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      Long-Term Expression of Human Clotting Factor IX from Retrovirally Transduced Primary Human Keratinocytes In Vivo

      , , ,
      Human Gene Therapy
      Mary Ann Liebert Inc

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          Living tissue formed in vitro and accepted as skin-equivalent tissue of full thickness.

          Living skin-equivalent grafts consisting of fibroblasts cast in collagen lattices and seeded with epidermal cells were successfully grafted onto the donors of the cells. The grafts were vascularized, did not evoke a homograft reaction, inhibited wound contraction, filled the wound space, and persisted.
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            Redesign of retrovirus packaging cell lines to avoid recombination leading to helper virus production.

            Retrovirus vectors can be made in the absence of helper virus by using retrovirus packaging cell lines. Helper-free virus is critical for a variety of gene transfer studies. The most useful packaging cell lines contain helper virus DNA from which the signal required for packaging of the viral RNA genome into virions has been deleted. However, we showed that the ability to package virus is conferred at very low frequency to cells infected with virus from these packaging cell lines, presumably by low-frequency transmission of the deleted virus genome. In addition, these packaging cell lines can interact with some retroviral vectors to yield replication-competent virus. We constructed packaging cell lines containing helper virus DNA that had several alterations in addition to deletion of the packaging signal. The new packaging cells retained the useful features of previously available lines but did not yield helper virus after introduction of any of the vectors tested, and transfer of the packaging function was not detected.
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              Clonal analysis of stably transduced human epidermal stem cells in culture.

              We have transduced normal human keratinocytes with retroviral constructs expressing a bacterial beta-galactosidase (beta-gal) gene or a human interleukin-6 (hIL-6) cDNA under control of a long terminal repeat. Efficiency of gene transfer averaged approximately 50% and 95% of clonogenic keratinocytes for beta-gal and hIL-6, respectively. Both genes were stably integrated and expressed for more than 150 generations. Clonal analysis showed that both holoclones and their transient amplifying progeny expressed the transgene permanently. Southern blot analysis on isolated clones showed that many keratinocyte stem cells integrated multiple proviral copies in their genome and that the synthesis of the exogenous gene product in vitro was proportional to the number of proviral integrations. When cohesive epidermal sheets prepared from stem cells transduced with hIL-6 were grafted on athymic animals, the serum levels of hIL-6 were strictly proportional to the rate of secretion in vitro and therefore to the number of proviral integrations. The possibility of specifying the level of transgene expression and its permanence in a homogeneous clone of stem cell origin opens new perspectives in the long-term treatment of genetic disorders.
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                Author and article information

                Journal
                Human Gene Therapy
                Human Gene Therapy
                Mary Ann Liebert Inc
                1043-0342
                1557-7422
                May 20 1998
                May 20 1998
                : 9
                : 8
                : 1187-1195
                Article
                10.1089/hum.1998.9.8-1187
                019485c2-e3c8-4107-841b-2696a554a90e
                © 1998

                http://www.liebertpub.com/nv/resources-tools/text-and-data-mining-policy/121/

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