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Titlebook: Lentivirus Gene Engineering Protocols; Maurizio Federico Book 20031st edition Humana Press 2003

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Cardiomyocytes in cardiomyocytes. They can be useful for gene reporter studies, but are of little value when a gene needs to be introduced into a large number of cardiac cells. Therefore, viral vectors are used to achieve this goal. Type 5 adenoviruses work well in cardiomyocytes, but they are hard to produce, an
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Airway Epitheliais transmembrane conductance regulator gene (CFTR) that lead to abnormal secretions, recurrent infection and inflammation, bronchiectasis, and premature death. Because airways disease is the major cause of morbidity and mortality in cystic fibrosis, gene therapy efforts have focused on luminal deliv
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Corneal Cellsnsduction of the cornea is useful for studying the efficacy of gene products on inhibition of corneal neovascularization (.), amelioration of corneal inflammatory disease, or promotion of corneal wound healing in animal models. Ex vivo transduction can also be used for transfer of genes into corneal
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Retinal Tissueof inherited retinal degenerations (.). Retinal degenerative disorders are highly heterogeneous, both genetically and phenotypically (.). Different mutations within a single gene (such as rhodopsin) can not only result in different modes of inheritance (autosomal dominant as well as recessive) of th
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The Choice of a Suitable Lentivirus Vector of HIV structural and regulatory sequences in both the transfer and the packaging constructs and have virtually abolished the safety concerns originally raised by the idea of transducing human cells with a derivative of HIV (reviewed in ..). These vectors are now a very promising alternative to tra
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Small- to Large-Scale Production of Lentivirus Vectorsent cotransfection of COS-7 cells with this .-deleted vector and a gp160 expression vector resulted in packaging of the defective HIV-gpt genome into infectious virions. Upon infection of susceptible cells, the . drug resistance gene was transmitted and expressed, allowing transduced cells to be sel
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Detection and Titration of Lentivirus Vector Preparations be conducted based on the number of vector particles added per target cell and will therefore be standardized yielding more reproducible results. The numerical relationship between vector particles utilized per single target cell is designated as the multiplicity of infection (MOI). Establishing an
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