In Vivo Gene Transfer to Mouse Spermatogenic Cells by Deoxyribonucleic Acid Injection into Seminiferous Tubules and Subsequent Electroporation1

Yamazaki, Yukiko; Fujimoto, Hirokazu; Ando, Hironori; Ohyama, Takashi; Hirota, Yoshiko; Noce, Toshiaki

doi:10.1095/biolreprod59.6.1439

Cited by 91 publications

(71 citation statements)

References 27 publications

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“…Its advantages, compared with other nonviral gene delivery systems, are that gene expression is drastically increased (2-to 4-log fold), longlasting (months), and very specific and localized . This technique has also been successful in various tissues such as skeletal muscle (Muramatsu et al, 1998;Aihara and Miyazaki, 1999;Gehl and Mir, 1999;Imai and Isaka, 1999;Mathiesen, 1999;Rizzuto et al, 1999;Bettan et al, 2000;Lemieux et al, 2000;Maruyama et al, 2000;Vicat et al, 2000;Lucas and Heller, 2001;Muramatsu et al, 2001), liver (Suzuki et al, 1998;Heller et al, 2000), testis (Muramatsu et al, 1997;Yamazaki et al, 1998;Yamazaki et al, 2000), skin (Johnson et al, 1998;Vanbever and Preat, 1999;Glasspool-Malone et al, 2000), cornea (Oshima et al, 1998;Sakamoto et al, 1999), cardiaovascular (Harrison et al, 1998;Martin et al, 2000) and mammary tumor tissue Wells et al, 2000;Lohr et al, 2001). In particular, gene delivery to skeletal muscle is a promising strategy for the systemic secretion of therapeutic proteins.…”

Section: Introductionmentioning

confidence: 99%

Optimal salt concentration of vehicle for plasmid DNA enhances gene transfer mediated by electroporation

Lee

Cho²,

Jang³

et al. 2002

Exp Mol Med

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In vivo electroporation has emerged as a leading technology for developing nonviral gene therapies, and the various technical parameters governing electroporation efficiency have been optimized by both theoretical and experimental analysis. However, most electroporation parameters focused on the electric conditions and the preferred vehicle for plasmid DNA injections has been normal saline. We hypothesized that salts in vehicle for plasmid DNA must affect the efficiency of DNA transfer because cations would alter ionic atmosphere, ionic strength, and conductivity of their medium. Here, we show that half saline (71 mM) is an optimal vehicle for in vivo electroporation of naked DNA in skeletal muscle. With various salt concentrations, two reporter genes, luciferase and β β β β-galactosidase were injected intramuscularly under our optimal electric condition (125 V/cm, 4 pulses x 2 times, 50 ms, 1 Hz). Exact salt concentrations of DNA vehicle were measured by the inductively coupled plasma-atomic emission spectrometer (ICP-AES) and the conductivity change in the tissue induced by the salt in the medium was measured by Low-Frequency (LF) Impedance Analyzer. Luciferase expression increased as cation concentration of vehicle decreased and this result can be visualized by X-Gal staining. However, at lower salt concentration, transfection efficiency was diminished because the hypoosmotic stress and electrical injury by low conductivity induced myofiber damage. At optimal salt concentration (71 mM), we observed a 3-fold average increase in luciferase expression in comparison with the normal saline condition (p < 0.01). These results provide a valuable experimental parameter for in vivo gene therapy mediated by electroporation.

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Section: Introductionmentioning

confidence: 99%

Optimal salt concentration of vehicle for plasmid DNA enhances gene transfer mediated by electroporation

Lee

Cho²,

Jang³

et al. 2002

Exp Mol Med

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“…Furthermore, genetic modification of Sertoli cells could be used to correct defective Sertoli cells, thus providing a method to treat those cases of male infertility that might be the results of defects in Sertoli cell function. However, although germ cells can be transfected by using several methods (15)(16)(17), there is currently no technique that allows long-term, widespread transgene expression in Sertoli cells (16,18). Adenoviruses have potential as gene therapy vectors in human patients because of their relatively high cloning capacity and amenability to production in high titers (19).…”

mentioning

confidence: 99%

Adenovirus-mediated gene delivery and in vitro microinsemination produce offspring from infertile male mice

Kanatsu-Shinohara

Ogura²,

Ikegawa³

et al. 2002

Proc. Natl. Acad. Sci. U.S.A.

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Sertoli cells play a pivotal role in spermatogenesis through their interactions with germ cells. To set up a strategy for treating male infertility caused by Sertoli cell dysfunction, we developed a Sertoli cell gene transfer system by using an adenovirus vector, which maintained long-term transgene expression in the testes of infertile mice. Introduction of an adenovirus carrying the mouse Steel (Sl) gene into Sertoli cells restored partial spermatogenesis in infertile Steel͞Steel dickie (Sl͞Sl d ) mutant mouse testes. Although these males remained infertile, round spermatids and spermatozoa from the testes produced normal fertile offspring after intracytoplasmic injection into oocytes. None of the offspring showed evidence of germ line transmission of adenoviral DNA. Thus, we demonstrate a successful treatment for infertility by using a gene therapy vector. Therefore, adenovirus-mediated gene delivery into Sertoli cells not only provides an efficient and convenient means for studying germ cell-Sertoli cell interactions through manipulation of the germ cell microenvironment in vivo, but also is a useful method to treat male infertility resulting from a Sertoli cell defect.

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“…As a possible alternative and more effective method for generating transgenic mice, several researchers have attempted testis-mediated gene transfer using an in vivo electroporation method. After injection of exogenous DNA into the testis, the testes are held between a tweezer-type electrode, and square electric pulses are applied several times at 20-50 volts (Muramatsu, 1996(Muramatsu, , 1997Yamazaki, 1998Yamazaki, , 2000Umemoto, 2002. Expression of the exogenous gene was clearly observed in germ cells of seminiferous tubules 48 hours after transfecting the mouse testis by in vivo electroporation (Muramatsu, 1997).…”

Section: Electroporationmentioning

confidence: 99%

Therapeutic Potential of Gene Transfer to Testis; Myth or Reality?

Kojima¹,

Mizuno²,

Umemoto³

et al. 2011

Gene Therapy Applications

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In Vivo Gene Transfer to Mouse Spermatogenic Cells by Deoxyribonucleic Acid Injection into Seminiferous Tubules and Subsequent Electroporation1

Cited by 91 publications

References 27 publications

Optimal salt concentration of vehicle for plasmid DNA enhances gene transfer mediated by electroporation

Optimal salt concentration of vehicle for plasmid DNA enhances gene transfer mediated by electroporation

Adenovirus-mediated gene delivery and in vitro microinsemination produce offspring from infertile male mice

Therapeutic Potential of Gene Transfer to Testis; Myth or Reality?

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