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          pRevTet-On 說明書

          發(fā)布時間:2013/7/23      點擊次數(shù):4125

          四環(huán)素調(diào)控系統(tǒng) pRevTet-On

          pRevTet-On

          型號 載體名稱 出品公司 載體用途
          VSC0469 pRevTet-On Clontech 四環(huán)素調(diào)控系統(tǒng)

           

          Description:

          pRevTet-On is a retroviral vector expressing the reverse tetracycline-controlled transactivator 

          (rtTA) from the CMV promoter. This vector is derived from pLNCX, a retroviral vector created 

          using elements of Moloney murine leukemia virus (MoMuLV) and Moloney murine sarcoma 

          virus (MoMuSV) as described (1). rtTA is a fusion of amino acids 1–207 of the reverse tet 

          repressor (rTetR) and the negatively charged C-terminal activation domain (130 amino acids) 

          of the VP16 protein of Herpes Simplex Virus. rTetR was derived from TetR and differs by four 

          point mutations, which are responsible for its opposite response to doxycycline. The 5' viral 

          LTR controls expression of the transcript that contains Ψ+

           (the extended viral packaging signal) 

          and the neomycin resistance gene (Neor

          ) for antibiotic selection in mammalian cells. rtTA is 

          derived from vectors described previously (2–4). pRevTet-On also includes the E. coli Ampr

          gene for antibiotic selection in bacteria.

          Use:

          pRevTet-On can be used to establish stable Tet-On cell lines via retrovirus-mediated gene 

          transfer (5). Retroviral gene transfer allows the highly efficient transduction of virtually all 

          dividing cell types. The RevTet Systems are also suitable for establishing transgenic animals. In 

          combination with the pRev-TRE retroviral expression vector, a gene of interest can be inducibly 

          expressed at high levels in response to varying concentrations of the tetracycline derivative 

          doxycycline (Dox). rtTA binds to the Tet-response element (TRE), thus activating transcription in the presence of Dox. The response of rtTA to Dox is thus opposite to the response of 

          tTA. As Dox is removed from the culture medium, transcription from the inducible promoter 

          is turned off in a highly dose-dependent manner. pRevTet-On lacks the viral genes gag, pol, 

          and env, which are supplied by the packaging cell line. It can be transfected into a high titer 

          packaging cell line and thereby mediate production of infectious, replication-incompetent 

          retroviral particles (1, 6–7).The transcript produced by the pRevTet-On construct is recognized 

          by the viral structural proteins expressed in a packaging cell line and packaged into infectious 

          retroviral particles. Because the RNA transcript packaged in these particles does not contain 

          the viral genes, it cannot replicate in the target cells that it infects. 

          The level of induction in cell populations infected with this vector depends on the efficiency 

          of infection, the site of integration, and the titer of the virus. Viral supernatants with titers >105

          cfu/ml should be produced to achieve high-level induction.

           

          質(zhì)粒圖譜: 
          pRevTet-On 質(zhì)粒圖譜

           

           


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