination site
 Strand exchange requires only the small 34 bp minimal FRT site FRT 位點 The FRT site, originally isolated from Saccharomyces cerevisiae, serves as a binding site for Flp recombinase and has been well-characterized (Gronostajski and Sadowski, 1985;Jayaram, 1985; Sauer, 1994; Senecoff et al., 1985). The minimal FRT site consists of a 34bp sequence containing two 13 bp imperfect inverted repeats separated by an 8 bp spacer that includes an Xba I restriction site. An additional 13 bp repeat is found in most FRT sites, but is not required for cleavage (Andrews et al., 1985). While Flp recombinase binds to all three of the 13 bp repeats, strand cleavage actually occurs at the boundaries of the 8 bp spacer region (Andrews et al., 1985; Senecoff et al., 1985).

upstream of the hygromycin resistance gene for Flp recombinase-mediated integration and selection of the pcDNA5/FRT/V5-His-TOPO construct following cotransfection of the vector (with pOG44) into a Flp-In mammalian host cell line. The FRT site serves as both the recognition and cleavage site for the Flp recombinase and allows recombination to occur immediately adjacent to the hygromycin resistance gene. The Flp recombinase is expressed from the pOG44 plasmid. For more information about the FRT site and recombination, see the next page. For more information about pOG44, refer to the pOG44 manual or the Flp-In System manual.

The hygromycin resistance gene in pcDNA5/FRT/V5-His-TOPO lacks a promoter and an ATG initiation codon; therefore, transfection of the pcDNA5/FRT/V5-His-TOPO plasmid alone into mammalian host cells will not confer hygromycin resistance to the cells. The SV40 promoter and ATG initiation codon required for expression of the hygromycin resistance gene are integrated into the genome (in the Flp-In host cell line) and are only brought into the correct proximity and frame with the hygromycin resistance gene through Flp recombinase-mediated integration of pcDNA5/FRT/V5-His-TOPO at the FRT site. For more information about the generation of the Flp-In host cell line and details of the Flp-In System, refer to the Flp-In System manual. TOPO克隆原理 The plasmid vector, pcDNA5/FRT/V5-His-TOPO, is supplied linearized with:
 Single 3′ thymidine (T) overhangs for TA Cloning
 Topoisomerase covalently bound to the vector (this is referred to as “activated” vector) Taq polymerase has a nontemplate-dependent terminal transferase activity that adds a single deoxyadenosine (A) to the 3′ ends of PCR products. The linearized vector supplied in this kit has single, overhanging 3′ deoxythymidine (T) residues. This allows PCR inserts to ligate efficiently with the vector.
Topoisomerase I from Vaccinia virus binds to duplex DNA at specific sites and cleaves the phosphodiester backbone after 5′-CCCTT in one strand (Shuman, 1991). The energy from the broken phosphodiester backbone is conserved by formation of a covalent bond between the 3′ phosphate of the cleaved strand and a tyrosyl residue (Tyr-274) of topoisomerase I.The phospho-tyrosyl bond between the DNA and enzyme can subsequently be attacked by the 5′ hydroxyl of the original cleaved strand, reversing the reaction and releasing topoisomerase (Shuman, 1994). TOPO Cloning exploits this reaction to efficiently clone PCR products. 
TOPO克隆技術(shù)原理



pcDNA5/FRT/V5-His-TOPO載體序列

hz-8194R FAM40A  FAM家族蛋白40A抗體
hz-8195R FAM120B  組織激活過氧化酶活化增生受體γ蛋白抗體
hz-8196R FAM55D  FAM55D蛋白抗體
hz-8197R TAAL6  腫瘤相關(guān)蛋白抗原L6抗體
hz-8198R FAM46C  FAM46C蛋白抗體
hz-8199R FAM168A/TCRP1  舌癌化療耐藥相關(guān)蛋白1
hz-4105R Filamin A/FLNA  細絲蛋白A抗體
hz-8200R phospho-MYF5 (phospho Ser49)  磷酸化生肌決定因子Myf5抗體
hz-0438R AT2R/AT1  血管緊張素Ⅱ受體1抗體
hz-8201R PMCA4B  細胞膜鈣ATP酶4B抗體
hz-8202R BRN4/POU3F4  腦轉(zhuǎn)錄因子4蛋白抗體
hz-5350R phospho-Filamin A/FLNA (Ser2151)  磷酸化細絲蛋白A抗體
hz-5351R phospho-Filamin A/FLNA (Ser2522)  磷酸化細絲蛋白A抗體
hz-1707R Angiotensin I/Angiotensinogen  血管緊張素I抗體
hz-0587R Angiotensin II  血管緊張素Ⅱ抗體
hz-8204R NEEP21  NEEP21蛋白抗體
hz-5354R phospho-Filamin A/FLNA (Tyr1046)  磷酸化細絲蛋白A抗體
hz-3877R Angiotensin III  血管緊張素III抗體
hz-8205R FAM129B  FAM129B蛋白抗體
hz-8206R FAM82A1/RMD2  微管動力調(diào)節(jié)蛋白2抗體

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