Transfection into Mouse/Rat Testis, Ovary, Prostate, Gonad, and Uterus by Electroporation

Transfection into Mouse/Rat Testis, Ovary, Prostate, Gonad, and Uterus by Electroporation

APPLICATIONS

Electroporated Transgene-Rescued Spermatogenesis in Infertile Mutant Mice with a Sertoli Cell Defect

 

Stereomicroscopic views of transfected testes charged with various voltages and observed under visible (A) or excitation (B) light after 5 wk.

 

Voltage is indicated on each testis (A). 
Loss of testicular weight 5 wk after electric charge in 12-day-old testes (C). 
All values are means  SD (measured number of testes charged with 0, 10, 15, 20, 25, 30, 40, and 50 V are 4, 4, 4, 12, 12, 15, 10, and 12, respectively).

Cross-sections of a testis at 5 wk after being charged with 50 V, observed with fluorescence microscope under excitation light (D, left), followed by counterstaining of the same section with hematoxylin (D, right) or another section just stained with hematoxylin (E).

 

In higher voltage charged testes, luminal enlargement of seminiferous tubules (D) or complete degeneration of seminiferous tubules under the capsule (D, left) was observed. In these testes, many fluorescence-positive Sertoli cells were identified easily (E, right), like in 20V charged testes (Day 35).

Bars = 2mm (A, B) or 100μm (D, E).

 

Kentaro Yomogida, School of Human Environmental Sciences, Mukogawa Women’s University
*BIOLOGY of REPRODUCTION, Volume 67, Issue 3, Pages 712-717, September 2002

PUBLICATIONS

Electroporation

Drug Delivery and Transfection

Electro Cell Fusion

Fluorescent Staining

Single-Cell/Micro-Particle Transfer

Cell Freezing

Mechanical Vibration