• 商品货号：FH1739

• 规格：10μl质粒
• 原核抗性：氨苄青霉素Amp
• 筛选标记：荧光素酶Luc
• 克隆菌株：大肠杆菌DH5α
• 质粒简介：         pE2F-TA-Luc单荧光素酶信号通路报告质粒。pE2F-TA-Luc is designed to monitor the induction of E2F-mediated signal transduction pathways. E2F, a major target of the retinoblastoma gene (Rb), is a key regulator of cell-cycle checkpoints in mammalian cells . E2F plays a critical role in stimulating expression of genes encoding growth-promoting proteins, and is involved in regulating the expression of important genes during cell proliferation . The E2F protein forms a heterodimer complex with the DP1 protein, which binds to E2F response elements and initiates transcription of genes necessary for DNA replication. Studies have shown that deregulation of E2F results in a loss of cell-cycle checkpoints—thereby predisposing cells to uncontrolled growth . pE2F-TA-Luc contains four copies of the E2F enhancer element (6), located upstream of the minimal TA promoter, the TATA box from the herpes simplex virus thymidine kinase promoter (PTA). Located downstream of PTA is the firefly luciferase reporter gene (luc). Upon binding of the E2F/DP1 complex to the cis-acting E2F enhancer element, transcription is induced and the reporter gene is activated. The luciferase coding sequence is followed by the SV40 late polyadenylation signal to ensure proper, efficient processing of the luciferase transcript in eukaryotic cells. A synthetic transcription blocker (TB) is located upstream of the cis-acting enhancer element. It is composed of adjacent polyadenylation and transcription pause sites for blocking nonspecific transcription (7). The vector backbone also contains an f1 origin for single-stranded DNA production, a pUC origin of replication, and an ampicillin resistance gene for propagation and selection in E. coli. 
          pE2F-TA-Luc is designed for monitoring cell-cycle signaling in mammalian cells by assaying for luciferase activity. For example, induction of E2F-mediated signal transduction pathways may be compared across different cell types or cell states by transiently transfecting this vector into appropriate cell lines. After transfection, treat each culture individually with a drug candidate or stimulus of interest, then compare the activation of the E2F response element by assaying for the luciferase reporter gene. Additionally, you can monitor pathway activation by cotransfecting this vector with an expression vector containing a gene of interest. Luciferase is a highly sensitive enzymatic reporter that can be assayed by any standard luciferase-detection method, providing quantitative data on induction levels. pE2F-TA-Luc can be transfected into mammalian cells by any standard method. For selecting stable clones, cotransfect with a vector containing an antibiotic resistance gene, such as neomycin, hygromycin, or puromycin, and selecting resistant clones.
• 质粒图谱1： png/1-1G220145919D9.png

质粒序列： 点击查看序列

测序所得的部分序列
ORIGIN

        1 acatttctct atcgataggt accgagctct tacgcgtgct agccttggcg ggagatagaa

       61 cttggcggga gataggaact tggcgggaga taggaacttg gcgggagata ggaaagatct

      121 agactctaga gggtatataa tggaagctcg aattccagct tggcattccg gtactgttgg

      181 taaaaagctt ggcattccgg tactgttggt aaagccacca tggaagacgc caaaaacata

      241 aagaaaggcc cggcgccatt ctatccgctg gaagatggaa ccgctggaga gcaactgcat

      301 aaggctatga agagatacgc cctggttcct ggaacaattg cttttacaga tgcacatatc

      361 gaggtggaca tcacttacgc tgagtacttc gaaatgtccg ttcggttggc agaagctatg

      421 aaacgatatg ggctgaatac aaatcacaga atcgtcgtat gcagtgaaaa ctctcttcaa

      481 ttctttatgc cggtgttggg cgcgttattt atcggagttg cagttgcgcc cgcgaacgac

      541 atttataatg aacgtgaatt gctcaacagt atgggcattt cgcagcctac cgtggtgttc

      601 gtttccaaaa aggggttgca aaaaattttg aacgtgcaaa aaaagctccc aatcatccaa

      661 aaaattatta tcatggattc taaaacggat taccagggat ttcagtcgat gtacacgttc

      721 gtcacatctc atctacctcc cggttttaat gaatacgatt ttgtgccaga gtccttcgat

      781 agggacaaga caattgcact gatcatgaac tcctctggat ctactggtct gcctaaaggt

      841 gtcgctctgc ctcatagaac tgcctgcgtg agattctcgc atgccagaga tcctattttt

      901 ggcaatcaaa tcattccgga tactgcgatt ttaagtgttg ttccattcca tcacggtttt

      961 ggaatgttta ctacactcgg atatttgata tgtggatttc gagtcgtctt aatgtataga

     1021 tttgaagaag agctgtttct gaggagcctt cagattacag gattcaaagt gcgctgctgg

     1081 tgcaacccta attctcttct cgcaaagcac tctgatgaca atcgagttta tctaaattta

     1141 acacgaatgg cttctgggtg ccgctcccct ctttaggagt cgggaggcga ttgccaagag

     1201 tcaatctgcc aggcatcagg gcaagagaat attgggcatc gctgtcgaag gacatacact

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